TY - JOUR A1 - Sarukhanyan, Edita A1 - Shanmugam, Tipack Ayothyapattanam A1 - Dandekar, Thomas T1 - In silico studies reveal Peramivir and Zanamivir as an optimal drug treatment even if H7N9 avian type influenza virus acquires further resistance JF - Molecules N2 - An epidemic of avian type H7N9 influenza virus, which took place in China in 2013, was enhanced by a naturally occurring R294K mutation resistant against Oseltamivir at the catalytic site of the neuraminidase. To cope with such drug-resistant neuraminidase mutations, we applied the molecular docking technique to evaluate the fitness of the available drugs such as Oseltamivir, Zanamivir, Peramivir, Laninamivir, L-Arginine and Benserazide hydrochloride concerning the N9 enzyme with single (R294K, R119K, R372K), double (R119_294K, R119_372K, R294_372K) and triple (R119_294_372K) mutations in the pocket. We found that the drugs Peramivir and Zanamivir score best amongst the studied compounds, demonstrating their high binding potential towards the pockets with the considered mutations. Despite the fact that mutations changed the shape of the pocket and reduced the binding strength for all drugs, Peramivir was the only drug that formed interactions with the key residues at positions 119, 294 and 372 in the pocket of the triple N9 mutant, while Zanamivir demonstrated the lowest RMSD value (0.7 Å) with respect to the reference structure. KW - H7N9 influenza virus KW - neuraminidase KW - mutation KW - binding pocket KW - molecular docking Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-288240 SN - 1420-3049 VL - 27 IS - 18 ER - TY - JOUR A1 - Gupta, Shishir K. A1 - Minocha, Rashmi A1 - Thapa, Prithivi Jung A1 - Srivastava, Mugdha A1 - Dandekar, Thomas T1 - Role of the pangolin in origin of SARS-CoV-2: an evolutionary perspective JF - International Journal of Molecular Sciences N2 - After the recent emergence of SARS-CoV-2 infection, unanswered questions remain related to its evolutionary history, path of transmission or divergence and role of recombination. There is emerging evidence on amino acid substitutions occurring in key residues of the receptor-binding domain of the spike glycoprotein in coronavirus isolates from bat and pangolins. In this article, we summarize our current knowledge on the origin of SARS-CoV-2. We also analyze the host ACE2-interacting residues of the receptor-binding domain of spike glycoprotein in SARS-CoV-2 isolates from bats, and compare it to pangolin SARS-CoV-2 isolates collected from Guangdong province (GD Pangolin-CoV) and Guangxi autonomous regions (GX Pangolin-CoV) of South China. Based on our comparative analysis, we support the view that the Guangdong Pangolins are the intermediate hosts that adapted the SARS-CoV-2 and represented a significant evolutionary link in the path of transmission of SARS-CoV-2 virus. We also discuss the role of intermediate hosts in the origin of Omicron. KW - COVID-19 KW - SARS-CoV-2 KW - origin KW - evolution KW - intermediate host KW - pangolin KW - mutation KW - recombination KW - adaptation KW - transmission KW - comparative sequence analysis Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-285995 SN - 1422-0067 VL - 23 IS - 16 ER - TY - JOUR A1 - Dhillon, Maninder Singh A1 - Dahms, Thorsten A1 - Kübert-Flock, Carina A1 - Steffan-Dewenter, Ingolf A1 - Zhang, Jie A1 - Ullmann, Tobias T1 - Spatiotemporal Fusion Modelling Using STARFM: Examples of Landsat 8 and Sentinel-2 NDVI in Bavaria JF - Remote Sensing N2 - The increasing availability and variety of global satellite products provide a new level of data with different spatial, temporal, and spectral resolutions; however, identifying the most suited resolution for a specific application consumes increasingly more time and computation effort. The region’s cloud coverage additionally influences the choice of the best trade-off between spatial and temporal resolution, and different pixel sizes of remote sensing (RS) data may hinder the accurate monitoring of different land cover (LC) classes such as agriculture, forest, grassland, water, urban, and natural-seminatural. To investigate the importance of RS data for these LC classes, the present study fuses NDVIs of two high spatial resolution data (high pair) (Landsat (30 m, 16 days; L) and Sentinel-2 (10 m, 5–6 days; S), with four low spatial resolution data (low pair) (MOD13Q1 (250 m, 16 days), MCD43A4 (500 m, one day), MOD09GQ (250 m, one-day), and MOD09Q1 (250 m, eight day)) using the spatial and temporal adaptive reflectance fusion model (STARFM), which fills regions’ cloud or shadow gaps without losing spatial information. These eight synthetic NDVI STARFM products (2: high pair multiply 4: low pair) offer a spatial resolution of 10 or 30 m and temporal resolution of 1, 8, or 16 days for the entire state of Bavaria (Germany) in 2019. Due to their higher revisit frequency and more cloud and shadow-free scenes (S = 13, L = 9), Sentinel-2 (overall R\(^2\) = 0.71, and RMSE = 0.11) synthetic NDVI products provide more accurate results than Landsat (overall R\(^2\) = 0.61, and RMSE = 0.13). Likewise, for the agriculture class, synthetic products obtained using Sentinel-2 resulted in higher accuracy than Landsat except for L-MOD13Q1 (R\(^2\) = 0.62, RMSE = 0.11), resulting in similar accuracy preciseness as S-MOD13Q1 (R\(^2\) = 0.68, RMSE = 0.13). Similarly, comparing L-MOD13Q1 (R\(^2\) = 0.60, RMSE = 0.05) and S-MOD13Q1 (R\(^2\) = 0.52, RMSE = 0.09) for the forest class, the former resulted in higher accuracy and precision than the latter. Conclusively, both L-MOD13Q1 and S-MOD13Q1 are suitable for agricultural and forest monitoring; however, the spatial resolution of 30 m and low storage capacity makes L-MOD13Q1 more prominent and faster than that of S-MOD13Q1 with the 10-m spatial resolution. KW - Landsat KW - Sentinel-2 KW - NDVI KW - fusion KW - agriculture KW - grassland KW - forest KW - urban KW - water Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-323471 SN - 2072-4292 VL - 14 IS - 3 ER - TY - THES A1 - Schilcher, Felix T1 - Regulation of the nurse-forager transition in honeybees (\(Apis\) \(mellifera\)) T1 - Regulation des Ammen–Sammlerinnen-Übergangs in Honigbienen (\(Apis\) \(mellifera\)) N2 - Honeybees are among the few animals that rely on eusociality to survive. While the task of queen and drones is only reproduction, all other tasks are accomplished by sterile female worker bees. Different tasks are mostly divided by worker bees of different ages (temporal polyethism). Young honeybees perform tasks inside the hive like cleaning and nursing. Older honeybees work at the periphery of the nest and fulfill tasks like guarding the hive entrance. The oldest honeybees eventually leave the hive to forage for resources until they die. However, uncontrollable circumstances might force the colony to adapt or perish. For example, the introduced Varroa destructor mite or the deformed wing virus might erase a lot of in-hive bees. On the other hand, environmental events might kill a lot of foragers, leaving the colony with no new food intake. Therefore, adaptability of task allocation must be a priority for a honeybee colony. In my dissertation, I employed a wide range of behavioral, molecular biological and analytical techniques to unravel the underlying molecular and physiological mechanisms of the honeybee division of labor, especially in conjunction with honeybee malnourishment. The genes AmOARα1, AmTAR1, Amfor and vitellogenin have long been implied to be important for the transition from in-hive tasks to foraging. I have studied in detail expression of all of these genes during the transition from nursing to foraging to understand how their expression patterns change during this important phase of life. My focus lay on gene expression in the honeybee brain and fat body. I found an increase in the AmOARα1 and the Amforα mRNA expression with the transition from in-hive tasks to foraging and a decrease in expression of the other genes in both tissues. Interestingly, I found the opposite pattern of the AmOARα1 and AmTAR1 mRNA expression in the honeybee fat body during orientation flights. Furthermore, I closely observed juvenile hormone titers and triglyceride levels during this crucial time. Juvenile hormone titers increased with the transition from in-hive tasks to foraging and triglyceride levels decreased. Furthermore, in-hive bees and foragers also differ on a behavioral and physiological level. For example, foragers are more responsive towards light and sucrose. I proposed that modulation via biogenic amines, especially via octopamine and tyramine, can increase or decrease the responsiveness of honeybees. For that purpose, in-hive bees and foragers were injected with both biogenic amines and the receptor response was quantified 1 using electroretinography. In addition, I studied the behavioral response of the bees to light using a phototaxis assay. Injecting octopamine increased the receptor response and tyramine decreased it. Also, both groups of honeybees showed an increased phototactic response when injected with octopamine and a decreased response when injected with tyramine, independent of locomotion. Additionally, nutrition has long been implied to be a driver for division of labor. Undernourished honeybees are known to speed up their transition to foragers, possibly to cope with the missing resources. Furthermore, larval undernourishment has also been implied to speed up the transition from in-hive bees to foragers, due to increasing levels of juvenile hormone titers in adult honeybees after larval starvation. Therefore, I reared honeybees in-vitro to compare the hatched adult bees of starved and overfed larvae to bees reared under the standard in-vitro rearing diet. However, first I had to investigate whether the in-vitro rearing method affects adult honeybees. I showed effects of in-vitro rearing on behavior, with in-vitro reared honeybees foraging earlier and for a shorter time than hive reared honeybees. Yet, nursing behavior was unaffected. Afterwards, I investigated the effects of different larval diets on adult honeybee workers. I found no effects of malnourishment on behavioral or physiological factors besides a difference in weight. Honeybee weight increased with increasing amounts of larval food, but the effect seemed to vanish after a week. These results show the complexity and adaptability of the honeybee division of labor. They show the importance of the biogenic amines octopamine and tyramine and of the corresponding receptors AmOARα1 and AmTAR1 in modulating the transition from inhive bees to foragers. Furthermore, they show that in-vitro rearing has no effects on nursing behavior, but that it speeds up the transition from nursing to foraging, showing strong similarities to effects of larval pollen undernourishment. However, larval malnourishment showed almost no effects on honeybee task allocation or physiology. It seems that larval malnourishment can be easily compensated during the early lifetime of adult honeybees. N2 - Honigbienen gehören zu den wenigen Spezies, die in eusozialen Gemeinschaften leben. Die eierlegende Königin und die männlichen Drohnen dienen nur der Fortpflanzung. Alle anderen Arbeiten von den sterilen Arbeiterinnen ausgeführt werden. Die Arbeitsteilung wird meistens anhand des Alters der Bienen organisiert. Junge Arbeiterinnen bleiben im Inneren der Kolonie und führen beispielsweise Putzarbeiten und Ammentätigkeiten aus. Mit zunehmendem Alter verlagern sich ihre Tätigkeiten immer mehr in Richtung des Nestausgangs wo sie, unteranderem als Wächterbienen, den Stockeingang bewachen. Die ältesten Honigbienen verlassen das Nest, um Honig, Pollen, Wasser oder Propolis zu sammeln, bis sie am Ende sterben. Allerdings können unvorhersehbare Ereignisse dazu führen, dass sich die Kolonie anpassen muss, um nicht unterzugehen. Krankheiten wie der Flügeldeformationsvirus oder die, durch den Menschen eingeführte, Varroa destructor Milbe können auf einen Schlag eine große Zahl an Bienen auslöschen. Des Weiteren können beispielsweise starke Unwetter dafür sorgen, dass etliche Sammlerinnen auf ihrem Sammelflug sterben und die Kolonie ohne neuen Nektar oder Pollen zurückgelassen wird. Es liegt auf der Hand, dass eine starre Arbeitsverteilung nicht ausreicht, um solchen Umständen entgegenzuwirken und, dass eine gewisse Flexibilität notwendig ist. In meiner Dissertation habe ich eine weitreichende Anzahl an verhaltensbiologischen und molekularbiologischen Techniken verwendet, um die molekularen und physiologischen Mechanismen der Arbeitsteilung bei Honigbienen aufzuklären, vor allem im Bezug auf den Übergang von Ammenbienen zu Sammlerinnen. Es ist seit langer Zeit bekannt, dass die Gene AmOARα1, AmTAR1, Amfor und Vitellogenin beim Übergang von Ammenbienen zu Sammlerinnen von zentraler Bedeutung sind. Deshalb habe ich die Expression dieser Gene, sowohl im Gehirn als auch im Fettkörper, in genau diesem Zusammenhang betrachtet und die unterschiedlichen Veränderungen der Expressionsmuster während dieser wichtigen Phase im Leben einer Honigbiene analysiert. Ich konnte zeigen, dass sowohl die mRNA Expression des AmOARα1 und des Amforα beim Übergang von Ammenbienen zu Sammlerinnen anstieg, während die Expression der anderen Kandidatengene im gleichen Zeitraum sowohl im Gehirn als auch im Fettkörper abfiel. Interessanterweise zeigten die Expressionsmuster des AmOARα1 und des Am3 TAR1, während der Orientierungsflüge, genau in die entgegengesetzte Richtung. Zusätzlich habe ich mir bei denselben Bienen auch den Juvenilhormongehalt in der Hämolymphe und die Menge an Triglyceriden im Fettkörper angeschaut. Der Juvenilhormongehalt nahm schlagartig zu, als die Bienen mit dem Sammeln begannen. Die Menge an Triglyceriden nahm allerdings von Ammenbienen, über Bienen während des Orientierungsfluges zu Sammlerinnen konstant ab. Des Weiteren war bereits bekannt, dass sich Ammenbienen und Sammlerinnen nicht nur auf genetischer, sondern auch auf verhaltensbiologischer und physiologischer Ebene voneinander unterscheiden. Zum Beispiel sind Sammlerinnen empfindlicher für Licht und Saccharose. Ich stellte die Hypothese auf, dass die Empfindlichkeit von Honigbienen für solche Schwellen durch biogene Amine, insbesondere Oktopamin und Tyramin, moduliert werden kann. Oktopamin sollte die Empfindlichkeit von Bienen erhöhen, wohingegen Tyramin diese verringern sollte. Hierfür injizierte ich Stockbienen und Sammlerinnen beide biogenen Amine und analysierte die Rezeptorantwort mit einem Elektroretinogramm (ERG) und die Lichtempfindlichkeit in einer Phototaxisarena. Oktopamininjektion führte dazu, dass die Rezeptorantwort im ERG erhöht wurde und dass beide Gruppen eine erhöhte Lichtempfindlichkeit aufwiesen. Tyramin hatte in beiden Experimenten genau den gegenteiligen Effekt. Allerdings kann der Ammen-Sammlerinnen-Übergang nicht nur durch biogene Amine moduliert werden, auch die Ernährung hat einen großen Einfluss. Zum Beispiel fangen unterernährte Honigbienen eher an zu sammeln als satte Honigbienen. Des Weiteren sollte auch die larvale Unterernährung bereits einen Einfluss auf die spätere Arbeitsteilung haben, da man bei Arbeiterinnen, die im Larvenstadium bereits unterernährt waren, eine erhöhte Menge an Juvenilhormon festgestellt hatte. Dies sieht man auch beim Übergang von Ammenbienen zu Sammlerinnen. Deshalb nutzte ich eine Methode zur artifiziellen Aufzucht von Honigbienen, um die Standarddiät, die diese normalerweise erhalten, zu variieren. Allerdings musste ich zuerst den Effekt der in-vitro Aufzucht auf im Stock aufgezogene Honigbienen untersuchen. Ich konnte zeigen, dass die artifizielle Aufzucht das Sammelverhalten erwachsener Honigbienen signifikant beeinflusste, während das Ammenverhalten der in-vitro aufgezogenen Bienen nicht beeinflusst wurde. Artifiziell aufgezogene Honigbienen begannen, im Vergleich zu normalen Bienen, früher zu sammeln und sammelten für eine kürzere Zeit. Danach zog ich unterernährte, normal ernährte und überfütterte Honigbienen in-vitro 4 auf. Ich fand Unterschiede im Gewicht zwischen den Behandlungsgruppen. Unterernährte Bienen waren die leichtesten und überfütterte Bienen wogen am meisten. Dieser Unterschied verschwand aber über die Zeit. Des Weiteren konnte ich keinen Einfluss der Ernährung auf das Ammenverhalten oder das Sammelverhalten zeigen. Dieser Ergebnisse zeigen sowohl die Komplexität als auch das Anpassungsvermögen der Arbeitsteilung von Honigbienen. Sie zeigen, dass sowohl die beiden biogenen Amine Oktopamin und Tyramin, als auch die dazugehörigen Rezeptoren AmOARα1 und AmTAR1 bei der Modulation des Ammen-Sammlerinnen-Übergangs eine große Rolle spielen. Des Weiteren zeigen die Ergebnisse des Vergleichs von artifiziell und im Stock aufgezogenen Bienen, starke Gemeinsamkeiten zu einer larvalen Unterernährung mit Pollen. Jedoch scheint eine allgemeine larvale Unterernährung kaum einen Effekt auf den AmmenSammlerinnen-Übergang zu haben. Diese scheint während der ersten Lebenstage von Honigbienen relativ leicht kompensiert werden zu können. KW - Biene KW - juvenile hormone KW - nurse bee KW - forager KW - division of labor KW - malnourishment KW - diet KW - bee KW - honeybee Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-289352 ER - TY - JOUR A1 - Kortmann, Mareike A1 - Angelstam, Per A1 - Mayer, Marius A1 - Leibl, Franz A1 - Reichert, Jessica A1 - Thorn, Christine A1 - Thorn, Simon T1 - Disturbance severity and human–nature relationships: A new approach to analyze people’s well-being along a bark beetle infestation gradient JF - Forests N2 - Contact to nature and greenspace is important for emotional well-being and can promote human health. Forest landscapes provide such access to greenspace, especially in protected areas. However, forested protected areas are impacted by natural disturbances such as bark beetle infestations. On the one hand, such disturbances have positive impacts on ecological processes and biodiversity. On the other hand, they have allegedly negative impacts on the recreational value of a landscape. Limited knowledge about the public’s perception of forests subject to natural disturbances still hampers forest management to balance ecological functions and visitors’ recreational experience. Thus, our aim was to determine how attitudes towards nature influence the personal well-being in a naturally disturbed landscape. We investigated self-reported well-being and attitudes towards nature in a standardized questionnaire-based survey of 1008 German inhabitants in an experimentally adapted landscape visualization. Self-reported well-being was generally highest in landscapes with relatively few bark-beetle-killed trees. This was especially the case for people who felt included with nature and preferred an appreciative use or preservation of nature. Conversely, people who had previously visited a national park with visible bark beetle infestations rated their personal well-being highest in landscapes with larger proportions of beetle-killed trees. Our results indicate that it is necessary to analyze people’s knowledge about and relations to forest landscapes as well as concepts of nature conservation, natural landscapes, and biodiversity to gain a better understanding of people’s perceptions of natural disturbances. KW - bark beetle disturbance KW - major environmental values KW - well-being KW - inclusion of nature in one’s self KW - national park Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-297429 SN - 1999-4907 VL - 13 IS - 11 ER - TY - JOUR A1 - Henriksson, Sofia A1 - Calderón-Montaño, José Manuel A1 - Solvie, Daniel A1 - Warpman Berglund, Ulrika A1 - Helleday, Thomas T1 - Overexpressed c-Myc sensitizes cells to TH1579, a mitotic arrest and oxidative DNA damage inducer JF - Biomolecules N2 - Previously, we reported that MTH1 inhibitors TH588 and TH1579 selectively induce oxidative damage and kill Ras-expressing or -transforming cancer cells, as compared to non-transforming immortalized or primary cells. While this explains the impressive anti-cancer properties of the compounds, the molecular mechanism remains elusive. Several oncogenes induce replication stress, resulting in under replicated DNA and replication continuing into mitosis, where TH588 and TH1579 treatment causes toxicity and incorporation of oxidative damage. Hence, we hypothesized that oncogene-induced replication stress explains the cancer selectivity. To test this, we overexpressed c-Myc in human epithelial kidney cells (HA1EB), resulting in increased proliferation, polyploidy and replication stress. TH588 and TH1579 selectively kill c-Myc overexpressing clones, enforcing the cancer cell selective killing of these compounds. Moreover, the toxicity of TH588 and TH1579 in c-Myc overexpressing cells is rescued by transcription, proteasome or CDK1 inhibitors, but not by nucleoside supplementation. We conclude that the molecular toxicological mechanisms of how TH588 and TH1579 kill c-Myc overexpressing cells have several components and involve MTH1-independent proteasomal degradation of c-Myc itself, c-Myc-driven transcription and CDK activation. KW - MTH1 KW - TH588 KW - TH1579 KW - c-Myc KW - replication stress KW - DNA damage KW - cell death KW - cancer Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-297547 SN - 2218-273X VL - 12 IS - 12 ER - TY - INPR A1 - Dandekar, Thomas T1 - Protein folding and crystallization applied to qubit interactions and fundamental physics yields a modified inflation model for cosmology N2 - Protein folding achieves a clear solution structure in a huge parameter space (the so-called protein folding problem). Proteins fold in water, and get by this a highly ordered structure. Finally, inside a protein crystal for structure resolution, you have everywhere the same symmetries as there is everywhere the same unit cell. We apply this to qubit interactions to do fundamental physics: in a modified cosmology, we replace the big bang by a condensation event in an eternal all-encompassing ocean of free qubits. Interactions of qubits in the qubit ocean are quite rare but provide a nucleus or seed for a new universe (domain) as the qubits become decoherent and freeze-out into defined bit ensembles. Second, we replace inflation by a crystallization event triggered by the nucleus of interacting qubits to which rapidly more and more qubits attach (like in everyday crystal growth). The crystal unit cell guarantees same symmetries everywhere inside the crystal. The textbook inflation scenario to explain the same laws of nature in our domain is replaced by the unit cell of the crystal formed. Interacting qubits solidify, quantum entropy decreases (but increases in the ocean around). In a modified inflation scenario, the interacting qubits form a rapidly growing domain where the n**m states become separated ensemble states, rising long-range forces stop ultimately further growth. Then standard cosmology with the hot fireball model takes over. Our theory agrees well with lack of inflation traces in cosmic background measurements. We explain by cosmological crystallization instead of inflation: early creation of large-scale structure of voids and filaments, supercluster formation, galaxy formation, and the dominance of matter: the unit cell of our crystal universe has a matter handedness avoiding anti-matter. We prove initiation of qubit interactions can only be 1,2,4 or 8-dimensional (agrees with E8 symmetry of our universe). Repulsive forces at ultrashort distances result from quantization, long-range forces limit crystal growth. Crystals come and go in the qubit ocean. This selects for the ability to lay seeds for new crystals, for self-organization and life-friendliness. The phase space of the crystal agrees with the standard model of the basic four forces for n quanta. It includes all possible ensemble combinations of their quantum states m, a total of n**m states. Neighbor states reach according to transition possibilities (S-matrix) with emergent time from entropic ensemble gradients. However, in our four dimensions there is only one bit overlap to neighbor states left (almost solid, only below Planck quantum there is liquidity left). The E8 symmetry of heterotic string theory has six curled-up, small dimensions which help to keep the qubit crystal together and will never expand. Mathematics focusses on the Hurwitz proof applied to qubit interaction, a toy model of qubit interaction and repulsive forces of qubits. Vacuum energy gets appropriate low inside the crystal. We give first energy estimates for free qubits vs bound qubits, misplacements in the qubit crystal and entropy increase during qubit decoherence / crystal formation. Scalar fields for color interaction/confinement and gravity are derived from the qubit-interaction field. KW - protein folding KW - crystallization KW - qubit interaction KW - decoherence KW - modified inflation Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-346156 ER - TY - THES A1 - Kohl, Patrick Laurenz T1 - The buzz beyond the beehive: population demography, parasite burden and limiting factors of wild-living honeybee colonies in Germany T1 - Das Summen fern des Bienenstocks: Populationsdemographie, Parasitenlast und limitierende Faktoren wildlebender Honigbienenvölker in Deutschland N2 - The western honeybee (Apis mellifera) is widely known as the honey producer and pollinator managed by beekeepers but neglected as a wild bee species. Central European honeybee populations have been anthropogenically disturbed since about 1850 through introgression and moderate artificial selection but have never been truly domesticated due to a lack of mating control. While their decline in the wild was historically attributed to the scarcity of nesting cavities, a contemporary view considers the invasion of the parasitic mite Varroa destructor in the 1970s as the major driver. However, there are no longitudinal population data available that could substantiate either claim. Based on the insight that introduced European honeybees form viable wild populations in eastern North America and reports on the occurrence of wild-living colonies from various European countries, we systematically studied the ecology of wild-living honeybees in Germany. First, we investigated whether wild-living honeybees colonising German forests form a self-sustaining population. Second, we asked how the parasite burden of wild-living colonies relates to that of managed colonies. And third, we explored whether the winter mortality of wild-living colonies is associated with parasite burden, nest depredation, or the lack of resources on the landscape scale. Between 2017 and 2021, we monitored listed trees with black woodpecker cavities for honeybees in the managed forests of three study regions (Swabian Alb, counties Coburg and Lichtenfels, county Weilheim-Schongau). Continuity of occupation was determined using microsatellite genetic markers. Wild-living colonies predictably colonised forests in summer, when about 10% of all cavities were occupied. The annual colony survival rate and colony lifespan (based on N=112 colonies) were 10.6% and 0.6 years, with 90% of colonies surviving summer (July–September), 16% surviving winter (September–April), and 72% surviving spring (April–July). The average maximum and minimum colony densities were 0.23 (July) and 0.02 (April) colonies per km^2. During the (re-)colonisation of forests in spring, swarms preferred cavities that had already been occupied by other honeybee colonies. We estimate the net reproductive rate of the population to be R0= 0.318, meaning that it is currently not self-sustaining but maintained by the annual immigration of swarms from managed hives. The wild-living colonies are feral in a behavioural sense. We compared the occurrence of 18 microparasites among feral colonies (N=64) and managed colonies (N=74) using qPCR. Samples were collected in four regions (the three regions mentioned above and the city of Munich) in July 2020; they consisted of 20 workers per colony captured at flight entrances. We distinguished five colony types representing differences in colony age and management histories. Besides strong regional variation, feral colonies consistently hosted fewer microparasite taxa (median: 5, range 1–8) than managed colonies (median: 6, range 4–9) and had different parasite communities. Microparasites that were notably less prevalent among feral colonies were Trypanosomatidae, Chronic bee paralysis virus, and Deformed wing viruses A and B. In the comparison of five colony types, parasite burden was lowest in newly founded feral colonies, intermediate in overwintered feral colonies and managed nucleus colonies, and highest in overwintered managed colonies and hived swarms. This suggests that the natural mode of colony reproduction by swarming, which creates pauses in brood production, and well-dispersed nests, which reduce horizontal transmission, explain the reduced parasite burden in feral compared to managed colonies. To explore the roles of three potential drivers of feral colony winter mortality, we combined colony observations gathered during the monitoring study with data on colony-level parasite burden, observations and experiments on nest depredation, and landscape analyses. There was no evidence for an effect of summertime parasite burden on subsequent winter mortality: colonies that died (N=57) did not have a higher parasite burden than colonies that survived (N=10). Camera traps (N=15) installed on cavity trees revealed that honeybee nests are visited by a range of vertebrate species throughout the winter at rates of up to 10 visits per week. Four woodpecker species, great tits, and pine martens acted as true nest depredators. The winter survival rate of colonies whose nest entrances were protected by screens of wire mesh (N=32) was 50% higher than that of colonies with unmanipulated entrances (N=40). Analyses of land cover maps revealed that the landscapes surrounding surviving colonies (N=19) contained on average 6.4 percentage points more resource-rich cropland than landscapes surrounding dying colonies (N=94). We estimate that tens of thousands of swarms escape from apiaries each year to occupy black woodpecker cavities and other hollow spaces in Germany and that feral colonies make up about 5% of the regional honeybee populations. They are unlikely to contribute disproportionately to the spread of bee diseases. Instead, by spatially complementing managed colonies, they contribute to the pollination of wild plants in forests. Honeybees occupying tree cavities likely have various effects on forest communities by acting as nest site competitors or prey, and by accumulating biomass in tree holes. Nest depredation (a consequence of a lack of well-protected nest sites) and food resource limitation seem to be more important than parasites in hampering feral colony survival. The outstanding question is how environmental and intrinsic factors interact in preventing population establishment. Nest boxes with movable frames could be used to better study the environmental drivers of feral colonies’ mortality. Pairs of wild (self-sustaining) and managed populations known to exist outside Europe could provide answers to whether modern apiculture creates honeybee populations maladapted to life in the wild. In Europe, large continuous forests might represent evolutionary refuges for wild honeybees. N2 - Die Honigbiene (Apis mellifera) ist als Nutztier weitbekannt, doch als Wildtier vernachlässigt. Seit etwa 1850 sind ihre Populationen in Mitteleuropa durch Introgression und moderate künstliche Selektion vom Menschen beeinflusst. Die Art wurde jedoch aufgrund fehlender Paarungskontolle nie wirklich domestiziert. Früher wurde der Rückgang wildlebender Honigbienen dem Verlust geeigneter Nistplätze zugeschrieben. Heute wird meist die Bienenmilbe Varroa destructor als Hauptursache angenommen. Es gibt allerdings keine Langzeitdaten, welche diese Annahmen stützen könnten. Basierend auf der Erkenntnis, dass eingeführte Honigbienen in Nordamerika stabile wilde Populationen bilden, und aufgrund von Berichten über das Vorkommen wildlebender Bienenvölker in verschiedenen Ländern Europas, widmeten wir uns dem systematischen Studium wildlebender Honigbienen in Deutschland. Zunächst untersuchten wir, ob waldbewohnende Bienenvölker eine selbsterhaltende Population bilden. Zweitens stellten wir die Frage, inwiefern sich wildlebende und imkerlich gehaltene Völker in ihrer Parasitenlast unterscheiden. Drittens testeten wir, ob Winterverluste wildlebender Bienenvölker mit Parasitendruck, Nestprädation oder mangelndem Nahrungsangebot auf Landschaftsebene in Verbindung stehen. In Wirtschaftswäldern dreier Untersuchungsgebiete (Schwäbische Alb, Landkreise Coburg und Lichtenfels, Landkreis Weilheim-Schongau) kontrollierten wir zwischen 2017 und 2021 bekannte Höhlenbäume des Schwarzspechts auf Besiedlung durch Honigbienen. Das Überleben einzelner Bienenvölker wurde zusätzlich mittels Analyse von Mikrosatelliten DNA überprüft. Nach verlässlichem Muster besiedelten Honigbienen jeden Sommer etwa 10% der Baumhöhlen. Die jährliche Überlebensrate und die Lebenserwartung der Völker (N=112) betrugen 10,6% und 0,6 Jahre, wobei 90% den Sommer (Juli–September), 16% den Winter (September–April) und 72% das Frühjahr (April–Juli) überlebten. Die durchschnittliche maximale (Juli) und minimale (April) Koloniedichte betrug 0,23 bzw. 0,02 Bienenvölker pro km^2. Während der (Wieder)Besiedlung von Wäldern im Frühjahr bevorzugten Bienenschwärme solche Baumhöhlen, welche zuvor schon von Bienen besiedelt worden waren. Die Nettoreproduktionsrate der wildlebenden Population wird auf R0= 0,318 geschätzt, was bedeutet, dass diese zurzeit nicht selbsterhaltend ist, sondern durch die jährliche Einwanderung von Bienenschwärmen aus der Imkerei aufrechterhalten wird. Wir untersuchten wildlebende (N=64) und imkerlich gehaltene Bienenvölker (N=74) auf den Befall mit 18 verschiedenen Mikroparasiten mittels qPCR. Die Proben stammten aus den drei oben genannten Gebieten sowie aus dem Stadtgebiet von München. Eine Probe bestand aus 20 Arbeiterinnen, welche am Flugloch gefangen wurden. Wir unterschieden fünf Kolonietypen aufgrund des Alters (jünger oder älter als ein Jahr) und der unmittelbaren Geschichte der Bewirtschaftung durch Imkerinnen und Imker. Abgesehen von regionalen Unterschieden in der Parasitenlast waren wildlebende Völker mit einer geringeren Anzahl Parasitentaxa befallen (Median: 5, Spanne: 1–8) als imkerlich gehaltene Völker (Median: 6, Spanne: 4–9) und wiesen eine veränderte Zusammensetzung von Parasiten auf. Seltener bei wildlebenden Bienenvölkern waren besonders Trypanosomatidae, das Chronische-Paralysevirus, sowie die Flügeldeformationsviren A und B. Im Vergleich der fünf Kolonietypen war die Parasitenlast bei neu gegründeten wildlebenden Völkern am geringsten, intermediär bei überwinterten wildlebenden Völkern und Brutablegern, und am höchsten bei überwinterten Wirtschaftsvölkern und bei durch Schwärme gegründeten imkerlich gehaltenen Völkern. Dies deutet darauf hin, dass das Schwärmen (Entstehung von Brutpausen) sowie die größere Distanz zwischen Nestern (Verminderung der horizontalen Krankheitsübertragung) die geringere Parasitenlast wildlebender Bienenvölker erklären. Wir kombinierten Beobachtungen zum Winterüberleben aus dem Monitoring mit Daten zur Parasitenlast, mit Beobachtungen und Experimenten zur Nestprädation und mit Landschaftsanalysen. Es ergab sich kein Hinweis auf einen Zusammenhang zwischen Parasitenlast im Sommer und anschließendem Überwinterungserfolg: Völker, welche den Winter nicht überlebten (N=57), hatten zuvor keine höhere Parasitenlast als solche, welche den Winter überlebten (N=10). Kamerafallen (N=15) offenbarten, dass Honigbienennester im Winter von einer Vielzahl von Vögeln und Säugern mit bis zu 10 Besuchen pro Woche heimgesucht werden. Vier Spechtarten, Kohlmeisen und Baummarder wurden als echte Nestplünderer identifiziert. Bienenvölker, deren Nesteingang mit Maschendraht geschützt war (N=32), hatten eine 50% höhere Winterüberlebensrate als Völker ohne Schutz (N=40). Die Analyse von Landnutzungskarten zeigte, dass sich Bienenvölker, welche den Winter überlebten (N=19), in Landschaften mit durchschnittlich 6,4% höherem Anteil von Ackerflächen befanden als solche, die den Winter nicht überlebten (N=94). Wir schätzen, dass in Deutschland jährlich zehntausende Schwärme von Bienenständen entfliehen, um sich in Spechthöhlen oder anderen Hohlräumen anzusiedeln. Der Anteil wildlebender Völker an der Gesamtbienenpopulation beträgt im Sommer etwa 5%. Sie spielen vermutlich eine untergeordnete Rolle bei der Verbreitung von Bienenkrankheiten. Durch die Ergänzung imkerlich gehaltener Völker in Waldgebieten tragen sie zur Bestäubung waldbewohnender Pflanzenarten bei. Die Besiedlung von Baumhöhlen sollte vielseitige Auswirkungen auf Lebensgemeinschaften im Wald haben: Bienenvölker konkurrieren um Nistplätze, sind reiche Beute im Winter und akkumulieren organisches Material. Nestprädation (eine Folge des Mangels an sicheren Nisthöhlen) und Ressourcenlimitierung spielen offenbar derzeit eine größere Rolle als Parasiten bei der Erklärung von Winterverlusten. Eine offene Frage ist, inwiefern Umwelt und genetische Dispositionen die Etablierung wilder Honigbienenpopulationen verhindern. Künstliche Nistkästen könnten genutzt werden, um die Rolle von Umweltfaktoren genauer zu untersuchen. Populationen wilder Honigbienen außerhalb Europas könnten Erkenntnisse dazu liefern, inwiefern sich die moderne Imkerei auf die Anpassungen der Honigbienen als Wildtier auswirkt. In Europa könnten große zusammenhängende Waldgebiete als evolutionäre Refugien für wilde Honigbienen dienen. KW - Biene KW - Insektensterben KW - Wald KW - Spechte KW - Imkerei KW - wild honey bees KW - swarming KW - tree cavity KW - monitoring KW - bee diseases KW - Wilde Honigbienen KW - Bienenschwarm KW - Baumhöhle KW - Monitoring KW - Bienenkrankheiten KW - Nisthöhle Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-330327 ER - TY - THES A1 - Bergmann Borges, Alyssa T1 - The endo-lysosomal system of \(Trypanosoma\) \(brucei\): insights from a protist cell model T1 - Das Endo-lysosomale System von \(Trypanosoma\) \(brucei\): Erkenntnisse aus einem Protisten-Zellmodell N2 - Most of the studies in cell biology primarily focus on models from the opisthokont group of eukaryotes. However, opisthokonts do not encompass the full diversity of eukaryotes. Thus, it is necessary to broaden the research focus to other organisms to gain a comprehensive understanding of basic cellular processes shared across the tree of life. In this sense, Trypanosoma brucei, a unicellular eukaryote, emerges as a viable alternative. The collaborative efforts in genome sequencing and protein tagging over the past two decades have significantly expanded our knowledge on this organism and have provided valuable tools to facilitate a more detailed analysis of this parasite. Nevertheless, numerous questions still remain. The survival of T. brucei within the mammalian host is intricately linked to the endo-lysosomal system, which plays a critical role in surface glycoprotein recycling, antibody clearance, and plasma membrane homeostasis. However, the dynamics of the duplication of the endo-lysosomal system during T. brucei proliferation and its potential relationship with plasma membrane growth remain poorly understood. Thus, as the primary objective, this thesis explores the endo-lysosomal system of T. brucei in the context of the cell cycle, providing insights on cell surface growth, endosome duplication, and clathrin recruitment. In addition, the study revisits ferritin endocytosis to provide quantitative data on the involvement of TbRab proteins (TbRab5A, TbRab7, and TbRab11) and the different endosomal subpopulations (early, late, and recycling endosomes, respectively) in the transport of this fluid-phase marker. Notably, while these subpopulations function as distinct compartments, different TbRabs can be found within the same region or structure, suggesting a potential physical connection between the endosomal subpopulations. The potential physical connection of endosomes is further explored within the context of the cell cycle and, finally, the duplication and morphological plasticity of the lysosome are also investigated. Overall, these findings provide insights into the dynamics of plasma membrane growth and the coordinated duplication of the endo-lysosomal system during T. brucei proliferation. The early duplication of endosomes suggests their potential involvement in plasma membrane growth, while the late duplication of the lysosome indicates a reduced role in this process. The recruitment of clathrin and TbRab GTPases to the site of endosome formation supports the assumption that the newly formed endosomal system is active during cell division and, consequently, indicates its potential role in plasma membrane homeostasis. Furthermore, considering the vast diversity within the Trypanosoma genus, which includes ~500 described species, the macroevolution of the group was investigated using the combined information of the 18S rRNA gene sequence and structure. The sequence-structure analysis of T. brucei and other 42 trypanosome species was conducted in the context of the diversity of Trypanosomatida, the order in which trypanosomes are placed. An additional analysis focused on Trypanosoma highlighted key aspects of the group’s macroevolution. To explore these aspects further, additional trypanosome species were included, and the changes in the Trypanosoma tree topology were analyzed. The sequence-structure phylogeny confirmed the independent evolutionary history of the human pathogens T. brucei and Trypanosoma cruzi, while also providing insights into the evolution of the Aquatic clade, paraphyly of groups, and species classification into subgenera. N2 - Die meisten Studien in der Zellbiologie konzentrieren sich in erster Linie auf Modelle aus der Opisthokont-Gruppe der Eukaryonten. Die Opisthokonten umfassen jedoch nicht die gesamte Vielfalt der Eukaryonten. Daher ist es notwendig, den Forschungsschwerpunkt auf andere Organismen auszuweiten, um ein umfassendes Verständnis grundlegender zellulärer Prozesse zu erlangen, die im gesamten Lebensbaum vorkommen. In diesem Sinne stellt Trypanosoma brucei, ein einzelliger Eukaryote, eine brauchbare Alternative dar. Die gemeinsamen Anstrengungen bei der Genomsequenzierung und der Markierung von Proteinen in den letzten zwei Jahrzehnten haben unser Wissen über diesen Organismus erheblich erweitert und wertvolle Instrumente für eine detailliertere Analyse dieses Parasiten bereitgestellt. Dennoch bleiben noch zahlreiche Fragen offen. Das Überleben von T. brucei im Säugetierwirt ist eng mit dem endo-lysosomalen System verknüpft, das eine entscheidende Rolle beim Recycling von Oberflächenglykoproteinen, der Antikörper-Clearance und der Homöostase der Plasmamembran spielt. Die Dynamik der Verdoppelung des endo-lysosomalen Systems während der Vermehrung von T. brucei und seine mögliche Beziehung zum Wachstum der Plasmamembran sind jedoch noch wenig bekannt. In dieser Arbeit wird daher das endo-lysosomale System von T. brucei im Kontext des Zellzyklus untersucht, um Erkenntnisse über das Wachstum der Zelloberfläche, die Verdopplung der Endosomen und die Clathrin-Rekrutierung zu gewinnen. Darüber hinaus wird in der Studie die Ferritin-Endozytose erneut untersucht, um quantitative Daten über die Beteiligung der TbRab-Proteine (TbRab5A, TbRab7 und TbRab11) und der verschiedenen endosomalen Subpopulationen (frühe, späte bzw. Recycling-Endosomen) am Transport dieses Flüssigphasenmarkers zu erhalten. Bemerkenswert ist, dass diese Subpopulationen zwar als unterschiedliche Kompartimente fungieren, aber verschiedene TbRabs in derselben Region oder Struktur gefunden werden können, was auf eine mögliche physische Verbindung zwischen den endosomalen Subpopulationen hindeutet. Die potenzielle physikalische Verbindung von Endosomen wird im Zusammenhang mit dem Zellzyklus weiter erforscht, und schließlich werden auch die Verdopplung und die morphologische Plastizität des Lysosoms untersucht. Insgesamt bieten diese Ergebnisse Einblicke in die Dynamik des Plasmamembranwachstums und die koordinierte Verdopplung des endo-lysosomalen Systems während der Proliferation von T. brucei. Die frühe Verdoppelung der Endosomen deutet auf ihre mögliche Beteiligung am Plasmamembranwachstum hin, während die späte Verdoppelung der Lysosomen auf eine geringere Rolle in diesem Prozess hindeutet. Die Rekrutierung von Clathrin- und TbRab-GTPasen an der Stelle der Endosomenbildung unterstützt die Annahme, dass das neu gebildete endosomale System während der Zellteilung aktiv ist, und deutet folglich auf seine potenzielle Rolle bei der Homöostase der Plasmamembran hin. In Anbetracht der enormen Vielfalt innerhalb der Gattung Trypanosoma, die etwa 500 beschriebene Arten umfasst, wurde die Makroevolution der Gruppe anhand der kombinierten Informationen der 18S rRNA-Gensequenz und Struktur untersucht. Die Sequenz-Struktur-Analyse von T. brucei und anderen 42 Trypanosomen-Arten wurde im Zusammenhang mit der Vielfalt der Trypanosomatida, der Ordnung, in die Trypanosomen eingeordnet werden, durchgeführt. Eine zusätzliche Analyse, die sich auf Trypanosoma konzentrierte, hob Schlüsselaspekte der Makroevolution dieser Gruppe hervor. Um diese Aspekte weiter zu erforschen, wurden zusätzliche Trypanosomenarten einbezogen und die Veränderungen in der Topologie des Trypanosoma-Baums analysiert. Die Sequenz-Struktur-Phylogenie bestätigte die unabhängige Evolutionsgeschichte der humanen Krankheitserreger T. brucei und Trypanosoma cruzi, während sie gleichzeitig Einblicke in die Evolution der aquatischen Klade, die Paraphylie von Gruppen und die Klassifizierung der Arten in Untergattungen lieferte. KW - 18S rRNA KW - Endocytose KW - Zellzyklus KW - Phylogenie KW - Endocytosis KW - Cell cycle KW - Trypanosoma KW - Phylogeny KW - Sequence-Structure KW - Endosomes KW - Lysosome Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-329248 ER - TY - JOUR A1 - Kotlyar, Mischa J. A1 - Krebs, Markus A1 - Solimando, Antonio Giovanni A1 - Marquardt, André A1 - Burger, Maximilian A1 - Kübler, Hubert A1 - Bargou, Ralf A1 - Kneitz, Susanne A1 - Otto, Wolfgang A1 - Breyer, Johannes A1 - Vergho, Daniel C. A1 - Kneitz, Burkhard A1 - Kalogirou, Charis T1 - Critical evaluation of a microRNA-based risk classifier predicting cancer-specific survival in renal cell carcinoma with tumor thrombus of the inferior vena cava JF - Cancers N2 - (1) Background: Clear cell renal cell carcinoma extending into the inferior vena cava (ccRCC\(^{IVC}\)) represents a clinical high-risk setting. However, there is substantial heterogeneity within this patient subgroup regarding survival outcomes. Previously, members of our group developed a microRNA(miR)-based risk classifier — containing miR-21-5p, miR-126-3p and miR-221-3p expression — which significantly predicted the cancer-specific survival (CSS) of ccRCC\(^{IVC}\) patients. (2) Methods: Examining a single-center cohort of tumor tissue from n = 56 patients with ccRCC\(^{IVC}\), we measured the expression levels of miR-21, miR-126, and miR-221 using qRT-PCR. The prognostic impact of clinicopathological parameters and miR expression were investigated via single-variable and multivariable Cox regression. Referring to the previously established risk classifier, we performed Kaplan–Meier analyses for single miR expression levels and the combined risk classifier. Cut-off values and weights within the risk classifier were taken from the previous study. (3) Results: miR-21 and miR-126 expression were significantly associated with lymphonodal status at the time of surgery, the development of metastasis during follow-up, and cancer-related death. In Kaplan–Meier analyses, miR-21 and miR-126 significantly impacted CSS in our cohort. Moreover, applying the miR-based risk classifier significantly stratified ccRCC\(^{IVC}\) according to CSS. (4) Conclusions: In our retrospective analysis, we successfully validated the miR-based risk classifier within an independent ccRCC\(^{IVC}\) cohort. KW - kidney cancer KW - RCC KW - venous infiltration KW - biomarker KW - miR KW - risk stratification Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-311040 SN - 2072-6694 VL - 15 IS - 7 ER - TY - JOUR A1 - Rackevei, Antonia S. A1 - Borges, Alyssa A1 - Engstler, Markus A1 - Dandekar, Thomas A1 - Wolf, Matthias T1 - About the analysis of 18S rDNA sequence data from trypanosomes in barcoding and phylogenetics: tracing a continuation error occurring in the literature JF - Biology N2 - The variable regions (V1–V9) of the 18S rDNA are routinely used in barcoding and phylogenetics. In handling these data for trypanosomes, we have noticed a misunderstanding that has apparently taken a life of its own in the literature over the years. In particular, in recent years, when studying the phylogenetic relationship of trypanosomes, the use of V7/V8 was systematically established. However, considering the current numbering system for all other organisms (including other Euglenozoa), V7/V8 was never used. In Maia da Silva et al. [Parasitology 2004, 129, 549–561], V7/V8 was promoted for the first time for trypanosome phylogenetics, and since then, more than 70 publications have replicated this nomenclature and even discussed the benefits of the use of this region in comparison to V4. However, the primers used to amplify the variable region of trypanosomes have actually amplified V4 (concerning the current 18S rDNA numbering system). KW - RNA secondary structure KW - variable regions KW - V1–V9 KW - V4 KW - V7/V8 KW - Trypanosoma Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-297562 SN - 2079-7737 VL - 11 IS - 11 ER - TY - JOUR A1 - Flemming, S. A1 - Hankir, M. A1 - Ernestus, R.-I. A1 - Seyfried, F. A1 - Germer, C.-T. A1 - Meybohm, P. A1 - Wurmb, T. A1 - Vogel, U. A1 - Wiegering, A. T1 - Surgery in times of COVID-19 — recommendations for hospital and patient management JF - Langenbeck's Archives of Surgery N2 - Background The novel coronavirus disease 2019 (COVID-19), caused by severe acute respiratory syndrome coronavirus 2(SARS-CoV-2), has escalated rapidly to a global pandemic stretching healthcare systems worldwide to their limits. Surgeonshave had to immediately react to this unprecedented clinical challenge by systematically repurposing surgical wards. Purpose To provide a detailed set of guidelines developed in a surgical ward at University Hospital Wuerzburg to safelyaccommodate the exponentially rising cases of SARS-CoV-2 infected patients without compromising the care of emergencysurgery and oncological patients or jeopardizing the well-being of hospital staff. Conclusions The dynamic prioritization of SARS-CoV-2 infected and surgical patient groups is key to preserving life whilemaintaining high surgical standards. Strictly segregating patient groups in emergency rooms, non-intensive care wards andoperating areas prevents viral spread while adequately training and carefully selecting hospital staff allow them to confidentlyand successfully undertake their respective clinical duties. KW - SARS-CoV-2 KW - COVID-19 KW - Surgery Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-231766 SN - 1435-2443 VL - 405 ER - TY - THES A1 - Münch, Luca T1 - Die Rolle transposabler Elemente in der Genese des malignen Melanom im Fischmodell Xiphophorus T1 - The role of transposable elements in malignant melanoma development in the Xiphophorus fish model N2 - Der Name der transposablen Elemente beruht auf ihrer Fähigkeit, ihre genomische Position verändern zu können. Durch Chromosomenaberrationen, Insertionen oder Deletionen können ihre genomischen Transpositionen genetische Instabilität verursachen. Inwieweit sie darüber hinaus regulatorischen Einfluss auf Zellfunktionen besitzen, ist Gegenstand aktueller Forschung ebenso wie die daraus resultierende Frage nach der Gesamtheit ihrer biologischen Signifikanz. Die Weiterführung experimenteller Forschung ist unabdingbar, um weiterhin offenen Fragen nachzugehen. Das Xiphophorus-Melanom-Modell stellt hierbei eines der ältesten Tiermodelle zur Erforschung des malignen Melanoms dar. Durch den klar definierten genetischen Hintergrund eignet es sich hervorragend zur Erforschung des bösartigen schwarzen Hautkrebses, welcher nach wie vor die tödlichste aller bekannten Hautkrebsformen darstellt. Die hier vorliegende Arbeit beschäftigt sich mit der Rolle transposabler Elemente in der malignen Melanomgenese von Xiphophorus. N2 - The term “transposable elements” (TEs) is based on their ability to change their genomic position. Through insertions, deletions or chromosomal aberrations, their genomic mobility can cause genetic instability. The extent to which they further exert regulatory influence on cellular functions is the subject of current research, as is the resulting question of their overall biological significance. To further pursue these questions the continuation of experimental research is indispensable. In this regard, the Xiphophorus- melanoma-model represents one of the oldest animal models for the study of malignant melanoma. Thanks to its clearly defined genetic background, it is excellently suited for research into melanoma, which continues to be the most lethal of all known forms of skin cancer. The work presented here investigated the role of transposable elements in malignant melanomagenesis of Xiphophorus. KW - Transposon KW - Platy KW - Melanom KW - Überexpression KW - Schwertkärpfling KW - Expression KW - expression KW - Xiphophorus KW - xiphophorus Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-289228 ER - TY - JOUR A1 - Yang, Manli A1 - Rajeeve, Karthika A1 - Rudel, Thomas A1 - Dandekar, Thomas T1 - Comprehensive Flux Modeling of Chlamydia trachomatis Proteome and qRT-PCR Data Indicate Biphasic Metabolic Differences Between Elementary Bodies and Reticulate Bodies During Infection JF - Frontiers in Microbiology N2 - Metabolic adaptation to the host cell is important for obligate intracellular pathogens such as Chlamydia trachomatis (Ct). Here we infer the flux differences for Ct from proteome and qRT-PCR data by comprehensive pathway modeling. We compare the comparatively inert infectious elementary body (EB) and the active replicative reticulate body (RB) systematically using a genome-scale metabolic model with 321 metabolites and 277 reactions. This did yield 84 extreme pathways based on a published proteomics dataset at three different time points of infection. Validation of predictions was done by quantitative RT-PCR of enzyme mRNA expression at three time points. Ct’s major active pathways are glycolysis, gluconeogenesis, glycerol-phospholipid (GPL) biosynthesis (support from host acetyl-CoA) and pentose phosphate pathway (PPP), while its incomplete TCA and fatty acid biosynthesis are less active. The modeled metabolic pathways are much more active in RB than in EB. Our in silico model suggests that EB and RB utilize folate to generate NAD(P)H using independent pathways. The only low metabolic flux inferred for EB involves mainly carbohydrate metabolism. RB utilizes energy -rich compounds to generate ATP in nucleic acid metabolism. Validation data for the modeling include proteomics experiments (model basis) as well as qRT-PCR confirmation of selected metabolic enzyme mRNA expression differences. The metabolic modeling is made fully available here. Its detailed insights and models on Ct metabolic adaptations during infection are a useful modeling basis for future studies. KW - metabolic modeling KW - metabolic flux KW - infection biology KW - elementary body KW - reticulate body KW - Chlamydia trachomatis Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-189434 SN - 1664-302X VL - 10 IS - 2350 ER - TY - JOUR A1 - Yadav, Preeti A1 - Selvaraj, Bhuvaneish T. A1 - Bender, Florian L. P. A1 - Behringer, Marcus A1 - Moradi, Mehri A1 - Sivadasan, Rajeeve A1 - Dombert, Benjamin A1 - Blum, Robert A1 - Asan, Esther A1 - Sauer, Markus A1 - Julien, Jean-Pierre A1 - Sendtner, Michael T1 - Neurofilament depletion improves microtubule dynamics via modulation of Stat3/stathmin signaling JF - Acta Neuropathologica N2 - In neurons, microtubules form a dense array within axons, and the stability and function of this microtubule network is modulated by neurofilaments. Accumulation of neurofilaments has been observed in several forms of neurodegenerative diseases, but the mechanisms how elevated neurofilament levels destabilize axons are unknown so far. Here, we show that increased neurofilament expression in motor nerves of pmn mutant mice, a model of motoneuron disease, causes disturbed microtubule dynamics. The disease is caused by a point mutation in the tubulin-specific chaperone E (Tbce) gene, leading to an exchange of the most C-terminal amino acid tryptophan to glycine. As a consequence, the TBCE protein becomes instable which then results in destabilization of axonal microtubules and defects in axonal transport, in particular in motoneurons. Depletion of neurofilament increases the number and regrowth of microtubules in pmn mutant motoneurons and restores axon elongation. This effect is mediated by interaction of neurofilament with the stathmin complex. Accumulating neurofilaments associate with stathmin in axons of pmn mutant motoneurons. Depletion of neurofilament by Nefl knockout increases Stat3-stathmin interaction and stabilizes the microtubules in pmn mutant motoneurons. Consequently, counteracting enhanced neurofilament expression improves axonal maintenance and prolongs survival of pmn mutant mice. We propose that this mechanism could also be relevant for other neurodegenerative diseases in which neurofilament accumulation and loss of microtubules are prominent features. KW - Amyotrophic-lateral-sclerosis KW - Transgenic mice KW - Mouse model KW - Alzheimers disease KW - Neurofilament KW - Progressive motor neuronopathy KW - Axonal transport KW - Intermediate filaments KW - Motoneuron disease KW - Lacking neurofilaments KW - Missense mutation KW - Axon degeneration KW - Microtubules KW - Stathmin KW - Stat3 Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-188234 VL - 132 IS - 1 ER - TY - JOUR A1 - Weiss, Esther A1 - Schlegel, Jan A1 - Terpitz, Ulrich A1 - Weber, Michael A1 - Linde, Jörg A1 - Schmitt, Anna-Lena A1 - Hünniger, Kerstin A1 - Marischen, Lothar A1 - Gamon, Florian A1 - Bauer, Joachim A1 - Löffler, Claudia A1 - Kurzai, Oliver A1 - Morton, Charles Oliver A1 - Sauer, Markus A1 - Einsele, Hermann A1 - Loeffler, Juergen T1 - Reconstituting NK Cells After Allogeneic Stem Cell Transplantation Show Impaired Response to the Fungal Pathogen Aspergillus fumigatus JF - Frontiers in Immunology N2 - Delayed natural killer (NK) cell reconstitution after allogeneic stem cell transplantation (alloSCT) is associated with a higher risk of developing invasive aspergillosis. The interaction of NK cells with the human pathogen Aspergillus (A.) fumigatus is mediated by the fungal recognition receptor CD56, which is relocated to the fungal interface after contact. Blocking of CD56 signaling inhibits the fungal mediated chemokine secretion of MIP-1α, MIP-1β, and RANTES and reduces cell activation, indicating a functional role of CD56 in fungal recognition. We collected peripheral blood from recipients of an allograft at defined time points after alloSCT (day 60, 90, 120, 180). NK cells were isolated, directly challenged with live A. fumigatus germ tubes, and cell function was analyzed and compared to healthy age and gender-matched individuals. After alloSCT, NK cells displayed a higher percentage of CD56\(^{bright}\)CD16\(^{dim}\) cells throughout the time of blood collection. However, CD56 binding and relocalization to the fungal contact side were decreased. We were able to correlate this deficiency to the administration of corticosteroid therapy that further negatively influenced the secretion of MIP-1α, MIP-1β, and RANTES. As a consequence, the treatment of healthy NK cells ex vivo with corticosteroids abrogated chemokine secretion measured by multiplex immunoassay. Furthermore, we analyzed NK cells regarding their actin cytoskeleton by Structured Illumination Microscopy (SIM) and flow cytometry and demonstrate an actin dysfunction of NK cells shown by reduced F-actin content after fungal co-cultivation early after alloSCT. This dysfunction remains until 180 days post-alloSCT, concluding that further actin-dependent cellular processes may be negatively influenced after alloSCT. To investigate the molecular pathomechansism, we compared CD56 receptor mobility on the plasma membrane of healthy and alloSCT primary NK cells by single-molecule tracking. The results were very robust and reproducible between tested conditions which point to a different molecular mechanism and emphasize the importance of proper CD56 mobility. KW - natural killer cell KW - stem cell transplantation KW - corticosteroids KW - CCL3 KW - CCL4 KW - CCL5 Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-212581 SN - 1664-3224 VL - 11 ER - TY - JOUR A1 - Rother, Lisa A1 - Kraft, Nadine A1 - Smith, Dylan B. A1 - El Jundi, Basil A1 - Gill, Richard J. A1 - Pfeiffer, Keram T1 - A micro-CT-based standard brain atlas of the bumblebee JF - Cell and Tissue Research N2 - In recent years, bumblebees have become a prominent insect model organism for a variety of biological disciplines, particularly to investigate learning behaviors as well as visual performance. Understanding these behaviors and their underlying neurobiological principles requires a clear understanding of brain anatomy. Furthermore, to be able to compare neuronal branching patterns across individuals, a common framework is required, which has led to the development of 3D standard brain atlases in most of the neurobiological insect model species. Yet, no bumblebee 3D standard brain atlas has been generated. Here we present a brain atlas for the buff-tailed bumblebee Bombus terrestris using micro-computed tomography (micro-CT) scans as a source for the raw data sets, rather than traditional confocal microscopy, to produce the first ever micro-CT-based insect brain atlas. We illustrate the advantages of the micro-CT technique, namely, identical native resolution in the three cardinal planes and 3D structure being better preserved. Our Bombus terrestris brain atlas consists of 30 neuropils reconstructed from ten individual worker bees, with micro-CT allowing us to segment neuropils completely intact, including the lamina, which is a tissue structure often damaged when dissecting for immunolabeling. Our brain atlas can serve as a platform to facilitate future neuroscience studies in bumblebees and illustrates the advantages of micro-CT for specific applications in insect neuroanatomy. KW - neuropils KW - Bombus terrestris KW - insect standard brain atlas KW - iterative shape averaging KW - reconstruction Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-267783 SN - 1432-0878 VL - 386 IS - 1 ER - TY - JOUR A1 - Fathy, Moustafa A1 - Darwish, Mostafa A. A1 - Abdelhamid, Al-Shaimaa M. A1 - Alrashedy, Gehad M. A1 - Othman, Othman Ali A1 - Naseem, Muhammad A1 - Dandekar, Thomas A1 - Othman, Eman M. T1 - Kinetin ameliorates cisplatin-induced hepatotoxicity and lymphotoxicity via attenuating oxidative damage, cell apoptosis and inflammation in rats JF - Biomedicines N2 - Though several previous studies reported the in vitro and in vivo antioxidant effect of kinetin (Kn), details on its action in cisplatin-induced toxicity are still scarce. In this study we evaluated, for the first time, the effects of kinetin in cisplatin (cp)- induced liver and lymphocyte toxicity in rats. Wistar male albino rats were divided into nine groups: (i) the control (C), (ii) groups 2,3 and 4, which received 0.25, 0.5 and 1 mg/kg kinetin for 10 days; (iii) the cisplatin (cp) group, which received a single intraperitoneal injection of CP (7.0 mg/kg); and (iv) groups 6, 7, 8 and 9, which received, for 10 days, 0.25, 0.5 and 1 mg/kg kinetin or 200 mg/kg vitamin C, respectively, and Cp on the fourth day. CP-injected rats showed a significant impairment in biochemical, oxidative stress and inflammatory parameters in hepatic tissue and lymphocytes. PCR showed a profound increase in caspase-3, and a significant decline in AKT gene expression. Intriguingly, Kn treatment restored the biochemical, redox status and inflammatory parameters. Hepatic AKT and caspase-3 expression as well as CD95 levels in lymphocytes were also restored. In conclusion, Kn mitigated oxidative imbalance, inflammation and apoptosis in CP-induced liver and lymphocyte toxicity; therefore, it can be considered as a promising therapy. KW - cisplatin KW - hepatotoxicity KW - lymphotoxicity KW - oxidative stress KW - AKT KW - CD95 KW - caspase-3 Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-281686 SN - 2227-9059 VL - 10 IS - 7 ER - TY - JOUR A1 - Leidinger, Ludwig A1 - Vedder, Daniel A1 - Cabral, Juliano Sarmento T1 - Temporal environmental variation may impose differential selection on both genomic and ecological traits JF - Oikos N2 - The response of populations and species to changing conditions determines how community composition will change functionally, including via trait shifts. Selection from standing variation has been suggested to be more efficient than acquiring new mutations. Yet, studies on community trait composition and trait selection largely focus on phenotypic variation in ecological traits, whereas the underlying genomic traits remain understudied. Using a genome‐explicit, niche‐ and individual‐based model, we address the potential interactions between genomic and ecological traits shaping communities under an environmental selective forcing, namely temporal positively autocorrelated environmental fluctuation. In this model, all ecological traits are explicitly coded by the genome. For our experiments, we initialized 90 replicate communities, each with ca 350 initial species, characterized by random genomic and ecological trait combinations, on a 2D spatially explicit landscape with two orthogonal gradients (temperature and resource use). We exposed each community to two contrasting scenarios: without (i.e. static environments) and with temporal variation. We then analyzed emerging compositions of both genomic and ecological traits at the community, population and genomic levels. Communities in variable environments were species poorer than in static environments, and populations more abundant, whereas genomes had lower genetic linkage, mean genetic variation and a non‐significant tendency towards higher numbers of genes. The surviving genomes (i.e. those selected by variable environments) coded for enhanced environmental tolerance and smaller biomass, which resulted in faster life cycles and thus also in increased potential for evolutionary rescue. Under temporal environmental variation, larger, less linked genomes retained more variation in mean dispersal ability at the population level than at genomic level, whereas the opposite trend emerged for biomass. Our results provide clues to how sexually‐reproducing diploid plant communities might react to variable environments and highlights the importance of genomic traits and their interaction with ecological traits for eco‐evolutionary responses to changing climates. KW - environmental variability KW - genomic traits KW - mechanistic model KW - rapid evolution KW - standing variation Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-238945 VL - 130 IS - 7 SP - 1100 EP - 1115 ER - TY - JOUR A1 - Sponsler, Douglas B. A1 - Bratman, Eve Z. T1 - Beekeeping in, of or for the city? A socioecological perspective on urban apiculture JF - People and Nature N2 - The term ‘urban beekeeping’ connotes a host of meanings—sociopolitical, commercial, ecological and personal—beyond the mere description of where bees and beekeepers happen to coincide. Yet, these meanings are seldom articulated explicitly or brought into critical engagement with the relevant fields of urban ecology and political ecology. Beginning with a brief account of the history of urban beekeeping in the United States, we draw upon urban ecological theory to construct a conceptual model of urban beekeeping that distinguishes beekeeping in, of and for the city. In our model, beekeeping in the city describes the mere importation of the traditionally rural practice of beekeeping into urban spaces for the private reasons of the individual beekeeper, whereas beekeeping of the city describes beekeeping that is consciously tailored to the urban context, often accompanied by (semi)professionalization of beekeepers and the formation of local expert communities (i.e. beekeeping associations). Beekeeping for the city describes a shift in mindset in which beekeeping is directed to civic ends beyond the boundaries of the beekeeping community per se. Using this framework, we identify and discuss specific socioecological assets and liabilities of urban beekeeping, and how these relate to beekeeping in, of and for the city. We then formulate actionable guidelines for maturing the practice of urban beekeeping into a beneficent and self‐critical form of urban ecological citizenship; these include fostering self‐regulation within the beekeeping community, harnessing beekeeping as a ‘gateway’ experience for a broader rapprochement between urban residents and nature, and recognizing the political‐ecological context of beekeeping with respect to matters of socioecological justice. KW - environmental justice KW - honey bee KW - multispecies studies KW - policy KW - pollinator KW - urban greening Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-239949 VL - 3 IS - 3 SP - 550 EP - 559 ER - TY - JOUR A1 - Kriegel, Peter A1 - Fritze, Michael‐Andreas A1 - Thorn, Simon T1 - Surface temperature and shrub cover drive ground beetle (Coleoptera: Carabidae) assemblages in short‐rotation coppices JF - Agricultural and Forest Entomology N2 - Increasing demand for biomass has led to an on‐going intensification of fuel wood plantations with possible negative effects on open land biodiversity. Hence, ecologists increasingly call for measures that reduce those negative effects on associated biodiversity. However, our knowledge about the efficiency of such measures remains scarce. We investigated the effects of gap implementation in short rotation coppices (SRCs) on carabid diversity and assemblage composition over 3 years, with pitfall traps in gaps, edges and interiors. In parallel, we quantified soil surface temperature, shrub‐ and herb cover. Edges had the highest number of species and abundances per trap, whereas rarefied species richness was significantly lower in short rotation coppice interiors than in other habitat types. Carabid community composition differed significantly between habitat types. The main environmental drivers were temperature for number of species and abundance and shrub cover for rarefied species richness. We found significantly higher rarefied species richness in gaps compared with interiors. Hence, we argue that gap implementation benefits overall diversity in short rotation coppices. Furthermore, the differences in species community composition between habitat types through increased species turnover support carabid diversity in short rotation coppices. These positive effects were largely attributed to microclimate conditions. However, to maintain positive effects, continuous management of herb layer might be necessary. KW - Carabidae KW - fuel wood KW - short‐rotation coppice KW - shrub‐cover KW - temperature Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-239873 VL - 23 IS - 4 SP - 400 EP - 410 ER - TY - JOUR A1 - Sieger, Charlotte Sophie A1 - Hovestadt, Thomas T1 - The degree of spatial variation relative to temporal variation influences evolution of dispersal JF - Oikos N2 - In the face of ongoing global climate and land use change, organisms have multiple possibilities to cope with the modification of their environment. The two main possibilities are to either adapt locally or disperse to a more suitable habitat. The evolution of both local adaptation and dispersal interacts and can be influenced by the spatial and temporal variation (of e.g. temperature or precipitation). In an individual based model (IBM), we explore evolution of phenotypes in landscapes with varying degree of spatial relative to global temporal variation in order to examine its influence on the evolution of dispersal, niche optimum and niche width. The relationship between temporal and spatial variation did neither influence the evolution of local adaptation in the niche optimum nor of niche widths. Dispersal probability is highly influenced by the spatio‐temporal relationship: with increasing spatial variation, dispersal probability decreases. Additionally, the shape of the distribution of the trait values over patch attributes switches from hump‐ to U‐shaped. At low spatial variance more individuals emigrate from average habitats, at high spatial variance more from extreme habitats. The comparatively high dispersal probability in extreme patches of landscapes with a high spatial variation can be explained by evolutionary succession of two kinds of adaptive response. Early in the simulations, extreme patches in landscapes with a high spatial variability act as sink habitats, where population persistence depends on highly dispersive individuals with a wide niche. With ongoing evolution, local adaptation of the remaining individuals takes over, but simultaneously a possible bet‐hedging strategy promotes higher dispersal probabilities in those habitats. Here, in generations that experience extreme shifts from the temporal mean of the patch attribute, the expected fitness becomes higher for dispersing individuals than for philopatric individuals. This means that under certain circumstances, both local adaptation and high dispersal probability can be selected for for coping with the projected environmental changes in the future. KW - bet-hedging KW - dispersal KW - ecological niche KW - evolution KW - individual based model KW - spatial variation KW - temporal variation Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-239049 VL - 129 IS - 11 SP - 1611 EP - 1622 ER - TY - JOUR A1 - Wolf, Matthias T1 - How to teach about what is a species JF - Biology N2 - To ask students what a species is always has something rhetorical about it. Too quickly comes the rote answer, often learned by heart without ever thinking about it: “A species is a reproductive community of populations (reproductively isolated from others), which occupies a specific niche in nature” (Mayr 1982). However, do two people look alike because they are twins or are they twins because they look alike? “Two organisms do not belong to the same species because they mate and reproduce, but they only are able to do so because they belong to the same species” (Mahner and Bunge 1997). Unfortunately, most biology (pre-university) teachers have no opinion on whether species are real or conceptual, simply because they have never been taught the question themselves, but rather one answer they still pass on to their students today, learned by heart without ever thinking about it. Species are either real or conceptual and, in my opinion, it is this “or” that we should teach about. Only then can we discuss those fundamental questions such as who or what is selected, who or what evolves and, finally, what is biodiversity and phylogenetics all about? Individuals related to each other by the tree of life. KW - biospecies KW - species as individuals KW - species as natural kinds KW - species concept KW - species problem Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-241052 SN - 2079-7737 VL - 10 IS - 6 ER - TY - JOUR A1 - Kouhestani, Dina A1 - Geis, Maria A1 - Alsouri, Saed A1 - Bumm, Thomas G. P. A1 - Einsele, Hermann A1 - Sauer, Markus A1 - Stuhler, Gernot T1 - Variant signaling topology at the cancer cell–T-cell interface induced by a two-component T-cell engager JF - Cellular & Molecular Immunology N2 - No abstract available. KW - immunotherapy KW - tumour immunology Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-241189 VL - 18 ER - TY - JOUR A1 - Boff, Samuel A1 - Henrique, Jessica Amaral A1 - Friedel, Anna A1 - Raizer, Josué T1 - Disentangling the path of pollinator attraction in temporarily colored flowers JF - International Journal of Tropical Insect Science N2 - Plants may use different strategies to attract pollinators in long distance (e.g. floral display) and in short distance (e.g. ratio between differentially colored flowers) scales. The Verbenaceae Lantana canescens Kunth is a wide spread species in open sites of the Brazilian Pantanal wetland. Individuals of this generalist species can produce a variable number of open inflorescences with yellow and white flowers that are organized in whorls. In this study we tested the hypothesis that increased floral display (long distance attraction) and the ratio between yellow and white flowers (short distance attraction) enhances the number of pollinator species and individuals. We observed flower visitors and calculated floral parameters in 38 plots of 1 m2 each, that contained a varying number of flowering L. canescens individuals. Non-metric multidimensional scaling and Bray-Curtis distances were used to account for flower visitor composition and the relative visitation rate, respectively. We used a structural equation model to test the power of each predictor variable on the visitation rate and a covariance analysis to disentangle the effect of each independent variable on the frequency of plant-pollinator interactions. We found that the number of flower visitors and the visitation rate increased with increasing number of inflorescences. Disentangling long and short distance attraction indicated that the number of inflorescences (per plot) and the number of yellow flowers (yellowing effect) contributed most to flower visitation at long and short distance, respectively. KW - floral display KW - lantana canescens KW - pantanal wetland KW - honey bees KW - neotropical region KW - pollinator attraction Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-235402 VL - 41 ER - TY - JOUR A1 - Hutin, Stephanie A1 - Ling, Wai Li A1 - Tarbouriech, Nicolas A1 - Schoehn, Guy A1 - Grimm, Clemens A1 - Fischer, Utz A1 - Burmeister, Wim P. T1 - The vaccinia virus DNA helicase structure from combined single-particle cryo-electron microscopy and AlphaFold2 prediction JF - Viruses N2 - Poxviruses are large DNA viruses with a linear double-stranded DNA genome circularized at the extremities. The helicase-primase D5, composed of six identical 90 kDa subunits, is required for DNA replication. D5 consists of a primase fragment flexibly attached to the hexameric C-terminal polypeptide (res. 323–785) with confirmed nucleotide hydrolase and DNA-binding activity but an elusive helicase activity. We determined its structure by single-particle cryo-electron microscopy. It displays an AAA+ helicase core flanked by N- and C-terminal domains. Model building was greatly helped by the predicted structure of D5 using AlphaFold2. The 3.9 Å structure of the N-terminal domain forms a well-defined tight ring while the resolution decreases towards the C-terminus, still allowing the fit of the predicted structure. The N-terminal domain is partially present in papillomavirus E1 and polyomavirus LTA helicases, as well as in a bacteriophage NrS-1 helicase domain, which is also closely related to the AAA+ helicase domain of D5. Using the Pfam domain database, a D5_N domain followed by DUF5906 and Pox_D5 domains could be assigned to the cryo-EM structure, providing the first 3D structures for D5_N and Pox_D5 domains. The same domain organization has been identified in a family of putative helicases from large DNA viruses, bacteriophages, and selfish DNA elements. KW - DNA replication KW - helicase KW - Pfam domain KW - poxvirus KW - cryo-electron microscopy KW - structure prediction KW - SF3 helicase KW - orthopoxvirus KW - DNA helicase Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-290523 SN - 1999-4915 VL - 14 IS - 10 ER - TY - JOUR A1 - Mehmood, Rashid A1 - Alsaleh, Alanoud A1 - Want, Muzamil Y. A1 - Ahmad, Ijaz A1 - Siraj, Sami A1 - Ishtiaq, Muhammad A1 - Alshehri, Faizah A. A1 - Naseem, Muhammad A1 - Yasuhara, Noriko T1 - Integrative molecular analysis of DNA methylation dynamics unveils molecules with prognostic potential in breast cancer JF - BioMedInformatics N2 - DNA methylation acts as a major epigenetic modification in mammals, characterized by the transfer of a methyl group to a cytosine. DNA methylation plays a pivotal role in regulating normal development, and misregulation in cells leads to an abnormal phenotype as is seen in several cancers. Any mutations or expression anomalies of genes encoding regulators of DNA methylation may lead to abnormal expression of critical molecules. A comprehensive genomic study encompassing all the genes related to DNA methylation regulation in relation to breast cancer is lacking. We used genomic and transcriptomic datasets from the Cancer Genome Atlas (TGCA) Pan-Cancer Atlas, Genotype-Tissue Expression (GTEx) and microarray platforms and conducted in silico analysis of all the genes related to DNA methylation with respect to writing, reading and erasing this epigenetic mark. Analysis of mutations was conducted using cBioportal, while Xena and KMPlot were utilized for expression changes and patient survival, respectively. Our study identified multiple mutations in the genes encoding regulators of DNA methylation. The expression profiling of these showed significant differences between normal and disease tissues. Moreover, deregulated expression of some of the genes, namely DNMT3B, MBD1, MBD6, BAZ2B, ZBTB38, KLF4, TET2 and TDG, was correlated with patient prognosis. The current study, to our best knowledge, is the first to provide a comprehensive molecular and genetic profile of DNA methylation machinery genes in breast cancer and identifies DNA methylation machinery as an important determinant of the disease progression. The findings of this study will advance our understanding of the etiology of the disease and may serve to identify alternative targets for novel therapeutic strategies in cancer. KW - DNA methylation KW - epigenetic modification KW - breast cancer KW - genomics KW - in silico analysis Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-321171 SN - 2673-7426 VL - 3 IS - 2 SP - 434 EP - 445 ER - TY - JOUR A1 - Geiger, Nina A1 - Kersting, Louise A1 - Schlegel, Jan A1 - Stelz, Linda A1 - Fähr, Sofie A1 - Diesendorf, Viktoria A1 - Roll, Valeria A1 - Sostmann, Marie A1 - König, Eva-Maria A1 - Reinhard, Sebastian A1 - Brenner, Daniela A1 - Schneider-Schaulies, Sibylle A1 - Sauer, Markus A1 - Seibel, Jürgen A1 - Bodem, Jochen T1 - The acid ceramidase is a SARS-CoV-2 host factor JF - Cells N2 - SARS-CoV-2 variants such as the delta or omicron variants, with higher transmission rates, accelerated the global COVID-19 pandemic. Thus, novel therapeutic strategies need to be deployed. The inhibition of acid sphingomyelinase (ASM), interfering with viral entry by fluoxetine was reported. Here, we described the acid ceramidase as an additional target of fluoxetine. To discover these effects, we synthesized an ASM-independent fluoxetine derivative, AKS466. High-resolution SARS-CoV-2–RNA FISH and RTqPCR analyses demonstrate that AKS466 down-regulates viral gene expression. It is shown that SARS-CoV-2 deacidifies the lysosomal pH using the ORF3 protein. However, treatment with AKS488 or fluoxetine lowers the lysosomal pH. Our biochemical results show that AKS466 localizes to the endo-lysosomal replication compartments of infected cells, and demonstrate the enrichment of the viral genomic, minus-stranded RNA and mRNAs there. Both fluoxetine and AKS466 inhibit the acid ceramidase activity, cause endo-lysosomal ceramide elevation, and interfere with viral replication. Furthermore, Ceranib-2, a specific acid ceramidase inhibitor, reduces SARS-CoV-2 replication and, most importantly, the exogenous supplementation of C6-ceramide interferes with viral replication. These results support the hypotheses that the acid ceramidase is a SARS-CoV-2 host factor. KW - SARS-CoV-2 KW - ceramides KW - ceramidase KW - fluoxetine KW - acid sphingomyelinase Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-286105 SN - 2073-4409 VL - 11 IS - 16 ER - TY - JOUR A1 - Floren, Andreas A1 - Linsenmair, Karl Eduard A1 - Müller, Tobias T1 - Diversity and functional relevance of canopy arthropods in Central Europe JF - Diversity N2 - Although much is known about the ecology and functional importance of canopy arthropods in temperate forests, few studies have tried to assess the overall diversity and investigate the composition and dynamics of tree-specific communities. This has impeded a deeper understanding of the functioning of forests, and of how to maintain system services. Here, we present the first comprehensive data of whole arthropod communities, collected by insecticidal knockdown (fogging) from 1159 trees in 18 study areas in Central Europe during the last 25 years. The data includes 3,253,591 arthropods from 32 taxa (order, suborder, family) collected on 24 tree species from 18 genera. Fogging collects free-living, ectophytic arthropods in approximately the same number as they occur in the trees. To our knowledge, these are the most comprehensive data available today on the taxonomic composition of arboreal fauna. Assigning all arthropods to their feeding guild provided a proxy of their functional importance. The data showed that the canopy communities were regularly structured, with a clear dominance hierarchy comprised of eight ‘major taxa’ that represented 87% of all arthropods. Despite significant differences in the proportions of taxa on deciduous and coniferous trees, the composition of the guilds was very similar. The individual tree genera, on the other hand, showed significant differences in guild composition, especially when different study areas and years were compared, whereas tree-specific traits, such as tree height, girth in breast height or leaf cover, explained little of the overall variance. On the ordinal level, guild composition also differed significantly between managed and primary forests, with a simultaneous low within-group variability, indicating that management is a key factor determining the distribution of biodiversity and guild composition. KW - temperate forests KW - insecticidal knockdown KW - community structure KW - functional diversity KW - guild constancy KW - forest management KW - pristine forests KW - Bialowieza Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-285924 SN - 1424-2818 VL - 14 IS - 8 ER - TY - JOUR A1 - Rohmer, Carina A1 - Dobritz, Ronja A1 - Tuncbilek-Dere, Dilek A1 - Lehmann, Esther A1 - Gerlach, David A1 - George, Shilpa Elizabeth A1 - Bae, Taeok A1 - Nieselt, Kay A1 - Wolz, Christiane T1 - Influence of Staphylococcus aureus strain background on Sa3int phage life cycle switches JF - Viruses N2 - Staphylococcus aureus asymptomatically colonizes the nasal cavity of mammals, but it is also a leading cause of life-threatening infections. Most human nasal isolates carry Sa3 phages, which integrate into the bacterial hlb gene encoding a sphingomyelinase. The virulence factor-encoding genes carried by the Sa3-phages are highly human-specific, and most animal strains are Sa3 negative. Thus, both insertion and excision of the prophage could potentially confer a fitness advantage to S. aureus. Here, we analyzed the phage life cycle of two Sa3 phages, Φ13 and ΦN315, in different phage-cured S. aureus strains. Based on phage transfer experiments, strains could be classified into low (8325-4, SH1000, and USA300c) and high (MW2c and Newman-c) transfer strains. High-transfer strains promoted the replication of phages, whereas phage adsorption, integration, excision, or recA transcription was not significantly different between strains. RNASeq analyses of replication-deficient lysogens revealed no strain-specific differences in the CI/Mor regulatory switch. However, lytic genes were significantly upregulated in the high transfer strain MW2c Φ13 compared to strain 8325-4 Φ13. By transcriptional start site prediction, new promoter regions within the lytic modules were identified, which are likely targeted by specific host factors. Such host-phage interaction probably accounts for the strain-specific differences in phage replication and transfer frequency. Thus, the genetic makeup of the host strains may determine the rate of phage mobilization, a feature that might impact the speed at which certain strains can achieve host adaptation. KW - phage KW - virulence KW - induction KW - gene regulation KW - Staphylococcus KW - hemolysin Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-297209 SN - 1999-4915 VL - 14 IS - 11 ER - TY - JOUR A1 - Köhler, Franziska A1 - Reese, Lena A1 - Hendricks, Anne A1 - Kastner, Carolin A1 - Müller, Sophie A1 - Lock, Johan F. A1 - Germer, Christoph-Thomas A1 - Wiegering, Armin T1 - Low-grade mucinous neoplasms (LAMN) of the appendix in Germany between 2011 and 2018: a nationwide analysis based on data provided by the German Center for Cancer Registry Data (ZfKD) at the Robert Koch Institute (RKI) JF - Langenbeck’s Archives of Surgery N2 - Introduction Low-grade appendiceal mucinous neoplasms (LAMN) are semi-malignant tumors of the appendix which are incidentally found in up to 1% of appendectomy specimen. To this day, no valid descriptive analysis on LAMN is available for the German population. Methods Data of LAMN (ICD-10: D37.3) were collected from the population-based cancer registries in Germany, provided by the German Center for Cancer Registry Data (Zentrum für Krebsregisterdaten—ZfKD). Data was anonymized and included gender, age at diagnosis, tumor staging according to the TNM-classification, state of residence, information on the performed therapy, and survival data. Results A total of 612 cases were reported to the ZfKD between 2011 and 2018. A total of 63.07% were female and 36.93% were male. Great inhomogeneity in reporting cases was seen in the federal states of Germany including the fact that some federal states did not report any cases at all. Age distribution showed a mean age of 62.03 years (SD 16.15) at diagnosis. However, data on tumor stage was only available in 24.86% of cases (n = 152). A total of 49.34% of these patients presented with a T4-stage. Likewise, information regarding performed therapy was available in the minority of patients: 269 patients received surgery, 22 did not and for 312 cases no information was available. Twenty-four patients received chemotherapy, 188 did not, and for 400 cases, no information was available. Overall 5-year survival was estimated at 79.52%. Patients below the age of 55 years at time of diagnosis had a significantly higher 5-year survival rate compared to patients above the age of 55 years (85.77% vs. 73.27%). Discussion In this study, we observed an incidence of LAMN in 0.13% of all appendectomy specimen in 2018. It seems likely that not all cases were reported to the ZfKD; therefore, case numbers may be considered underestimated. Age and gender distribution goes in line with international studies with females being predominantly affected. Especially regarding tumor stage and therapy in depth information cannot be provided through the ZfKD-database. This data analysis emphasizes the need for further studies and the need for setting up a specialized registry for this unique tumor entity to develop guidelines for the appropriate treatment and follow-up. KW - LAMN KW - low-grade mucinous neoplasm KW - appendix KW - epidemiology KW - ZfKD KW - Germany Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-323919 VL - 407 IS - 8 ER - TY - JOUR A1 - Brosch, Philippa K. A1 - Korsa, Tessa A1 - Taban, Danush A1 - Eiring, Patrick A1 - Hildebrand, Sascha A1 - Neubauer, Julia A1 - Zimmermann, Heiko A1 - Sauer, Markus A1 - Shirakashi, Ryo A1 - Djuzenova, Cholpon S. A1 - Sisario, Dmitri A1 - Sukhorukov, Vladimir L. T1 - Glucose and inositol transporters, SLC5A1 and SLC5A3, in glioblastoma cell migration JF - Cancers N2 - (1) Background: The recurrence of glioblastoma multiforme (GBM) is mainly due to invasion of the surrounding brain tissue, where organic solutes, including glucose and inositol, are abundant. Invasive cell migration has been linked to the aberrant expression of transmembrane solute-linked carriers (SLC). Here, we explore the role of glucose (SLC5A1) and inositol transporters (SLC5A3) in GBM cell migration. (2) Methods: Using immunofluorescence microscopy, we visualized the subcellular localization of SLC5A1 and SLC5A3 in two highly motile human GBM cell lines. We also employed wound-healing assays to examine the effect of SLC inhibition on GBM cell migration and examined the chemotactic potential of inositol. (3) Results: While GBM cell migration was significantly increased by extracellular inositol and glucose, it was strongly impaired by SLC transporter inhibition. In the GBM cell monolayers, both SLCs were exclusively detected in the migrating cells at the monolayer edge. In single GBM cells, both transporters were primarily localized at the leading edge of the lamellipodium. Interestingly, in GBM cells migrating via blebbing, SLC5A1 and SLC5A3 were predominantly detected in nascent and mature blebs, respectively. (4) Conclusion: We provide several lines of evidence for the involvement of SLC5A1 and SLC5A3 in GBM cell migration, thereby complementing the migration-associated transportome. Our findings suggest that SLC inhibition is a promising approach to GBM treatment. KW - volume regulation KW - transportome KW - phlorizin Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-297498 SN - 2072-6694 VL - 14 IS - 23 ER - TY - THES A1 - Schmalz, Fabian Dominik T1 - Processing of behaviorally relevant stimuli at different levels in the bee brain T1 - Die Verarbeitung verhaltensrelevanter Stimuli auf unterschiedlichen Ebenen im Bienengehirn N2 - The behavior of honeybees and bumblebees relies on a constant sensory integration of abiotic or biotic stimuli. As eusocial insects, a sophisticated intraspecific communication as well as the processing of multisensory cues during foraging is of utter importance. To tackle the arising challenges, both honeybees and bumblebees have evolved a sophisticated olfactory and visual processing system. In both organisms, olfactory reception starts at the antennae, where olfactory sensilla cover the antennal surface in a sex-specific manner. These sensilla house olfactory receptor neurons (ORN) that express olfactory receptors. ORNs send their axons via four tracts to the antennal lobe (AL), the prime olfactory processing center in the bee brain. Here, ORNs specifically innervate spheroidal structures, so-called glomeruli, in which they form synapses with local interneurons and projection neurons (PN). PNs subsequently project the olfactory information via two distinct tracts, the medial and the lateral antennal-lobe tract, to the mushroom body (MB), the main center of sensory integration and memory formation. In the honeybee calyx, the sensory input region of the MB, PNs synapse on Kenyon cells (KC), the principal neuron type of the MB. Olfactory PNs mainly innervate the lip and basal ring layer of the calyx. In addition, the basal ring receives input from visual PNs, making it the first site of integration of visual and olfactory information. Visual PNs, carrying sensory information from the optic lobes, send their terminals not only to the to the basal ring compartment but also to the collar of the calyx. Receiving olfactory or visual input, KCs send their axons along the MB peduncle and terminate in the main output regions of the MB, the medial and the vertical lobe (VL) in a layer-specific manner. In the MB lobes, KCs synapse onto mushroom body output neurons (MBON). In so far barely understood processes, multimodal information is integrated by the MBONs and then relayed further into the protocerebral lobes, the contralateral brain hemisphere, or the central brain among others. This dissertation comprises a dichotomous structure that (i) aims to gain more insight into the olfactory processing in bumblebees and (ii) sets out to broaden our understanding of visual processing in honeybee MBONs. The first manuscript examines the olfactory processing of Bombus terrestris and specifically investigates sex-specific differences. We used behavioral (absolute conditioning) and electrophysiological approaches to elaborate the processing of ecologically relevant odors (components of plant odors and pheromones) at three distinct levels, in the periphery, in the AL and during olfactory conditioning. We found both sexes to form robust memories after absolute conditioning and to generalize towards the carbon chain length of the presented odors. On the contrary, electroantennographic (EAG) activity showed distinct stimulus and sex-specific activity, e.g. reduced activity towards citronellol in drones. Interestingly, extracellular multi-unit recordings in the AL confirmed stimulus and sex-specific differences in olfactory processing, but did not reflect the differences previously found in the EAG. Here, farnesol and 2,3-dihydrofarnesol, components of sex-specific pheromones, show a distinct representation, especially in workers, corroborating the results of a previous study. This explicitly different representation suggests that the peripheral stimulus representation is an imperfect indication for neuronal representation in high-order neuropils and ecological importance of a specific odor. The second manuscript investigates MBONs in honeybees to gain more insights into visual processing in the VL. Honeybee MBONs can be categorized into visually responsive, olfactory responsive and multimodal. To clarify which visual features are represented at this high-order integration center, we used extracellular multi-unit recordings in combination with visual and olfactory stimulation. We show for the first time that information about brightness and wavelength is preserved in the VL. Furthermore, we defined three specific classes of visual MBONs that distinctly encode the intensity, identity or simply the onset of a stimulus. The identity-subgroup exhibits a specific tuning towards UV light. These results support the view of the MB as the center of multimodal integration that categorizes sensory input and subsequently channels this information into specific MBON populations. Finally, I discuss differences between the peripheral representations of stimuli and their distinct processing in high-order neuropils. The unique activity of farnesol in manuscript 1 or the representation of UV light in manuscript 2 suggest that the peripheral representation of a stimulus is insufficient as a sole indicator for its neural activity in subsequent neuropils or its putative behavioral importance. In addition, I discuss the influence of hard-wired concepts or plasticity induced changes in the sensory pathways on the processing of such key stimuli in the peripheral reception as well as in high-order centers like the AL or the MB. The MB as the center of multisensory integration has been broadly examined for its olfactory processing capabilities and receives increasing interest about its visual coding properties. To further unravel its role of sensory integration and to include neglected modalities, future studies need to combine additional approaches and gain more insights on the multimodal aspects in both the input and output region. N2 - Honigbienen und Hummeln sind aufgrund ihrer Lebensweise auf die ständige Verarbeitung sensorischer Eindrücke abiotischen und biotischen Ursprungs angewiesen. Als eusoziale Insekten ist hierbei für beide Arten die Wahrnehmung innerartlicher Kommunikation wie auch die Verarbeitung multisensorischer Einflüsse während der Nahrungssuche von essenzieller Bedeutung. Um die daraus resultierenden vielfältigen Herausforderungen erfolgreich bewältigen zu können, verfügen Honigbienen und Hummeln über eine fortschrittliche Verarbeitung olfaktorischer und visueller Reize. In beiden Arten beginnt die Geruchsrezeption an den Antennen, welche geschlechtsspezifisch von zahlreichen olfaktorischen Sensillen besetzt sind. Diese beinhalten olfaktorische Rezeptorneurone (ORN), in welchen die Expression der Geruchsrezeptoren stattfindet. Axone der ORNs laufen dabei gebündelt über vier verschiedene Trakte in den Antennallobus (AL), das erste olfaktorische Verarbeitungszentrum im Bienengehirn. Im AL verschalten ORNs mit lokalen Interneuronen und Projektionsneuronen (PN) in kugelförmigen Strukturen, den sogenannten Glomeruli. PNs leiten die olfaktorische Information daraufhin über zwei charakteristische Trakte, den medialen und lateralen Antennallobustrakt, in den Pilzkörper (MB), das Verarbeitungszentrum für die Integration sensorischer Eindrücke und Gedächtnisbildung. Im Calyx der Honigbiene, der sensorischen Eingangsregion des MB, bilden die Endköpfchen der PNs synaptische Verbindungen mit Kenyonzellen (KC), den primären Nervenzellen im MB. Die Innervation des Calyx durch die PNs ist dabei spezifisch in drei verschiedenen Zonen organisiert, nämlich in Lippe, Hals und basalen Ring. Während die Lippe vornehmlich olfaktorische Information von PNs aus dem AL erhält, wird der basale Ring zusätzlich auch von visuellen PNs, welche Informationen aus dem optischen Lobus einbringen, angesteuert. Der basale Ring der Honigbiene wird dabei Ort der ersten räumlichen Integration visuellen und olfaktorischen Eingangs. Wiederum ähnlich zum unimodalen Eingang der Lippe, bezieht auch der Hals des Calyx grundsätzlich nur sensorischen Eingang einer Modalität, nämlich visuelle Information von PNs aus dem optischen Lobus. KCs verschalten im weiteren Verlauf die olfaktorischen und visuellen Informationen an Pilzkörperausgangsneurone (MBON). In einem bisher kaum erforschten Vorgang wird diese multimodale Information dabei verarbeitet und dann mithilfe der MBONs in verschiedene Bereiche des Gehirns geleitet, z.B. in die protocerebralen Loben, die kontralaterale Gehirnhemisphäre oder das Zentralgehirn. Diese Dissertation ist zweigeteilt und behandelt zuerst (i) die geschlechtsspezifische Verarbeitung olfaktorischer Reize in Hummeln und bespricht im zweiten Teil (ii) neue Einblicke in die neuronale Weiterverarbeitung visueller Reize durch MBONs in der Honigbiene. Manuskript 1 untersucht die Abläufe der Geruchsverarbeitung von Bombus terrestris und beschreibt geschlechtsspezifische Unterschiede. Hierbei wurden sowohl verhaltensbasierte als auch elektrophysiologische Methoden genutzt um die Wahrnehmung ökologisch relevanter Duftstoffe (Komponenten unterschiedlicher Pflanzendüfte oder Pheromone) auf drei verschiedene Weisen zu untersuchen, nämlich in der Peripherie, im AL und mittels olfaktorischer Konditionierung. Wir fanden in beiden Geschlechtern eine robuste Gedächtnisbildung nach absoluter Konditionierung und eine ausgeprägte Generalisierung anhand der Kohlenstoffkettenlänge der präsentierten Duftstoffe. Anders stellten sich die Ergebnisse der elektroantennographischen (EAG) Untersuchungen dar. Hier zeigten sowohl Drohnen als auch Arbeiterinnen neuronale Aktivität mit spezifischen Unterschieden zwischen den Stimuli, aber auch zwischen den Geschlechtern auf, z.B. löste die Applikation von Citronellol eine deutliche verringerte Reaktion in der EAG Aktivität der Drohnen aus. Interessanterweise zeigten auch extrazelluläre Ableitungen im AL stimulus- und geschlechtsspezifische Unterschiede, jedoch in unterschiedlicher Konstellation als in den EAG-Experimenten. Besonders Farnesol und 2,3-Dihydrofarnesol wiesen vor allem bei Arbeiterinnen eine deutliche Repräsentation in der neuronalen Aktivität auf; ein Alleinstellungsmerkmal welches für Farnesol bereits in einer früheren Studie beschrieben wurde. Diese explizit unterschiedliche neuronale Darstellung von Farnesol und 2,3-Dihydrofarnesol in der Peripherie und im AL führt zu der Annahme, dass die rezeptive Darstellung eines Stimulus in der Peripherie keine zuverlässigen Rückschlüsse über die neuronale Repräsentation in höheren Zentren oder die ökologische Relevanz zulässt. Im zweiten Manuskript stehen MBONs der Honigbiene im Fokus, um mehr Einblicke in die visuelle Verarbeitung im VL zu erlangen. Bisher können MBONs in folgende Klassen unterteilt werden: Visuelle, olfaktorische und multimodale MBONs, welche sensitiv für beide Modalitäten sind. Kern dieser Arbeit ist, mittels extrazellulärer Ableitungen festzustellen, welche zusätzlichen Aspekte eines visuellen Stimulus in diesem zentralen Verarbeitungszentrum repräsentiert sind. Dabei konnte zum ersten Mal gezeigt werden, dass Informationen über die Wellenlänge und die Intensität des Lichtstimulus im VL erhalten sind. Im weiteren Verlauf konnte eine Spezifizierung der bisherigen Kategorisierung visueller und multimodaler MBONs in drei weitere Untergruppen vollzogen werden: MBONs die spezifisch die Intensität, die Identität und dein Eingang eines Stimulus kodieren. Des Weiteren zeigte vor allem die Gruppe der Identitäts-MBONs eine bemerkenswerte Kategorisierung von UV-Licht. Diese neuen Erkenntnisse bestätigen die Ansicht, dass der MB, als Zentrum für sensorische Integration, eine Kategorisierung der verarbeiteten Eindrücke vornimmt und diese daraufhin auf die MBONs verschalten wird. Abschließend diskutiere ich Unterschiede in der peripheren Repräsentation von Stimuli und ihrer späteren neuronalen Verarbeitung. Hier zeige ich, die Aktivität von Farnesol in MS1 und UV-Licht MS2 als Beispiel nehmend, dass die periphere Repräsentation eines Stimulus keine sicheren Schlussfolgerungen über die nachfolgend induzierte neurale Aktivität oder die verhaltensrelevante Bedeutung zulässt. Im weiteren Verlauf werden dabei die Einflüsse konservierter Strukturen und plastischer Änderungen auf die Abläufe der sensorischen Peripherie oder der höheren Verarbeitungszentren, wie dem AL oder dem MB gezeigt. Obwohl der MB, das Zentrum für multimodale Integration und Gedächtnis, hinsichtlich seiner Rolle in der Geruchswahrnehmung ausgiebig erforscht ist, gibt es bezüglich der visuellen Verarbeitung oder dem Einfluss anderer Modalitäten noch ungeklärte Abläufe und Fragen. Wenngleich auch hier die Kenntnis speziell über die visuelle Verarbeitung im MB stetig zunimmt, sollten zukünftige Arbeiten mithilfe weiterer Methoden den MB Eingang und Ausgang explizit auf den Einfluss weiterer Modalitäten untersuchen, um so ein umfassenderes Bild über die Abläufe multimodaler Integration zu erhalten. KW - Biene KW - Elektrophysiologie KW - bee KW - electrophysiology KW - olfaction KW - vision KW - multi-unit recording KW - Olfaktorik KW - Sehen KW - Multi-Unit Aufnahmen Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-288824 ER - TY - JOUR A1 - Aupperle-Lellbach, Heike A1 - Heidrich, Daniela A1 - Kehl, Alexandra A1 - Conrad, David A1 - Brockmann, Maria A1 - Törner, Katrin A1 - Beitzinger, Christoph A1 - Müller, Tobias T1 - KITLG copy number germline variations in schnauzer breeds and their relevance in digital squamous cell carcinoma in black giant schnauzers JF - Veterinary Sciences N2 - Copy number variations (CNVs) of the KITLG gene seem to be involved in the oncogenesis of digital squamous cell carcinoma (dSCC). The aims of this study were (1) to investigate KITLG CNV in giant (GS), standard (SS), and miniature (MS) schnauzers and (2) to compare KITLG CNV between black GS with and without dSCC. Blood samples from black GS (22 with and 17 without dSCC), black SS (18 with and 4 without dSSC; 5 unknown), and 50 MS (unknown dSSC status and coat colour) were analysed by digital droplet PCR. The results are that (1) most dogs had a copy number (CN) value > 4 (range 2.5–7.6) with no significant differences between GS, SS, and MS, and (2) the CN value in black GS with dSCC was significantly higher than in those without dSCC (p = 0.02). CN values > 5.8 indicate a significantly increased risk for dSCC, while CN values < 4.7 suggest a reduced risk for dSCC (grey area: 4.7–5.8). Diagnostic testing for KITLG CNV may sensitise owners to the individual risk of their black GS for dSCC. Further studies should investigate the relevance of KITLG CNV in SS and the protective effects in MS, who rarely suffer from dSCC. KW - tumour KW - toe KW - miniature schnauzer KW - standard schnauzer KW - CNV KW - ddPCR KW - breed predisposition Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-303913 SN - 2306-7381 VL - 10 IS - 2 ER - TY - JOUR A1 - de Paz, Víctor A1 - Asís, Josep D. A1 - Holzschuh, Andrea A1 - Baños-Picón, Laura T1 - Effects of traditional orchard abandonment and landscape context on the beneficial arthropod community in a Mediterranean agroecosystem JF - Insects N2 - Agricultural abandonment is one of the main land-use changes in Europe, and its consequences on biodiversity are context- and taxa-dependent. While several studies have worked on this topic, few have focused on traditional orchards, especially in different landscapes and under a Mediterranean climate. In this context, we aimed to determine the effects of almond orchard abandonment on the communities of three groups of beneficial arthropods and the role of the landscape context in modulating these effects. Between February and September 2019, four samplings were carried out in twelve almond orchards (three abandoned and three traditional (active orchards under traditional agricultural management) located in simple landscapes as well as three abandoned and three traditional in complex landscapes). Abandoned and traditional almond orchards harbor different arthropod communities and diversity metrics that are strongly conditioned by seasonality. Abandoned orchards can favor pollinators and natural enemies, providing alternative resources in simple landscapes. However, the role that abandoned orchards play in simple landscapes disappears as the percentage of semi-natural habitats in the landscape increases. Our results show that landscape simplification, through the loss of semi-natural habitats, has negative consequences on arthropod biodiversity, even in traditional farming landscapes with small fields and high crop diversity. KW - abandonment KW - traditional almond orchard KW - spider KW - parasitoid KW - bee KW - landscape complexity Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-311190 SN - 2075-4450 VL - 14 IS - 3 ER - TY - JOUR A1 - Wersebeckmann, Vera A1 - Biegerl, Carolin A1 - Leyer, Ilona A1 - Mody, Karsten T1 - Orthopteran diversity in steep slope vineyards: the role of vineyard type and vegetation management JF - Insects N2 - The abandonment of traditional agricultural practices and subsequent succession are major threats to many open-adapted species and species-rich ecosystems. Viticulture on steep slopes has recently suffered from strong declines due to insufficient profitability, thus increasing the area of fallow land considerably. Changing cultivation systems from vertically oriented to modern vineyard terraces offers an opportunity to maintain management economically viable and thus reduces further abandonment. Hillside parallel terraces favor mechanization, and their embankments offer large undisturbed areas that could provide valuable habitats. We investigated the effects of vineyard abandonment, different vineyard management types (vertically oriented vs. terraced), and local parameters on Orthoptera diversity in 45 study sites along the Upper Middle Rhine Valley in Germany. Our results show that woody structures and vineyard abandonment reduced Orthoptera diversity at the local and landscape scale due to decreased habitat quality, especially for open-adapted species. In contrast, open inter-rows of actively managed vineyard types supported heat-adapted Caelifera species. On terrace embankments, extensive management and taller vegetation benefited Ensifera species, while short and mulched vegetation in vertically oriented vineyards favored the dominance of one single Caelifera species. Our results highlight the significance of maintaining viticultural management on steep slopes for the preservation of both open-adapted Orthoptera species and the cultural landscape. KW - abandonment KW - alternating management KW - biodiversity conservation KW - grasshopper KW - insect conservation KW - succession KW - traditional land use KW - vineyard terrace Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-304891 SN - 2075-4450 VL - 14 IS - 1 ER - TY - JOUR A1 - Dong, Meng A1 - Böpple, Kathrin A1 - Thiel, Julia A1 - Winkler, Bernd A1 - Liang, Chunguang A1 - Schueler, Julia A1 - Davies, Emma J. A1 - Barry, Simon T. A1 - Metsalu, Tauno A1 - Mürdter, Thomas E. A1 - Sauer, Georg A1 - Ott, German A1 - Schwab, Matthias A1 - Aulitzky, Walter E. T1 - Perfusion air culture of precision-cut tumor slices: an ex vivo system to evaluate individual drug response under controlled culture conditions JF - Cells N2 - Precision-cut tumor slices (PCTS) maintain tissue heterogeneity concerning different cell types and preserve the tumor microenvironment (TME). Typically, PCTS are cultured statically on a filter support at an air–liquid interface, which gives rise to intra-slice gradients during culture. To overcome this problem, we developed a perfusion air culture (PAC) system that can provide a continuous and controlled oxygen medium, and drug supply. This makes it an adaptable ex vivo system for evaluating drug responses in a tissue-specific microenvironment. PCTS from mouse xenografts (MCF-7, H1437) and primary human ovarian tumors (primary OV) cultured in the PAC system maintained the morphology, proliferation, and TME for more than 7 days, and no intra-slice gradients were observed. Cultured PCTS were analyzed for DNA damage, apoptosis, and transcriptional biomarkers for the cellular stress response. For the primary OV slices, cisplatin treatment induced a diverse increase in the cleavage of caspase-3 and PD-L1 expression, indicating a heterogeneous response to drug treatment between patients. Immune cells were preserved throughout the culturing period, indicating that immune therapy can be analyzed. The novel PAC system is suitable for assessing individual drug responses and can thus be used as a preclinical model to predict in vivo therapy responses. KW - precision-cut tumor slices KW - perfusion culture KW - tumor microenvironment KW - ovarian tumor KW - individual drug responses KW - mouse xenografts KW - preclinical model KW - personalized medicine Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-311030 SN - 2073-4409 VL - 12 IS - 5 ER - TY - JOUR A1 - Cerezo-Echevarria, Argiñe A1 - Kehl, Alexandra A1 - Beitzinger, Christoph A1 - Müller, Tobias A1 - Klopfleisch, Robert A1 - Aupperle-Lellbach, Heike T1 - Evaluating the histologic grade of digital squamous cell carcinomas in dogs and copy number variation of KIT Ligand — a correlation study JF - Veterinary Sciences N2 - Dark-haired dogs are predisposed to the development of digital squamous cell carcinoma (DSCC). This may potentially suggest an underlying genetic predisposition not yet completely elucidated. Some authors have suggested a potential correlation between the number of copies KIT Ligand (KITLG) and the predisposition of dogs to DSCC, containing a higher number of copies in those affected by the neoplasm. In this study, the aim was to evaluate a potential correlation between the number of copies of the KITLG and the histological grade of malignancy in dogs with DSCC. For this, 72 paraffin-embedded DSCCs with paired whole blood samples of 70 different dogs were included and grouped according to their haircoat color as follow: Group 0/unknown haircoat color (n = 11); Group 1.a/black non-Schnauzers (n = 15); group 1.b/black Schnauzers (n = 33); group 1.c/black and tan dogs (n = 7); group 2/tan animals (n = 4). The DSCCs were histologically graded. Additionally, KITLG Copy Number Variation (CNV) was determined by ddPCR. A significant correlation was observed between KITLG copy number and the histological grade and score value. This finding may suggest a possible factor for the development of canine DSCC, thus potentially having an impact on personalized veterinary oncological strategies and breeding programs. KW - canine KW - cancer KW - toe KW - grading KW - haircoat KW - color KW - genetics KW - gene Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-304824 SN - 2306-7381 VL - 10 IS - 2 ER - TY - THES A1 - Reuter, Christian Steffen T1 - Development of a tissue-engineered primary human skin infection model to study the pathogenesis of tsetse fly-transmitted African trypanosomes in mammalian skin T1 - Entwicklung eines primären humanen Hautinfektionsmodells basierend auf Gewebezüchtung zur Erforschung der Pathogenese von Tsetsefliegen-übertragenen Afrikanischen Trypanosomen in der Säugetierhaut N2 - Many arthropods such as mosquitoes, ticks, bugs, and flies are vectors for the transmission of pathogenic parasites, bacteria, and viruses. Among these, the unicellular parasite Trypanosoma brucei (T. brucei) causes human and animal African trypanosomiases and is transmitted to the vertebrate host by the tsetse fly. In the fly, the parasite goes through a complex developmental cycle in the alimentary tract and salivary glands ending with the cellular differentiation into the metacyclic life cycle stage. An infection in the mammalian host begins when the fly takes a bloodmeal, thereby depositing the metacyclic form into the dermal skin layer. Within the dermis, the cell cycle-arrested metacyclic forms are activated, re-enter the cell cycle, and differentiate into proliferative trypanosomes, prior to dissemination throughout the host. Although T. brucei has been studied for decades, very little is known about the early events in the skin prior to systemic dissemination. The precise timing and the mechanisms controlling differentiation of the parasite in the skin continue to be elusive, as does the characterization of the proliferative skin-residing trypanosomes. Understanding the first steps of an infection is crucial for developing novel strategies to prevent disease establishment and its progression. A major shortcoming in the study of human African trypanosomiasis is the lack of suitable infection models that authentically mimic disease progression. In addition, the production of infectious metacyclic parasites requires tsetse flies, which are challenging to keep. Thus, although animal models - typically murine - have produced many insights into the pathogenicity of trypanosomes in the mammalian host, they were usually infected by needle injection into the peritoneal cavity or tail vein, bypassing the skin as the first entry point. Furthermore, animal models are not always predictive for the infection outcome in human patients. In addition, the relatively small number of metacyclic parasites deposited by the tsetse flies makes them difficult to trace, isolate, and study in animal hosts. The focus of this thesis was to develop and validate a reconstructed human skin equivalent as an infection model to study the development of naturally-transmitted metacyclic parasites of T. brucei in mammalian skin. The first part of this work describes the development and characterization of a primary human skin equivalent with improved mechanical properties. To achieve this, a computer-assisted compression system was designed and established. This system allowed the improvement of the mechanical stability of twelve collagen-based dermal equivalents in parallel through plastic compression, as evaluated by rheology. The improved dermal equivalents provided the basis for the generation of the skin equivalents and reduced their contraction and weight loss during tissue formation, achieving a high degree of standardization and reproducibility. The skin equivalents were characterized using immunohistochemical and histological techniques and recapitulated key anatomical, cellular, and functional aspects of native human skin. Furthermore, their cellular heterogeneity was examined using single-cell RNA sequencing - an approach which led to the identification of a remarkable repertoire of extracellular matrix-associated genes expressed by different cell subpopulations in the artificial skin. In addition, experimental conditions were established to allow tsetse flies to naturally infect the skin equivalents with trypanosomes. In the second part of the project, the development of the trypanosomes in the artificial skin was investigated in detail. This included the establishment of methods to successfully isolate skin-dwelling trypanosomes to determine their protein synthesis rate, cell cycle and metabolic status, morphology, and transcriptome. Microscopy techniques to study trypanosome motility and migration in the skin were also optimized. Upon deposition in the artificial skin by feeding tsetse, the metacyclic parasites were rapidly activated and established a proliferative population within one day. This process was accompanied by: (I) reactivation of protein synthesis; (II) re-entry into the cell cycle; (III) change in morphology; (IV) increased motility. Furthermore, these observations were linked to potentially underlying developmental mechanisms by applying single-cell parasite RNA sequencing at five different timepoints post-infection. After the initial proliferative phase, the tsetse-transmitted trypanosomes appeared to enter a reversible quiescence program in the skin. These quiescent skin-residing trypanosomes were characterized by very slow replication, a strongly reduced metabolism, and a transcriptome markedly different from that of the deposited metacyclic forms and the early proliferative trypanosomes. By mimicking the migration from the skin to the bloodstream, the quiescent phenotype could be reversed and the parasites returned to an active proliferating state. Given that previous work has identified the skin as an anatomical reservoir for T. brucei during disease, it is reasonable to assume that the quiescence program is an authentic facet of the parasite's behavior in an infected host. In summary, this work demonstrates that primary human skin equivalents offer a new and promising way to study vector-borne parasites under close-to-natural conditions as an alternative to animal experimentation. By choosing the natural transmission route - the bite of an infected tsetse fly - the early events of trypanosome infection have been detailed with unprecedented resolution. In addition, the evidence here for a quiescent, skin-residing trypanosome population may explain the persistence of T. brucei in the skin of aparasitemic and asymptomatic individuals. This could play an important role in maintaining an infection over long time periods. N2 - Zahlreiche Arthropoden wie Stechmücken, Zecken, Wanzen und Fliegen sind Überträger für krankheitserregende Parasiten, Bakterien und Viren. Hierzu gehört der einzellige Parasit Trypanosoma brucei (T. brucei), welcher durch Tsetsefliegen übertragen wird und die Afrikanische Trypanosomiasis bei Menschen und Tieren verursacht. Der Entwicklungszyklus des Parasiten in der Fliege ist komplex und endet in der Speicheldrüse mit der Differenzierung in das metazyklische Lebensstadium. Diese metazyklischen Formen werden durch den Biss der blutsaugenden Tsetsefliege in die dermale Hautschicht des Säugetierwirts injiziert. Die zellzyklusarretierten metazyklischen Formen werden in der Dermis aktiviert und der Widereintritt in den Zellzyklus sowie die Differenzierung zu proliferativen Trypanosomen eingeleitet. Anschließend breitet sich der Parasit systemisch im Säugetierwirt aus. Obwohl T. brucei bereits seit Jahrzehnten erforscht wird, ist nur sehr wenig über das frühe Infektionsgeschehen in der Haut bekannt. Der genaue Zeitpunkt und die Mechanismen, die der Differenzierung des Parasiten in der Haut zugrunde liegen, sind unbekannt. Ebenso wurden die proliferativen Trypanosomen in der Haut bisher nur unzureichend charakterisiert. Das Verständnis über die ersten Schritte einer Infektion ist jedoch von entscheidender Bedeutung für die Entwicklung von neuen Strategien, die die Krankheitsentstehung und deren Fortschreiten verhindern sollen. Ein großes Hindernis bei der Erforschung der humanen Afrikanischen Trypanosomiasis ist der Mangel an geeigneten Infektionsmodellen, die den Krankheitsverlauf authentisch nachbilden. Außerdem werden für die Erzeugung der infektiösen metazyklischen Parasiten Tsetsefliegen benötigt, die aufwändig zu züchten sind. Tiermodelle haben es ermöglicht - hauptsächlich Mäuse -, viele Erkenntnisse über die Pathogenese von Trypanosomen im Säugetierwirt zu erlangen. Allerdings wurden diese überwiegend durch Nadelinjektion in den Bauchraum oder die Kaudalvene infiziert, wodurch die Haut als erste Eintrittspforte umgangen wurde. Darüber hinaus lassen Tiermodelle nicht immer Rückschlüsse auf den Infektionsverlauf beim Menschen zu. Zusätzlich erschwert die geringe Anzahl von metazyklischen Parasiten, die von Tsetsefliegen injiziert werden, die Isolation, Nachweis und Untersuchung im tierischen Wirt. Das Ziel der vorliegenden Arbeit war es, ein rekonstruiertes menschliches Hautäquivalent zu entwickeln und als Infektionsmodell zu validieren, um die Entwicklung von natürlich übertragenen metazyklischen Parasiten von T. brucei in der Säugetierhaut zu untersuchen. Der erste Teil dieser Arbeit beschreibt die Entwicklung und Charakterisierung eines primären menschlichen Hautäquivalents mit verbesserten mechanischen Eigenschaften. Zu diesem Zweck wurde ein computergesteuertes Kompressionssystem entworfen und hergestellt. Dieses System ermöglichte die gleichzeitige Verbesserung der mechanischen Stabilität von zwölf kollagenbasierten dermalen Äquivalenten durch plastische Kompression, die mittels Rheologie evaluiert wurden. Die verbesserten dermalen Äquivalente dienten als Fundament für die Erzeugung der Hautäquivalente und reduzierten deren Kontraktion und Gewichtsverlust während der Gewebebildung. Dadurch wurde ein hohes Maß an Standardisierung und Reproduzierbarkeit erreicht. Die Hautäquivalente wurden durch immunhistochemische und histologische Techniken charakterisiert und bildeten wichtige anatomische, zelluläre und funktionelle Aspekte der nativen menschlichen Haut nach. Des Weiteren wurde die zelluläre Heterogenität durch Einzelzell-RNA-Sequenzierung untersucht. Mit dieser Technik wurde ein umfangreiches Spektrum an extrazellulären Matrix-assoziierten Genen identifiziert, die von verschiedenen Zellsubpopulationen in der künstlichen Haut exprimiert werden. Zusätzlich wurden experimentelle Bedingungen etabliert, damit Tsetsefliegen eingesetzt werden konnten, um die Hautäquivalente auf natürlichem Weg mit Trypanosomen zu infizieren. Im zweiten Teil dieser Arbeit wurde die Entwicklung der Trypanosomen in der künstlichen Haut im Detail untersucht. Dies umfasste die Etablierung von Methoden zur erfolgreichen Isolierung der Trypanosomen aus der Haut, um deren Proteinsyntheserate, Zellzyklus- und Stoffwechselstatus, sowie Morphologie und Transkriptom zu bestimmen. Zusätzlich wurden Mikroskopietechniken zur Untersuchung der Trypanosomenmotilität und migration in der Haut optimiert. Nach der Injektion in die künstliche Haut durch Tsetsefliegen wurden die metazyklischen Parasiten schnell aktiviert und etablierten innerhalb eines Tages eine proliferative Population. Dieser Entwicklungsprozess wurde begleitet von (I) einer Reaktivierung der Proteinsynthese, (II) einem Wiedereintritt in den Zellzyklus, (III) einer Veränderung der Morphologie und (IV) einer erhöhten Motilität. Des Weiteren wurden diese Beobachtungen mit potentiell zugrundeliegenden entwicklungsbiologischen Mechanismen in Verbindung gebracht, indem eine Einzelzell RNA-Sequenzierung der Trypanosomen zu fünf verschiedenen Zeitpunkten nach der Infektion durchgeführt wurde. Nach der ersten proliferativen Phase traten die Tsetse-übertragenen Trypanosomen in der Haut in ein reversibles Ruhestadium ein. Diese ruhenden Trypanosomen waren durch eine sehr langsame Zellteilung, einen stark reduzierten Stoffwechsel und ein Transkriptom gekennzeichnet, dass sich deutlich von dem der injizierten metazyklischen Formen und der ersten proliferativen Trypanosomen unterschied. Durch Nachahmung der Migration von der Haut in den Blutkreislauf konnte dieser Phänotyp reaktiviert werden und die Parasiten kehrten in einen aktiven, proliferierenden Zustand zurück. Unter Berücksichtigung, dass vorangegangene Forschungsarbeiten die Haut als anatomisches Reservoir für T. brucei während des Krankheitsverlaufs identifiziert haben, ist anzunehmen, dass das Ruheprogramm eine authentische Facette im Verhalten des Parasiten in einem infizierten Wirt darstellt. Zusammenfassend zeigt diese Arbeit, das primäre menschliche Hautäquivalente eine neue und vielversprechende Möglichkeit bieten, vektorübertragene Parasiten unter naturnahen Bedingungen als Alternative zu Tierversuchen zu untersuchen. Durch die Verwendung des natürlichen Infektionsweges - dem Biss einer infizierten Tsetsefliege -, konnten die frühen Prozesse einer Trypanosomen-Infektion mit noch nie dagewesener Detailtiefe nachvollzogen werden. Des Weiteren könnte der hier erbrachte Nachweis einer ruhenden, hautresidenten Trypanosomen-Population die Persistenz von T. brucei in der Haut von aparasitämischen und asymptomatischen Personen erklären. Dies könnte eine wichtige Rolle bei der Aufrechterhaltung einer Infektion über lange Zeiträume spielen. KW - Trypanosoma brucei KW - Tissue Engineering KW - Trypanosomiasis KW - 3D-Zellkultur KW - Transkriptomanalyse KW - developmental differentiation KW - skin equivalent KW - artificial human skin KW - single-cell RNA sequencing KW - quiescence Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-251147 ER - TY - JOUR A1 - Dhillon, Maninder Singh A1 - Kübert-Flock, Carina A1 - Dahms, Thorsten A1 - Rummler, Thomas A1 - Arnault, Joel A1 - Steffan-Dewenter, Ingolf A1 - Ullmann, Tobias T1 - Evaluation of MODIS, Landsat 8 and Sentinel-2 data for accurate crop yield predictions: a case study using STARFM NDVI in Bavaria, Germany JF - Remote Sensing N2 - The increasing availability and variety of global satellite products and the rapid development of new algorithms has provided great potential to generate a new level of data with different spatial, temporal, and spectral resolutions. However, the ability of these synthetic spatiotemporal datasets to accurately map and monitor our planet on a field or regional scale remains underexplored. This study aimed to support future research efforts in estimating crop yields by identifying the optimal spatial (10 m, 30 m, or 250 m) and temporal (8 or 16 days) resolutions on a regional scale. The current study explored and discussed the suitability of four different synthetic (Landsat (L)-MOD13Q1 (30 m, 8 and 16 days) and Sentinel-2 (S)-MOD13Q1 (10 m, 8 and 16 days)) and two real (MOD13Q1 (250 m, 8 and 16 days)) NDVI products combined separately to two widely used crop growth models (CGMs) (World Food Studies (WOFOST), and the semi-empiric Light Use Efficiency approach (LUE)) for winter wheat (WW) and oil seed rape (OSR) yield forecasts in Bavaria (70,550 km\(^2\)) for the year 2019. For WW and OSR, the synthetic products’ high spatial and temporal resolution resulted in higher yield accuracies using LUE and WOFOST. The observations of high temporal resolution (8-day) products of both S-MOD13Q1 and L-MOD13Q1 played a significant role in accurately measuring the yield of WW and OSR. For example, L- and S-MOD13Q1 resulted in an R\(^2\) = 0.82 and 0.85, RMSE = 5.46 and 5.01 dt/ha for WW, R\(^2\) = 0.89 and 0.82, and RMSE = 2.23 and 2.11 dt/ha for OSR using the LUE model, respectively. Similarly, for the 8- and 16-day products, the simple LUE model (R\(^2\) = 0.77 and relative RMSE (RRMSE) = 8.17%) required fewer input parameters to simulate crop yield and was highly accurate, reliable, and more precise than the complex WOFOST model (R\(^2\) = 0.66 and RRMSE = 11.35%) with higher input parameters. Conclusively, both S-MOD13Q1 and L-MOD13Q1, in combination with LUE, were more prominent for predicting crop yields on a regional scale than the 16-day products; however, L-MOD13Q1 was advantageous for generating and exploring the long-term yield time series due to the availability of Landsat data since 1982, with a maximum resolution of 30 m. In addition, this study recommended the further use of its findings for implementing and validating the long-term crop yield time series in different regions of the world. KW - MODIS KW - Sentinel-2 KW - Landsat 8 KW - sustainable agriculture KW - decision-making KW - winter wheat KW - oil seed rape KW - resolution Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-311132 SN - 2072-4292 VL - 15 IS - 7 ER - TY - THES A1 - Gotthard, Hannes T1 - Targeting Colorectal Cancer Stem Cells with Hemibodies T1 - Eliminierung von Krebsstammzellen des kolorektalen Karzinoms mithilfe von Hemibodies N2 - The cancer stem cell hypothesis is a cancer development model which elicited great interest in the last decades stating that cancer heterogeneity arises from a stem cell through asymmetrical division. The Cancer Stem Cell subset is described as the only population to be tumorigenic and having the potential to renew. Conventional therapy often fails to eradicate CSC resulting in tumor relapse. Consequently, it is of great inter-est to eliminate this subset of cells to provide the best patient outcome. In the last years several approaches to target CSC were developed, one of them being immunotherapeu-tic targeting with antibodies. Since markers associated with CSC are also expressed on normal stem cells or healthy adjacent tissue in colorectal cancer, dual targeting strate-gies are preferred over targeting only a single antigen. Subsequently, the idea of dual targeting two CSC markers in parallel by a newly developed split T cell-engaging anti-body format termed as Hemibodies emerged. In a preliminary single cell RNA sequenc-ing analysis of colorectal cancer cells CD133, CD24, CD166 and CEA were identified as suitable targets for the combinatorial targeting strategy. Therefore, this study focused on trispecific and trivalent Hemibodies comprising a split binding moiety against CD3 and a binding moiety against either CD133, CD24, CD166 or CEA to overcome the occurrence of resistance and to efficiently eradicate all tumor cells including the CSC compartment. The study showed that the Hemibody combinations CD133xCD24, CD133xCD166 and CD133xCEA are able to eliminate double positive CHO cells with high efficacy while having a high specificity indicated by no killing of single antigen positive cells. A thera-peutic window ranging between one to two log levels could be achieved for all combina-tions mentioned above. The combinations CD133xCD24 and CD133xCD166 further-more proved its efficacy and specificity on established colorectal cancer cell lines. Be-sides the evaluation of specificity and efficacy the already introduced 1st generation of Hemibodies could be improved into a 2nd generation Hemibody format with increased half-life, stability and production yield. In future experiments the applicability of above-mentioned Hemibodies will be proven on patient-derived micro tumors to also include variables like tumor microenvironment and infiltration. N2 - In den letzten Jahrzenten wurde neben der klonalen Evolution ein weiteres Modell zur Krebsentstehung und dessen Heterogenität entwickelt: die Krebsstammzellhypothe-se. Diese Hypothese besagt, dass die Heterogenität eines Tumors durch asymmetri-sche Teilung von sogenannten Krebsstammzellen entsteht. Nur diese sind tumorigen und in der Lage Metastasen zu bilden. Außerdem werden Krebsstammzellen als re-sistent gegen konventionelle Therapien beschrieben, weshalb es nach einer anfängli-chen Tumorregression oft zu einem Rezidiv durch erneutes Auswachsen von zurück-bleibenden Krebsstammzellen kommt. Deshalb ist es von großem Interesse genau diese Population abzutöten, um eine erfolgreiche Therapie zu gewährleisten. In den letzten Jahren wurden zahlreiche Medikationen entwickelt, um Krebsstammzellen ge-zielt anzugreifen. Ein vielversprechender Ansatz ist hierbei die immuntherapeutische Adressierung mittels Antikörpern gegen Krebsstammzellmarkern. Einzelne Marker sind allerdings auch auf normalen Stammzellen und gesundem Gewebe exprimiert, weshalb Therapien, die auf mindestens zwei verschiedene Oberflächenproteine ab-zielen, erfolgsversprechender sind. In dieser Arbeit wurde ein neues T-Zell rekrutie-rendes Antikörperformat entwickelt, sogenannte Hemibodies. Hierbei handelt es sich um ein trispezifisches und trivalentes Format, bestehend aus jeweils zwei Fragmen-ten. Jedes Fragment besteht aus einer Bindedomäne gegen ein Krebsstammzellmar-ker und einer geteilten Bindedomäne gegen CD3. Durch Bindung beider Fragmente an einen Stammzellmarker kommt es zur Komplementierung der geteilten anti-CD3 Domäne und zur T-Zellrekrutierung. Der erste Teil der Arbeit befasst sich mit der bioin-formatischen Analyse von Einzelzell-RNA-Daten des kolorektalen Karzinoms (KRK) zur Identifizierung von potentiellen Krebsstammzellmarkern. Dabei konnten die Ober-flächenproteine CD24, CD133, CD166 und CEA und besonders deren Kombination als geeignete Zielstrukturen identifiziert werden. Die gegen oben genannte Antigene gerichteten Hemibodies zeigten in den Kombinationen CD133xCD24, CD133xCD166 und CD133xCEA auf doppelt positiven CHO-Zellen eine hohe Effektivität. Außerdem konnte die Spezifität durch ein Ausbleiben von Zelltod auf einzel-positiven CHO Zellen bewiesen werden. Die Kombinationen CD133xCD24 und CD133xCD166 konnten Effektivität und Spezifität auch auf etablierten Krebszellen zeigen. Die oben genann-ten Kombinationen waren in einem therapeutischen Fenster von ein bis zwei Logstu-fen funktional. Neben der Testung verschiedener Hemibody-Kombinationen konnten die bereits publizierten Hemibodies der ersten Generation in ein neues Format der zweiten Generation weiterentwickelt werden. Das neue Format zeigte eine verbesser-te Halbwertszeit, Stabilität und Produzierbarkeit. In zukünftigen Experimenten werden die in der Thesis benutzten Hemibodies auf Mikrotumoren getestet, um weitere Vari-ablen, die die Effektivität und Spezifität beeinflussen zu ermitteln. KW - Monoklonaler bispezifischer Antikörper KW - Antikörper KW - T-Lymphozyt KW - Immunreaktion KW - Dickdarmkrebs KW - Hemibody KW - Hemibodies KW - Colorectal Cancer KW - trispecific KW - T-cell engager KW - dual targeting KW - Bispecific T-cell engager KW - stem cells KW - Kolorektales Karzinom Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-303090 ER - TY - THES A1 - Meiser, Elisabeth T1 - Single-molecule dynamics at a bottleneck: a systematic study of the narrow escape problem in a disc T1 - Einzelmoleküldynamik an einem Engpass: Eine systematische Untersuchung des Narrow Escape Problems in einer Scheibe N2 - Diffusion facilitates numerous reactions within the biological context of a cell. It is remarkable how the cost-efficient random process of Brownian motion promotes fast reactions. From the narrow escape theory, it is possible to determine the mean first passage time of such processes based on their reaction space and diffusion coefficient. The narrow escape theory of Brownian particles is characterized by a confining domain with reflective boundaries and a small reaction site. In this thesis, the mean first passage time was systematically tested in a disc as a function of the escape opening size in vitro and in silico. For the in vitro experiments, a model system of patterned supported-lipid bilayers (SLB) was established. Such a model is prepared by a combined colloid metalization approach, where a gold scaffold on glass facilitates assembly of SLB patches of distinct sizes through vesicle fusion. The model setup was evaluated and found to match all necessary requirements to test the nar- row escape problem in vitro. In particular, the reflectivity of the boundaries, the unhindered, free diffusion of the tracer lipids, and the distinct area were assessed. Observed results of the mean first passage time agreed with the theory of the narrow escape problem. There was excellent agreement in both absolute values and across a range of small escape opening sizes. Additionally, I developed a straightforward method, a correction factor, to calculate the mean first passage time from incomplete experimental traces. By re-scaling the mean first passage time to the fraction of particles that escaped, I was able to overcome the lifetime limitations of fluorescent probes. Previously inaccessible measurements of the mean first passage time relying on fluorescent probes will be made possible through this approach. The in vitro experiments were complemented with various in silico experiments. The latter were based on random walk simulations in discs, mimicking the in vitro situation with its uncertainties. The lifetime of single particles was either set sufficiently long to allow all particles to escape, or was adjusted to meet the lifetime limitations observed in the in vitro experiments. A comparison of the mean first passage time from lifetime-unlimited particles to the corrected, lifetime-limited particles did support the use of the correction factor. In agreement with the narrow escape theory, it was experimentally found that the mean first passage time is independent of the start point of the particle within the domain. This is when the particle adheres to a minimum distance to the escape site. In general, the presented random walk simulations do accurately represent the in vitro experiments in this study. The required hardware for the establishment of an astigmatism-based 3D system was installed in the existing microscope. The first attempts to analyze the obtained 3D imaging data gave insight into the potential of the method to investigate molecule dynamics in living trypanosome cells. The full functionality will be realized with the ongoing improvement of image analysis outside of this thesis. N2 - Diffusion erleichtert zahlreiche Reaktionen im biologischen Kontext einer Zelle. Es ist bemerkenswert, wie der kosteneffiziente Zufallsprozess der Brownschen Bewegung schnelle Reaktionen fördert. Mit Hilfe der Narrow Escape Theorie kann die mittlere erste Durchgangszeit (mean first passage time) solcher Prozesse auf der Grundlage ihres Reaktionsraums und des Diffusionskoeffizienten bestimmt werden. Die Narrow Escape Theorie von Brownschen Teilchen wird durch einen begrenzten Bereich mit reflektierenden Grenzen und einen kleinen Reaktionsraum gekennzeichnet. In dieser Arbeit wurde die mittlere erste Durchgangszeit in einer Scheibe systematisch als Funktion der Größe der Fluchtöffnung in vitro und in silico untersucht. Fur die in vitro-Experimente wurde ein Modellsystem aus strukturierten, Glas gestützten Lipiddoppelschichten (SLB) erstellt. Dieses Modell wurde durch einen kombinierten Kolloid-Metallisierungsansatz hergestellt, bei dem eine strukturierte Goldschicht auf Glas die Bildung von SLB-Scheiben unterschiedlicher Größe durch die Vesikelfusion ermöglicht. Es wurde festgestellt, dass das Modell alle Anforderungen erfüllt, um das Narrow escape problem in vitro zu testen. Insbesondere wurde das Reflexionsvermögen der Grenzen, die ungehinderte, freie Diffusion der Lipide und die Präzision der Fläche bewertet. Die beobachteten Ergebnisse der mittleren ersten Durchgangszeit stimmen mit der NEP-Theorie ̈uberein. Es besteht eine hervorragende ̈Ubereinstimmung sowohl bei den absoluten Werten als auch systematisch ̈uber einen Bereich von kleinen Fluchtöffnungsgrößen. Außerdem zeige ich eine einfache Methode, einen Korrekturfaktor, zur Berechnung der mittleren ersten Durchgangszeit aus unvollstandigen Lipid Trajektorien des Experimentes. Indem ich die mittlere erste Durchgangszeit auf den Anteil der entkommenen Par- tikel skalierte, konnte ich die Einschränkungen der Lebensdauer von fluoreszenten Farbstoffen ausgleichen. Mit dieser Technik werden bisher unzugängliche Messungen der mittleren ersten Durchgangszeit auf der Grundlage von fluoreszenten Farbstoffen möglich. In einem umfassenden Ansatz wurden die in vitro-Experimente durch verschiedene in silico-Experimente ergänzt. Letztere basierten auf Random- Walk-Simulationen in Scheiben, die die in vitro-Situation mit ihren Unsicherheiten nachahmten. Die Lebensdauer einzelner Partikel wurde entweder so lang angesetzt, dass alle Partikel entkommen konnten, oder sie wurde so angepasst, dass sie den in den in vitro-Experimenten beobachteten Lebensdauerbeschränkungen entsprach. Ein Vergleich der mittleren ersten Durchgangszeit von unsterblichen Partikeln mit den korrigierten, lebensdauerbegrenzten Partikeln hat die Verwendung des Korrekturfaktors bestätigt. In ̈Ubereinstimmung mit der Narrow Escape Theorie wurde experimentell festgestellt, dass die mittlere erste Durchgangszeit unabhängig vom Startpunkt des Teilchens innerhalb der Domäne ist. Dies ist dann der Fall, wenn das Teilchen einen Mindestabstand zur Austrittsstelle einhält. Im Allgemeinen bilden die vorgestellten Random-Walk-Simulationen die in dieser Studie durchgeführten Experimente genau ab. Die erforderliche Hardware für die Einrichtung eines auf Astigmatismus basierenden 3D-Systems wurde in ein vorhandenes Mikroskop eingebaut. Erste Versuche, die gewonnenen 3D-Bilddaten zu analysieren, gaben einen Einblick in das Potenzial der Methode zur Untersuchung der Moleküldynamik im lebenden Trypanosom. Die volle Funktionalität wird mit der laufenden Verbesserung der Bildanalyse außerhalb dieser Arbeit realisiert werden. Ein Teil der Ergebnisse und Methoden dieser Dissertation wurde zur Veröffentlichung unter dem Titel ’Experiments in micro-patterned model membranes support the narrow escape theory’ eingereicht. KW - Freies Molekül KW - Kolloid KW - Bimolekulare Lipidschicht KW - Mikroskopie KW - Brownsche Bewegung KW - Narrow escape problem KW - mean first passage time KW - single-molecule localization microscopy KW - single particle tracking KW - Random-walk simulations Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-319650 ER - TY - JOUR A1 - Maloukh, Lina A1 - Nazzal, Yousef A1 - Kumarappan, Alagappan A1 - Howari, Fares A1 - Ambika, Lakshmi Kesari A1 - Yahmadi, Rihab A1 - Sharma, Manish A1 - Iqbal, Jibran A1 - Al-Taani, Ahmed A. A1 - Salem, Imen Ben A1 - Xavier, Cijo M. A1 - Naseem, Muhamad T1 - Metagenomic analysis of the outdoor dust microbiomes: a case study from Abu Dhabi, UAE JF - Atmosphere N2 - Outdoor dust covers a shattered range of microbial agents from land over transportation, human microbial flora, which includes pathogen and commensals, and airborne from the environment. Dust aerosols are rich in bacterial communities that have a major impact on human health and living environments. In this study, outdoor samples from roadside barricades, safety walls, and fences (18 samples) were collected from Abu Dhabi, UAE and bacterial diversity was assessed through a 16S rRNA amplicon next generation sequencing approach. Clean data from HiSeq produced 1,099,892 total reads pairs for 18 samples. For all samples, taxonomic classifications were assigned to the OTUs (operational taxonomic units) representative sequence using the Ribosomal Database Project database. Analysis such as alpha diversity, beta diversity, differential species analysis, and species relative abundance were performed in the clustering of samples and a functional profile heat map was obtained from the OTUs by using bioinformatics tools. A total of 2814 OTUs were identified from those samples with a coverage of more than 99%. In the phylum, all 18 samples had most of the bacterial groups such as Actinobacteria, Proteobacteria, Firmicutes, and Bacteroidetes. Twelve samples had Propionibacteria acnes and were mainly found in RD16 and RD3. Major bacteria species such as Propionibacteria acnes, Bacillus persicus, and Staphylococcus captis were found in all samples. Most of the samples had Streptococcus mitis, Staphylococcus capitis. and Nafulsella turpanensis and Enhydrobacter aerosaccus was part of the normal microbes of the skin. Salinimicrobium sp., Bacillus alkalisediminis, and Bacillus persicus are halophilic bacteria found in sediments. The heat map clustered the samples and species in vertical and horizontal classification, which represents the relationship between the samples and bacterial diversity. The heat map for the functional profile had high properties of amino acids, carbohydrate, and cofactor and vitamin metabolisms of all bacterial species from all samples. Taken together, our analyses are very relevant from the perspective of out-door air quality, airborne diseases, and epidemics, with broader implications for health safety and monitoring. KW - dust microbiomes KW - metagenomics KW - microbial diversity KW - pollution KW - GIS Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-304391 SN - 2073-4433 VL - 14 IS - 2 ER - TY - JOUR A1 - Moustafa, Moataz A. M. A1 - Fouad, Eman A. A1 - Ibrahim, Emad A1 - Erdei, Anna Laura A1 - Kárpáti, Zsolt A1 - Fónagy, Adrien T1 - The comparative toxicity, biochemical and physiological impacts of chlorantraniliprole and indoxacarb on Mamestra brassicae (Lepidoptera: Noctuidae) JF - Toxics N2 - Background: The cabbage moth, Mamestra brassicae, is a polyphagous pest that attacks several crops. Here, the sublethal and lethal effects of chlorantraniliprole and indoxacarb were investigated on the developmental stages, detoxification enzymes, reproductive activity, calling behavior, peripheral physiology, and pheromone titer of M. brasssicae. Methods: To assess pesticide effects, the second instar larvae were maintained for 24 h on a semi-artificial diet containing insecticides at their LC\(_{10}\), LC\(_{30}\), and LC\(_{50}\) concentrations. Results: M. brassicae was more susceptible to chlorantraniliprole (LC\(_{50}\) = 0.35 mg/L) than indoxacarb (LC\(_{50}\) = 1.71 mg/L). A significantly increased developmental time was observed with both insecticides at all tested concentrations but decreases in pupation rate, pupal weight, and emergence were limited to the LC50 concentration. Reductions in both the total number of eggs laid per female and the egg viability were observed with both insecticides at their LC\(_{30}\) and LC\(_{50}\) concentrations. Both female calling activity and the sex pheromone (Z11-hexadecenyl acetate and hexadecenyl acetate) titer were significantly reduced by chlorantraniliprole in LC\(_{50}\) concentration. Antennal responses of female antennae to benzaldehyde and 3-octanone were significantly weaker than controls after exposure to the indoxocarb LC\(_{50}\) concentration. Significant reductions in the enzymatic activity of glutathione S-transferases, mixed-function oxidases, and carboxylesterases were observed in response to both insecticides. KW - toxicity KW - sublethal effects KW - chlorantraniliprole KW - indoxacarb KW - Mamestra brassicae Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-303931 SN - 2305-6304 VL - 11 IS - 3 ER - TY - JOUR A1 - Coelho, Luis Pedro A1 - Alves, Renato A1 - Monteiro, Paulo A1 - Huerta-Cepas, Jaime A1 - Freitas, Ana Teresa A1 - Bork, Peer T1 - NG-meta-profiler: fast processing of metagenomes using NGLess, a domain-specific language JF - Microbiome N2 - Background Shotgun metagenomes contain a sample of all the genomic material in an environment, allowing for the characterization of a microbial community. In order to understand these communities, bioinformatics methods are crucial. A common first step in processing metagenomes is to compute abundance estimates of different taxonomic or functional groups from the raw sequencing data. Given the breadth of the field, computational solutions need to be flexible and extensible, enabling the combination of different tools into a larger pipeline. Results We present NGLess and NG-meta-profiler. NGLess is a domain specific language for describing next-generation sequence processing pipelines. It was developed with the goal of enabling user-friendly computational reproducibility. It provides built-in support for many common operations on sequencing data and is extensible with external tools with configuration files. Using this framework, we developed NG-meta-profiler, a fast profiler for metagenomes which performs sequence preprocessing, mapping to bundled databases, filtering of the mapping results, and profiling (taxonomic and functional). It is significantly faster than either MOCAT2 or htseq-count and (as it builds on NGLess) its results are perfectly reproducible. Conclusions NG-meta-profiler is a high-performance solution for metagenomics processing built on NGLess. It can be used as-is to execute standard analyses or serve as the starting point for customization in a perfectly reproducible fashion. NGLess and NG-meta-profiler are open source software (under the liberal MIT license) and can be downloaded from https://ngless.embl.de or installed through bioconda. KW - metagenomics KW - next-generation sequencing KW - domain-specific language Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-223161 VL - 7 IS - 84 ER - TY - JOUR A1 - Coelho, Luis Pedro A1 - Kultima, Jens Roat A1 - Costea, Paul Igor A1 - Fournier, Coralie A1 - Pan, Yuanlong A1 - Czarnecki-Maulden, Gail A1 - Hayward, Matthew Robert A1 - Forslund, Sofia K. A1 - Schmidt, Thomas Sebastian Benedikt A1 - Descombes, Patrick A1 - Jackson, Janet R. A1 - Li, Qinghong A1 - Bork, Peer T1 - Similarity of the dog and human gut microbiomes in gene content and response to diet JF - Microbiome N2 - Background Gut microbes influence their hosts in many ways, in particular by modulating the impact of diet. These effects have been studied most extensively in humans and mice. In this work, we used whole genome metagenomics to investigate the relationship between the gut metagenomes of dogs, humans, mice, and pigs. Results We present a dog gut microbiome gene catalog containing 1,247,405 genes (based on 129 metagenomes and a total of 1.9 terabasepairs of sequencing data). Based on this catalog and taxonomic abundance profiling, we show that the dog microbiome is closer to the human microbiome than the microbiome of either pigs or mice. To investigate this similarity in terms of response to dietary changes, we report on a randomized intervention with two diets (high-protein/low-carbohydrate vs. lower protein/higher carbohydrate). We show that diet has a large and reproducible effect on the dog microbiome, independent of breed or sex. Moreover, the responses were in agreement with those observed in previous human studies. Conclusions We conclude that findings in dogs may be predictive of human microbiome results. In particular, a novel finding is that overweight or obese dogs experience larger compositional shifts than lean dogs in response to a high-protein diet. KW - microbiome KW - diet KW - metagenomics KW - dog microbiome KW - human microbiome KW - mouse microbiome KW - pig microbiome Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-223177 VL - 6 ER - TY - JOUR A1 - Dedukh, Dmitrij A1 - Da Cruz, Irene A1 - Kneitz, Susanne A1 - Marta, Anatolie A1 - Ormanns, Jenny A1 - Tichopád, Tomáš A1 - Lu, Yuan A1 - Alsheimer, Manfred A1 - Janko, Karel A1 - Schartl, Manfred T1 - Achiasmatic meiosis in the unisexual Amazon molly, Poecilia formosa JF - Chromosome Research N2 - Unisexual reproduction, which generates clonal offspring, is an alternative strategy to sexual breeding and occurs even in vertebrates. A wide range of non-sexual reproductive modes have been described, and one of the least understood questions is how such pathways emerged and how they mechanistically proceed. The Amazon molly, Poecilia formosa, needs sperm from males of related species to trigger the parthenogenetic development of diploid eggs. However, the mechanism, of how the unreduced female gametes are produced, remains unclear. Cytological analyses revealed that the chromosomes of primary oocytes initiate pachytene but do not proceed to bivalent formation and meiotic crossovers. Comparing ovary transcriptomes of P. formosa and its sexual parental species revealed expression levels of meiosis-specific genes deviating from P. mexicana but not from P. latipinna. Furthermore, several meiosis genes show biased expression towards one of the two alleles from the parental genomes. We infer from our data that in the Amazon molly diploid oocytes are generated by apomixis due to a failure in the synapsis of homologous chromosomes. The fact that this failure is not reflected in the differential expression of known meiosis genes suggests the underlying molecular mechanism may be dysregulation on the protein level or misexpression of a so far unknown meiosis gene, and/or hybrid dysgenesis because of compromised interaction of proteins from diverged genomes. KW - meiosis KW - parthenogenesis KW - synaptonemal complex KW - recombination KW - crossing-over KW - achiasmatic KW - transcriptome KW - oogenesis Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-325128 VL - 30 IS - 4 ER - TY - JOUR A1 - Conrad, David A1 - Kehl, Alexandra A1 - Müller, Tobias A1 - Klopfleisch, Robert A1 - Aupperle-Lellbach, Heike T1 - Immunohistochemical and molecular genetic analysis of canine digital mast cell tumours JF - Animals N2 - Grading, immunohistochemistry and c-kit mutation status are criteria for assessing the prognosis and therapeutic options of canine cutaneous mast cell tumours (MCTs). As a subset, canine digital MCTs have rarely been explored in this context. Therefore, in this retrospective study, 68 paraffin-embedded canine digital MCTs were analysed, and histological grading was assessed according to Patnaik and Kiupel. The immunohistochemical markers KIT and Ki67 were used, as well as polymerase chain reaction (PCR) for mutational screening in c-kit exons 8, 9, 11 and 14. Patnaik grading resulted in 22.1% grade I, 67.6% grade II and 10.3% grade III tumours. Some 86.8% of the digital MCTs were Kiupel low-grade. Aberrant KIT staining patterns II and III were found in 58.8%, and a count of more than 23 Ki67-positive cells in 52.3% of the cases. Both parameters were significantly associated with an internal tandem duplication (ITD) in c-kit exon 11 (12.7%). French Bulldogs, which tend to form well-differentiated cutaneous MCTs, had a higher proportion of digital high-grade MCTs and ITD in c-kit exon 11 compared with mongrels. Due to its retrospective nature, this study did not allow for an analysis of survival data. Nevertheless, it may contribute to the targeted characterisation of digital MCTs. KW - dog KW - digit KW - toe KW - CD117 KW - Ki67 KW - KIT KW - grading KW - PCR KW - sequencing KW - c-kit Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-319199 SN - 2076-2615 VL - 13 IS - 10 ER - TY - JOUR A1 - Maichl, Daniela Simone A1 - Kirner, Julius Arthur A1 - Beck, Susanne A1 - Cheng, Wen-Hui A1 - Krug, Melanie A1 - Kuric, Martin A1 - Ade, Carsten Patrick A1 - Bischler, Thorsten A1 - Jakob, Franz A1 - Hose, Dirk A1 - Seckinger, Anja A1 - Ebert, Regina A1 - Jundt, Franziska T1 - Identification of NOTCH-driven matrisome-associated genes as prognostic indicators of multiple myeloma patient survival JF - Blood Cancer Journal N2 - No abstract available. KW - cancer microenvironment KW - myeloma Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-357598 VL - 13 ER - TY - JOUR A1 - Dhillon, Maninder Singh A1 - Dahms, Thorsten A1 - Kübert-Flock, Carina A1 - Liepa, Adomas A1 - Rummler, Thomas A1 - Arnault, Joel A1 - Steffan-Dewenter, Ingolf A1 - Ullmann, Tobias T1 - Impact of STARFM on crop yield predictions: fusing MODIS with Landsat 5, 7, and 8 NDVIs in Bavaria Germany JF - Remote Sensing N2 - Rapid and accurate yield estimates at both field and regional levels remain the goal of sustainable agriculture and food security. Hereby, the identification of consistent and reliable methodologies providing accurate yield predictions is one of the hot topics in agricultural research. This study investigated the relationship of spatiotemporal fusion modelling using STRAFM on crop yield prediction for winter wheat (WW) and oil-seed rape (OSR) using a semi-empirical light use efficiency (LUE) model for the Free State of Bavaria (70,550 km\(^2\)), Germany, from 2001 to 2019. A synthetic normalised difference vegetation index (NDVI) time series was generated and validated by fusing the high spatial resolution (30 m, 16 days) Landsat 5 Thematic Mapper (TM) (2001 to 2012), Landsat 7 Enhanced Thematic Mapper Plus (ETM+) (2012), and Landsat 8 Operational Land Imager (OLI) (2013 to 2019) with the coarse resolution of MOD13Q1 (250 m, 16 days) from 2001 to 2019. Except for some temporal periods (i.e., 2001, 2002, and 2012), the study obtained an R\(^2\) of more than 0.65 and a RMSE of less than 0.11, which proves that the Landsat 8 OLI fused products are of higher accuracy than the Landsat 5 TM products. Moreover, the accuracies of the NDVI fusion data have been found to correlate with the total number of available Landsat scenes every year (N), with a correlation coefficient (R) of +0.83 (between R\(^2\) of yearly synthetic NDVIs and N) and −0.84 (between RMSEs and N). For crop yield prediction, the synthetic NDVI time series and climate elements (such as minimum temperature, maximum temperature, relative humidity, evaporation, transpiration, and solar radiation) are inputted to the LUE model, resulting in an average R\(^2\) of 0.75 (WW) and 0.73 (OSR), and RMSEs of 4.33 dt/ha and 2.19 dt/ha. The yield prediction results prove the consistency and stability of the LUE model for yield estimation. Using the LUE model, accurate crop yield predictions were obtained for WW (R\(^2\) = 0.88) and OSR (R\(^2\) = 0.74). Lastly, the study observed a high positive correlation of R = 0.81 and R = 0.77 between the yearly R\(^2\) of synthetic accuracy and modelled yield accuracy for WW and OSR, respectively. KW - MOD13Q1 KW - precision agriculture KW - fusion KW - sustainable agriculture KW - decision making KW - winter wheat KW - oil-seed rape KW - crop models Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-311092 SN - 2072-4292 VL - 15 IS - 6 ER - TY - JOUR A1 - Brenner, Daniela A1 - Geiger, Nina A1 - Schlegel, Jan A1 - Diesendorf, Viktoria A1 - Kersting, Louise A1 - Fink, Julian A1 - Stelz, Linda A1 - Schneider-Schaulies, Sibylle A1 - Sauer, Markus A1 - Bodem, Jochen A1 - Seibel, Jürgen T1 - Azido-ceramides, a tool to analyse SARS-CoV-2 replication and inhibition — SARS-CoV-2 is inhibited by ceramides JF - International Journal of Molecular Sciences N2 - Recently, we have shown that C6-ceramides efficiently suppress viral replication by trapping the virus in lysosomes. Here, we use antiviral assays to evaluate a synthetic ceramide derivative α-NH2-ω-N3-C6-ceramide (AKS461) and to confirm the biological activity of C6-ceramides inhibiting SARS-CoV-2. Click-labeling with a fluorophore demonstrated that AKS461 accumulates in lysosomes. Previously, it has been shown that suppression of SARS-CoV-2 replication can be cell-type specific. Thus, AKS461 inhibited SARS-CoV-2 replication in Huh-7, Vero, and Calu-3 cells up to 2.5 orders of magnitude. The results were confirmed by CoronaFISH, indicating that AKS461 acts comparable to the unmodified C6-ceramide. Thus, AKS461 serves as a tool to study ceramide-associated cellular and viral pathways, such as SARS-CoV-2 infections, and it helped to identify lysosomes as the central organelle of C6-ceramides to inhibit viral replication. KW - ceramides KW - SARS-CoV-2 KW - azido-ceramides KW - sphingolipids Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-313581 SN - 1422-0067 VL - 24 IS - 8 ER - TY - JOUR A1 - Däullary, Thomas A1 - Imdahl, Fabian A1 - Dietrich, Oliver A1 - Hepp, Laura A1 - Krammer, Tobias A1 - Fey, Christina A1 - Neuhaus, Winfried A1 - Metzger, Marco A1 - Vogel, Jörg A1 - Westermann, Alexander J. A1 - Saliba, Antoine-Emmanuel A1 - Zdzieblo, Daniela T1 - A primary cell-based in vitro model of the human small intestine reveals host olfactomedin 4 induction in response to Salmonella Typhimurium infection JF - Gut Microbes N2 - Infection research largely relies on classical cell culture or mouse models. Despite having delivered invaluable insights into host-pathogen interactions, both have limitations in translating mechanistic principles to human pathologies. Alternatives can be derived from modern Tissue Engineering approaches, allowing the reconstruction of functional tissue models in vitro. Here, we combined a biological extracellular matrix with primary tissue-derived enteroids to establish an in vitro model of the human small intestinal epithelium exhibiting in vivo-like characteristics. Using the foodborne pathogen Salmonella enterica serovar Typhimurium, we demonstrated the applicability of our model to enteric infection research in the human context. Infection assays coupled to spatio-temporal readouts recapitulated the established key steps of epithelial infection by this pathogen in our model. Besides, we detected the upregulation of olfactomedin 4 in infected cells, a hitherto unrecognized aspect of the host response to Salmonella infection. Together, this primary human small intestinal tissue model fills the gap between simplistic cell culture and animal models of infection, and shall prove valuable in uncovering human-specific features of host-pathogen interplay. KW - intestinal enteroids KW - biological scaffold KW - Salmonella Typhimurium KW - OLFM4 KW - NOTCH KW - filamentous Salmonella Typhimurium KW - bacterial migration KW - bacterial virulence KW - 3D tissue model KW - olfactomedin 4 KW - infection Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-350451 VL - 15 IS - 1 ER - TY - JOUR A1 - Chumduri, Cindrilla A1 - Turco, Margherita Y. T1 - Organoids of the female reproductive tract JF - Journal of Molecular Medicine N2 - Healthy functioning of the female reproductive tract (FRT) depends on balanced and dynamic regulation by hormones during the menstrual cycle, pregnancy and childbirth. The mucosal epithelial lining of different regions of the FRT—ovaries, fallopian tubes, uterus, cervix and vagina—facilitates the selective transport of gametes and successful transfer of the zygote to the uterus where it implants and pregnancy takes place. It also prevents pathogen entry. Recent developments in three-dimensional (3D) organoid systems from the FRT now provide crucial experimental models that recapitulate the cellular heterogeneity and physiological, anatomical and functional properties of the organ in vitro. In this review, we summarise the state of the art on organoids generated from different regions of the FRT. We discuss the potential applications of these powerful in vitro models to study normal physiology, fertility, infections, diseases, drug discovery and personalised medicine. KW - female reproductive tract KW - organoids KW - reproductive health KW - pregnancy KW - fertility KW - infection KW - cancers Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-328374 VL - 99 IS - 4 ER - TY - JOUR A1 - Brenzinger, Kristof A1 - Costa, Ohana Y. A. A1 - Ho, Adrian A1 - Koorneef, Guusje A1 - Robroek, Bjorn A1 - Molenaar, Douwe A1 - Korthals, Gerard A1 - Bodelier, Paul L. E. T1 - Steering microbiomes by organic amendments towards climate-smart agricultural soils JF - Biology and Fertility of Soils N2 - We steered the soil microbiome via applications of organic residues (mix of cover crop residues, sewage sludge + compost, and digestate + compost) to enhance multiple ecosystem services in line with climate-smart agriculture. Our result highlights the potential to reduce greenhouse gases (GHG) emissions from agricultural soils by the application of specific organic amendments (especially digestate + compost). Unexpectedly, also the addition of mineral fertilizer in our mesocosms led to similar combined GHG emissions than one of the specific organic amendments. However, the application of organic amendments has the potential to increase soil C, which is not the case when using mineral fertilizer. While GHG emissions from cover crop residues were significantly higher compared to mineral fertilizer and the other organic amendments, crop growth was promoted. Furthermore, all organic amendments induced a shift in the diversity and abundances of key microbial groups. We show that organic amendments have the potential to not only lower GHG emissions by modifying the microbial community abundance and composition, but also favour crop growth-promoting microorganisms. This modulation of the microbial community by organic amendments bears the potential to turn soils into more climate-smart soils in comparison to the more conventional use of mineral fertilizers. KW - greenhouse gases KW - agricultural soils KW - organic amendment KW - flux measurements KW - microbial community abundance and compositions KW - plant growth Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-326930 VL - 57 IS - 8 ER - TY - JOUR A1 - Maihoff, Fabienne A1 - Sahler, Simone A1 - Schoger, Simon A1 - Brenzinger, Kristof A1 - Kallnik, Katharina A1 - Sauer, Nikki A1 - Bofinger, Lukas A1 - Schmitt, Thomas A1 - Nooten, Sabine S. A1 - Classen, Alice T1 - Cuticular hydrocarbons of alpine bumble bees (Hymenoptera: Bombus) are species-specific, but show little evidence of elevation-related climate adaptation JF - Frontiers in Ecology and Evolution N2 - Alpine bumble bees are the most important pollinators in temperate mountain ecosystems. Although they are used to encounter small-scale successions of very different climates in the mountains, many species respond sensitively to climatic changes, reflected in spatial range shifts and declining populations worldwide. Cuticular hydrocarbons (CHCs) mediate climate adaptation in some insects. However, whether they predict the elevational niche of bumble bees or their responses to climatic changes remains poorly understood. Here, we used three different approaches to study the role of bumble bees’ CHCs in the context of climate adaptation: using a 1,300 m elevational gradient, we first investigated whether the overall composition of CHCs, and two potentially climate-associated chemical traits (proportion of saturated components, mean chain length) on the cuticle of six bumble bee species were linked to the species’ elevational niches. We then analyzed intraspecific variation in CHCs of Bombus pascuorum along the elevational gradient and tested whether these traits respond to temperature. Finally, we used a field translocation experiment to test whether CHCs of Bombus lucorum workers change, when translocated from the foothill of a cool and wet mountain region to (a) higher elevations, and (b) a warm and dry region. Overall, the six species showed distinctive, species-specific CHC profiles. We found inter- and intraspecific variation in the composition of CHCs and in chemical traits along the elevational gradient, but no link to the elevational distribution of species and individuals. According to our expectations, bumble bees translocated to a warm and dry region tended to express longer CHC chains than bumble bees translocated to cool and wet foothills, which could reflect an acclimatization to regional climate. However, chain lengths did not further decrease systematically along the elevational gradient, suggesting that other factors than temperature also shape chain lengths in CHC profiles. We conclude that in alpine bumble bees, CHC profiles and traits respond at best secondarily to the climate conditions tested in this study. While the functional role of species-specific CHC profiles in bumble bees remains elusive, limited plasticity in this trait could restrict species’ ability to adapt to climatic changes. KW - pollinators KW - altitudinal gradient KW - cuticular hydrocarbon KW - desiccation KW - mountain KW - global change KW - translocation experiment KW - drought stress Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-304420 SN - 2296-701X VL - 11 ER - TY - JOUR A1 - Luther, Christian H. A1 - Brandt, Philipp A1 - Vylkova, Slavena A1 - Dandekar, Thomas A1 - Müller, Tobias A1 - Dittrich, Marcus T1 - Integrated analysis of SR-like protein kinases Sky1 and Sky2 links signaling networks with transcriptional regulation in Candida albicans JF - Frontiers in Cellular and Infection Microbiology N2 - Fungal infections are a major global health burden where Candida albicans is among the most common fungal pathogen in humans and is a common cause of invasive candidiasis. Fungal phenotypes, such as those related to morphology, proliferation and virulence are mainly driven by gene expression, which is primarily regulated by kinase signaling cascades. Serine-arginine (SR) protein kinases are highly conserved among eukaryotes and are involved in major transcriptional processes in human and S. cerevisiae. Candida albicans harbors two SR protein kinases, while Sky2 is important for metabolic adaptation, Sky1 has similar functions as in S. cerevisiae. To investigate the role of these SR kinases for the regulation of transcriptional responses in C. albicans, we performed RNA sequencing of sky1Δ and sky2Δ and integrated a comprehensive phosphoproteome dataset of these mutants. Using a Systems Biology approach, we study transcriptional regulation in the context of kinase signaling networks. Transcriptomic enrichment analysis indicates that pathways involved in the regulation of gene expression are downregulated and mitochondrial processes are upregulated in sky1Δ. In sky2Δ, primarily metabolic processes are affected, especially for arginine, and we observed that arginine-induced hyphae formation is impaired in sky2Δ. In addition, our analysis identifies several transcription factors as potential drivers of the transcriptional response. Among these, a core set is shared between both kinase knockouts, but it appears to regulate different subsets of target genes. To elucidate these diverse regulatory patterns, we created network modules by integrating the data of site-specific protein phosphorylation and gene expression with kinase-substrate predictions and protein-protein interactions. These integrated signaling modules reveal shared parts but also highlight specific patterns characteristic for each kinase. Interestingly, the modules contain many proteins involved in fungal morphogenesis and stress response. Accordingly, experimental phenotyping shows a higher resistance to Hygromycin B for sky1Δ. Thus, our study demonstrates that a combination of computational approaches with integration of experimental data can offer a new systems biological perspective on the complex network of signaling and transcription. With that, the investigation of the interface between signaling and transcriptional regulation in C. albicans provides a deeper insight into how cellular mechanisms can shape the phenotype. KW - sky kinases KW - kinase signaling KW - network analysis KW - transcriptome KW - transcriptional regulation KW - phosphoproteome KW - Candida albicans Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-311771 SN - 2235-2988 VL - 13 ER - TY - THES A1 - Bakari Soale, Majeed T1 - Regulation of the Variant Surface Glycoprotein (VSG) Expression and Characterisation of the Nucleolar DExD/H box Protein Hel66 in \(Trypanosoma\) \(brucei\) T1 - Regulation der Expression des variable Oberflächen- Glykoprotein (VSG) und Charakterisierung des nukleolären DExD/H box Protein Hel66 in \(Trypanosoma\) \(brucei\) N2 - The variant surface glycoprotein (VSG) of African trypanosomes plays an essential role in protecting the parasites from host immune factors. These trypanosomes undergo antigenic variation resulting in the expression of a single VSG isoform out of a repertoire of around 2000 genes. The molecular mechanism central to the expression and regulation of the VSG is however not fully understood. Gene expression in trypanosomes is unusual due to the absence of typical RNA polymerase II promoters and the polycistronic transcription of genes. The regulation of gene expression is therefore mainly post-transcriptional. Regulatory sequences, mostly present in the 3´ UTRs, often serve as key elements in the modulation of the levels of individual mRNAs. In T. brucei VSG genes, a 100 % conserved 16mer motif within the 3´ UTR has been shown to modulate the stability of VSG transcripts and hence their expression. As a stability-associated sequence element, the absence of nucleotide substitutions in the motif is however unusual. It was therefore hypothesised that the motif is involved in other essential roles/processes besides stability of the VSG transcripts. In this study, it was demonstrated that the 100 % conservation of the 16mer motif is not essential for cell viability or for the maintenance of functional VSG protein levels. It was further shown that the intact motif in the active VSG 3´ UTR is neither required to promote VSG silencing during switching nor is it needed during differentiation from bloodstream forms to procyclic forms. Crosstalk between the VSG and procyclin genes during differentiation to the insect vector stage is also unaffected in cells with a mutated 16mer motif. Ectopic overexpression of a second VSG however requires the intact motif to trigger silencing and exchange of the active VSG, suggesting a role for the motif in transcriptional VSG switching. The 16mer motif therefore plays a dual role in VSG in situ switching and stability of VSG transcripts. The additional role of the 16mer in the essential process of antigenic variation appears to be the driving force for the 100 % conservation of this RNA motif. A screen aimed at identifying candidate RNA-binding proteins interacting with the 16mer motif, led to the identification of a DExD/H box protein, Hel66. Although the protein did not appear to have a direct link to the 16mer regulation of VSG expression, the DExD/H family of proteins are important players in the process of ribosome biogenesis. This process is relatively understudied in trypanosomes and so this candidate was singled out for detailed characterisation, given that the 16mer story had reached a natural end point. Ribosome biogenesis is a major cellular process in eukaryotes involving ribosomal RNA, ribosomal proteins and several non-ribosomal trans-acting protein factors. The DExD/H box proteins are the most important trans-acting protein factors involved in the biosynthesis of ribosomes. Several DExD/H box proteins have been directly implicated in this process in yeast. In trypanosomes, very few of this family of proteins have been characterised and therefore little is known about the specific roles they play in RNA metabolism. Here, it was shown that Hel66 is involved in rRNA processing during ribosome biogenesis. Hel66 localises to the nucleolus and depleting the protein led to a severe growth defect. Loss of the protein also resulted in a reduced rate of global translation and accumulation of rRNA processing intermediates of both the small and large ribosomal subunits. Hel66 is therefore an essential nucleolar DExD/H protein involved in rRNA processing during ribosome biogenesis. As very few protein factors involved in the processing of rRNAs have been described in trypanosomes, this finding represents an important platform for future investigation of this topic. N2 - Das variable Oberflächen-Glykoprotein (“varaint surface glycoprotein“, VSG) der Afrikanischen Trypanosomen schützt den Parasiten vor Immunfaktoren des Wirtes. Trypanosomen beherrschen die antigene Variation und expremieren nur eine einzige VSG Isoform aus einem Repertoire von ungefähr 2000 Genen. Der molekulare Mechanismus der die Expression dieser VSG Gene reguliert ist nicht komplett bekannt. Die Genexpression ist in Trypanosomen sehr ungewöhnlich. Es gibt keine typischen Promotoren für RNA Polymerase II und Gene werden polycistronisch transkribiert. Daher ist die Regulation der Genexpression hauptsächlich posttranskriptional. Die Expression individueller mRNAs wird durch regulatorische Sequenzen reguliert, die sich häufig in den 3´ UTRs befinden. In den VSG Genen von T. brucei moduliert ein zu 100% konserviertes 16mer Motiv in der 3´ UTR die Stabilität der VSG Transkripte und damit deren Expression. Für eine Sequenz, die die Stabilität der mRNA reguliert, ist das Fehlen von Nukleotid Substitutionen sehr ungewöhnlich. Es wurde deshalb spekuliert, dass das 16mer Motiv neben der Stabilisierung des VSG Transkriptes noch an anderen essentiellen Prozessen beteiligt ist. In dieser Arbeit wurde gezeigt, dass die 100%ige Konservierung des 16mer Motives weder für das Überleben der Zellen, noch für den Erhalt der Expression des VSG Protein in funktioneller Menge notwendig ist. Außerdem wurde gezeigt dass das intakte Motiv in der 3´UTR des aktiven VSGs weder für das „VSG silencing“ während des VSG Austausches („switching“) noch für die Differenzierung von Blutbahnformen zu prozyklischen Formen benötigt wird. Auch die Interaktionen („crosstalk“), die während der Differenzierung zum Insekten Stadium zwischen den VSG und Prozyklin Genen stattfinden, sind in Zellen mit mutiertem 16mer Motiv noch funktionell. Die ektopische Überexpression eines zweiten VSGs benötigt allerdings das intakte Motiv, um das aktive VSG zu inaktivieren und auszutauschen: dies suggeriert eine Rolle des Motivs im transkriptionalen „VSG switching“. Das 16mer Motif spielt daher eine Doppelrolle bei der Regulation der Stabilität der VSG Transkripte und im VSG in situ „switching“. Letzteres, die Rolle im essentiellen Prozess der antigenen Variation, ist dabei offensichtlich die treibende Kraft hinter der 100%igen Konservierung des RNA Motives. Eine Suche nach möglichen RNA bindenden Proteinen, die mit dem 16mer interagieren, führte zur Identifikation des DExD/H box Proteins Hel66. Obwohl das Protein wohl nicht direkt an der Regulation der VSG Expression über das 16mer beteiligt ist, spielen Mitglieder der DexD/H Proteinfamilie eine wichtige Rolle in der Biogenese von Ribosomen. Dieser Prozess ist in Trypanosomen noch nicht komplett verstanden und daher wurde das Protein für eine nähere Analyse ausgewählt, auch weil die 16mer Story ohne weitere Kandidaten zu einem Ende gekommen war. Die Biogenese von Ribosomen ist ein wichtiger zellulärer Prozess in Eukaryoten und benötigt ribosomale RNA, ribosomale Proteine sowie einige nicht-ribosomale, trans-agierende Protein Faktoren. Proteine der DExD/H box Familie sind die wichtigsten trans- agierenden Proteinfaktoren, die an der Biogenese der Ribosomen beteiligt sind. In der Hefe sind mehrere DExD/H box Proteine bekannt, die eine direkte Rolle in diesem Prozess spielen. In Trypanosomen sind erst sehr wenige Proteine aus dieser Familie untersucht worden und es ist daher kaum bekannt, welche spezifische Rollen sie im RNA Metabolismus spielen. In dieser Arbeit wurde gezeigt, dass Hel66 an der rRNA Prozessierung während der Biogenese der Ribosomen beteiligt ist. Hel66 ist im Nukleolus lokalisiert und die Reduktion des Proteins durch RNAi führte zu einem schweren Wachstumsphänotyp. Reduktion von Hel66 führte auch zu einer globalen Reduktion der Translation sowie zur Akkumulation von Synthese- Zwischenstadien der rRNAs sowohl der kleinen und als auch der großen ribosomalen Untereinheit. Hel66 ist daher ein essentielles nukleoläres DExD/H Protein dass an der Prozessierung der rRNA während der Biogenese der Ribosomen beteiligt ist. Da bisher erst wenige Proteine bekannt sind, die in Trypanosomen an diesem Prozess beteiligt sind, sind diese Ergebnisse ein sehr wichtiger Ausgangspunkt für weitere Untersuchungen in der Zukunft. KW - Trypanosoma brucei KW - Genexpression KW - Variant Surface Glycoprotein KW - VSG KW - DExD/H box protein KW - Ribosome biogenesis KW - rRNA processing KW - Ribosome Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-258090 ER - TY - JOUR A1 - Lu, Jinping A1 - Dreyer, Ingo A1 - Dickinson, Miles Sasha A1 - Panzer, Sabine A1 - Jaślan, Dawid A1 - Navarro-Retamal, Carlos A1 - Geiger, Dietmar A1 - Terpitz, Ulrich A1 - Becker, Dirk A1 - Stroud, Robert M. A1 - Marten, Irene A1 - Hedrich, Rainer T1 - Vicia faba SV channel VfTPC1 is a hyperexcitable variant of plant vacuole two pore channels JF - eLife N2 - To fire action-potential-like electrical signals, the vacuole membrane requires the two-pore channel TPC1, formerly called SV channel. The TPC1/SV channel functions as a depolarization-stimulated, non-selective cation channel that is inhibited by luminal Ca\(^{2+}\). In our search for species-dependent functional TPC1 channel variants with different luminal Ca\(^{2+}\) sensitivity, we found in total three acidic residues present in Ca\(^{2+}\) sensor sites 2 and 3 of the Ca\(^{2+}\)-sensitive AtTPC1 channel from Arabidopsis thaliana that were neutral in its Vicia faba ortholog and also in those of many other Fabaceae. When expressed in the Arabidopsis AtTPC1-loss-of-function background, wild-type VfTPC1 was hypersensitive to vacuole depolarization and only weakly sensitive to blocking luminal Ca\(^{2+}\). When AtTPC1 was mutated for these VfTPC1-homologous polymorphic residues, two neutral substitutions in Ca\(^{2+}\) sensor site 3 alone were already sufficient for the Arabidopsis At-VfTPC1 channel mutant to gain VfTPC1-like voltage and luminal Ca\(^{2+}\) sensitivity that together rendered vacuoles hyperexcitable. Thus, natural TPC1 channel variants exist in plant families which may fine-tune vacuole excitability and adapt it to environmental settings of the particular ecological niche. KW - A. thaliana KW - Brassicaceae KW - Fabaceae KW - pore KW - potassium channel KW - voltage gating KW - vacuolar calcium sensor Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-350264 VL - 12 ER - TY - JOUR A1 - Thomas, Sarah A1 - Fiebig, Juliane E. A1 - Kuhn, Eva-Maria A1 - Mayer, Dominik S. A1 - Filbeck, Sebastian A1 - Schmitz, Werner A1 - Krischke, Markus A1 - Gropp, Roswitha A1 - Mueller, Thomas D. T1 - Design of glycoengineered IL-4 antagonists employing chemical and biosynthetic glycosylation JF - ACS Omega N2 - Interleukin-4 (IL-4) plays a key role in atopic diseases. It coordinates T-helper cell differentiation to subtype 2, thereby directing defense toward humoral immunity. Together with Interleukin-13, IL-4 further induces immunoglobulin class switch to IgE. Antibodies of this type activate mast cells and basophilic and eosinophilic granulocytes, which release pro-inflammatory mediators accounting for the typical symptoms of atopic diseases. IL-4 and IL-13 are thus major targets for pharmaceutical intervention strategies to treat atopic diseases. Besides neutralizing antibodies against IL-4, IL-13, or its receptors, IL-4 antagonists can present valuable alternatives. Pitrakinra, an Escherichia coli-derived IL-4 antagonist, has been evaluated in clinical trials for asthma treatment in the past; however, deficits such as short serum lifetime and potential immunogenicity among others stopped further development. To overcome such deficits, PEGylation of therapeutically important proteins has been used to increase the lifetime and proteolytic stability. As an alternative, glycoengineering is an emerging strategy used to improve pharmacokinetics of protein therapeutics. In this study, we have established different strategies to attach glycan moieties to defined positions in IL-4. Different chemical attachment strategies employing thiol chemistry were used to attach a glucose molecule at amino acid position 121, thereby converting IL-4 into a highly effective antagonist. To enhance the proteolytic stability of this IL-4 antagonist, additional glycan structures were introduced by glycoengineering utilizing eucaryotic expression. IL-4 antagonists with a combination of chemical and biosynthetic glycoengineering could be useful as therapeutic alternatives to IL-4 neutralizing antibodies already used to treat atopic diseases. KW - Interleukin-4 (IL-4) KW - atopic diseases KW - IL-4 antagonists KW - glycoengineering KW - biosynthetic glycosylation KW - chemical glycosylation Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-350278 SN - 2470-1343 VL - 8 IS - 28 ER - TY - JOUR A1 - Adam, Alexander A1 - Deimel, Stephan A1 - Pardo-Medina, Javier A1 - García-Martínez, Jorge A1 - Konte, Tilen A1 - Limón, M. Carmen A1 - Avalos, Javier A1 - Terpitz, Ulrich T1 - Protein activity of the \(Fusarium\) \(fujikuroi\) rhodopsins CarO and OpsA and their relation to fungus−plant interaction JF - International Journal of Molecular Sciences N2 - Fungi possess diverse photosensory proteins that allow them to perceive different light wavelengths and to adapt to changing light conditions in their environment. The biological and physiological roles of the green light-sensing rhodopsins in fungi are not yet resolved. The rice plant pathogen Fusarium fujikuroi exhibits two different rhodopsins, CarO and OpsA. CarO was previously characterized as a light-driven proton pump. We further analyzed the pumping behavior of CarO by patch-clamp experiments. Our data show that CarO pumping activity is strongly augmented in the presence of the plant hormone indole-3-acetic acid and in sodium acetate, in a dose-dependent manner under slightly acidic conditions. By contrast, under these and other tested conditions, the Neurospora rhodopsin (NR)-like rhodopsin OpsA did not exhibit any pump activity. Basic local alignment search tool (BLAST) searches in the genomes of ascomycetes revealed the occurrence of rhodopsin-encoding genes mainly in phyto-associated or phytopathogenic fungi, suggesting a possible correlation of the presence of rhodopsins with fungal ecology. In accordance, rice plants infected with a CarO-deficient F. fujikuroi strain showed more severe bakanae symptoms than the reference strain, indicating a potential role of the CarO rhodopsin in the regulation of plant infection by this fungus. KW - fungal rhodopsins KW - CarO KW - OpsA KW - Fusarium fujikuroi KW - Oryza sativa KW - rice–plant infection KW - green light perception KW - indole-3-acetic acid (IAA) KW - bakanae KW - patch-clamp Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-285125 SN - 1422-0067 VL - 19 IS - 1 ER - TY - JOUR A1 - Moris, Victoria C. A1 - Christmann, Katharina A1 - Wirtgen, Aline A1 - Belokobylskij, Sergey A. A1 - Berg, Alexander A1 - Liebig, Wolf-Harald A1 - Soon, Villu A1 - Baur, Hannes A1 - Schmitt, Thomas A1 - Niehuis, Oliver T1 - Cuticular hydrocarbons on old museum specimens of the spiny mason wasp, Odynerus spinipes (Hymenoptera: Vespidae: Eumeninae), shed light on the distribution and on regional frequencies of distinct chemotypes JF - Chemoecology N2 - The mason wasp Odynerus spinipes shows an exceptional case of intrasexual cuticular hydrocarbon (CHC) profile dimorphism. Females of this species display one of two CHC profiles (chemotypes) that differ qualitatively and quantitatively from each other. The ratio of the two chemotypes was previously shown to be close to 1:1 at three sites in Southern Germany, which might not be representative given the Palearctic distribution of the species. To infer the frequency of the two chemotypes across the entire distributional range of the species, we analyzed with GC–MS the CHC profile of 1042 dry-mounted specimens stored in private and museum collections. We complemented our sampling by including 324 samples collected and preserved specifically for studying their CHCs. We were capable of reliably identifying the chemotypes in 91% of dry-mounted samples, some of which collected almost 200 years ago. We found both chemotypes to occur in the Far East, the presumed glacial refuge of the species, and their frequency to differ considerably between sites and geographic regions. The geographic structure in the chemotype frequencies could be the result of differential selection regimes and/or different dispersal routes during the colonization of the Western Palearctic. The presented data pave the route for disentangling these factors by providing information where to geographically sample O. spinipes for population genetic analyses. They also form the much-needed basis for future studies aiming to understand the evolutionary and geographic origin as well as the genetics of the astounding CHC profile dimorphism that O. spinipes females exhibit. KW - cuticular hydrocarbons KW - chemotypes KW - dry-mounted samples KW - collections KW - distribution Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-306999 SN - 0937-7409 SN - 1423-0445 VL - 31 IS - 5 ER - TY - THES A1 - Maier [verh. Hartmann], Carina Ramona T1 - Regulation of the Mevalonate Pathway by the Deubiquitinase USP28 in Squamous Cancer T1 - Regulation des Mevalonat Stoffwechselwegs durch die Deubiquitinase USP28 in Plattenepithelkarzinomen N2 - The reprogramming of metabolic pathways is a hallmark of cancer: Tumour cells are dependent on the supply with metabolites and building blocks to fulfil their increased need as highly proliferating cells. Especially de novo synthesis pathways are upregulated when the cells of the growing tumours are not able to satisfy the required metabolic levels by uptake from the environment. De novo synthesis pathways are often under the control of master transcription factors which regulate the gene expression of enzymes involved in the synthesis process. The master regulators for de novo fatty acid synthesis and cholesterogenesis are sterol regulatory element-binding proteins (SREBPs). While SREBP1 preferably controls the expression of enzymes involved in fatty acid synthesis, SREBP2 regulates the transcription of the enzymes of the mevalonate pathway and downstream processes namely cholesterol, isoprenoids and building blocks for ubiquinone synthesis. SREBP activity is tightly regulated at different levels: The post-translational modification by ubiquitination decreases the stability of active SREBPs. The attachment of K48-linked ubiquitin chains marks the transcription factors for the proteasomal degradation. In tumour cells, high levels of active SREBPs are essential for the upregulation of the respective metabolic pathways. The increased stability and activity of SREBPs were investigated in this thesis. SREBPs are ubiquitinated by the E3 ligase Fbw7 which leads to the subsequential proteolysis of the transcription factors. The work conducted in this thesis identified the counteracting deubiquitination enzyme USP28 which removes the ubiquitin chains from SREBPs and prevents their proteasomal degradation. It further revealed that the stabilization of SREBP2 by USP28 plays an important role in the context of squamous cancers. Increased USP28 levels are associated with a poor survival in patients with squamous tumour subtypes. It was shown that reduced USP28 levels in cell lines and in vivo result in a decrease of SREBP2 activity and downregulation of the mevalonate pathway. This manipulation led to reduced proliferation and tumour growth. A direct comparison of adenocarcinomas and squamous cell carcinomas in lung cancer patients revealed an upregulation of USP28 as well as SREBP2 and its target genes. Targeting the USP28-SREBP2 regulatory axis in squamous cell lines by inhibitors also reduced cell viability and proliferation. In conclusion, this study reports evidence for the importance of the mevalonate pathway regulated by the USP28-SREBP2 axis in tumour initiation and progression of squamous cancer. The combinatorial inhibitor treatment of USP28 and HMGCR, the rate limiting enzyme of the mevalonate pathway, by statins opens the possibility for a targeted therapeutic treatment of squamous cancer patients. N2 - Die Reprogrammierung metabolischer Stoffwechselwege ist ein Kennzeichen von Krebs: Tumorzellen sind abhängig von der Versorgung mit Metaboliten und Bausteinen, um ihren wachsenden Bedarf als hoch proliferierende Zellen zu decken. Vor allem die de novo Stoffwechselsynthesewege sich hochreguliert, wenn die Zellen des wachsenden Tumors nicht mehr in der Lage sind, ihr erforderliches metabolisches Niveau mithilfe der Aufnahme aus der Umgebung zu erfüllen. De novo Synthesewege sind oft unter der Kontrolle von zentralen Transkriptionsfaktoren die die Genexpression von Enzymen, die im Syntheseprozess beteiligt sind, regulieren. Die vorherrschenden Regulatoren, für die de novo Fettsäuresynthese und der Cholesterogenese sind die Steroid-regulatorisches-Element-bindende Proteine (SREBPs). Während SREBP1 bevorzugt die Expression von Enzymen die an der Fettsäuresynthese beteiligt sind kontrolliert, reguliert SREBP2 die Transkription von Enzymen des Mevalonat Stoffwechselwegs, sowie Prozesse unterhalb, namentlich die Cholesterol-, Isoprenoid- und die die Synthese von Bausteinen für die Ubiquinonsynthese. Die Aktivität von SREBP ist streng reguliert auf verschiedenen Ebenen: Die post-translationale Modifikation mittels Ubiquitinierung reduziert die Stabilität von aktiven SREBPs. Das Anhängen von K48-verlinkten Ubiquitinketten markiert die Transkriptionsfaktoren für den proteasomalen Abbau. In Tumorzellen sind hohe Niveaus von aktiven SREBPs essentiell für die Induktion der entsprechenden metabolischen Stoffwechselwege. Die erhöhte Stabilität und Aktivität von SREBPs wurden im Rahmen dieser Arbeit untersucht. SREBPs werden von der E3-Ligase Fbw7 ubiquitiniert, was zur Proteolyse der Transkriptionsfaktoren führt. In dieser Arbeit wurde gezeigt, dass das entgegenwirkende Deubiquitinierungsenzym USP28 die Ubiquitinketten von SREBPs entfernt und deren proteasomalen Abbau verhindert. Diese Forschungsarbeit zeigt weiterhin, dass die Stabilisierung von SREBP2 durch USP28 eine wichtige Rolle im Kontext von Epithelkarzinomen spielt. Erhöhte USP28 Niveaus werden mit einem schlechten Überleben von Patienten in der Krebs-Untergruppe der Plattenepithelkarzinomen verbunden. Es konnte gezeigt werden, dass reduzierte USP28 Niveaus, in Zelllinien und in vivo, niedrigere SREBP2-Aktivität und eine Herunterregulierung des Mevalonat Stoffwechselwegs ergeben. Diese Manipulation führte zu reduzierter Proliferation und Tumorwachstum. Ein direkter Vergleich von Adenokarzinomen und Plattenepithelkarzinomen in Lungenkrebspatienten zeigte zudem eine Hochregulierung von USP28 ebenso wie SREBP2 und dessen Zielgenen. Der gezielte Einsatz von Inhibitoren gegen die USP28-SREBP2 regulatorische Achse in Plattenepithelzellen reduzierte die Lebensfähigkeit und Proliferation der Zellen. Abschließend berichtet diese Forschungsarbeit von der Bedeutung des durch die USP28-SREBP2 Achse regulierten Mevalonat Stoffwechselwegs bei der Tumorinitiation und dem Fortschreiten von Plattenepithelkarzinomen. Die kombinatorische Behandlung mit USP28- und Inhibitoren der HMGCR, dem Schlüsselenzym des Mevalonat Stoffwechselwegs, mithilfe von Statinen eröffnet die Möglichkeit für eine gezielte therapeutische Behandlung von Patienten mit Plattenepithelkarzinomen. KW - Ubiquitin KW - Metabolismus KW - Deubiquitination KW - Mevalonate Pathway KW - Cancer Metabolism KW - Lung squamous cancer cells Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-348740 ER - TY - THES A1 - Pitsch, Maximilian Jonathan T1 - Zyklisches Adenosinmonophosphat (cAMP) als Äquivalent akkumulierter neuronaler Evidenz T1 - Cyclic adenosine monophosphate (cAMP) as an equivalent of accumulated neuronal evidence N2 - Die vier Crz-Neurone des ventralen Nervensystems von Drosophila melanogaster sammeln Evidenz, wann im Rahmen eines Paarungsakts zirka 6 Minuten vergangen sind. Diese Entscheidung ist für die männliche Fliege von Bedeutung, da das Männchen vor Ablauf dieser ~6 Minuten, welche den Zeitpunkt der Ejakulation darstellen, eher das eigene Leben opfern würde, als dass es die Paarung beenden würde. Nach Ablauf der ~6 Minuten fällt die Motivation des Männchens dagegen dramatisch ab. Im Rahmen der vorliegenden Arbeit wurde zunächst mittels optogenetischer neuronaler Inhibitionsprotokolle sowie Verhaltensanalysen das Phänomen der Evidenz-akkumulation in den Crz-Neuronen genauer charakterisiert. Dabei zeigte sich, dass die akkumulierte Evidenz auch während einer elektrischen Inhibition der Crz-Neurone persistierte. Dieses Ergebnis warf die Hypothese auf, dass das Äquivalent der akkumulierten Evidenz in den Crz-Neuronen biochemischer Natur sein könnte. Es wurde daraufhin ein Hochdurchsatzscreening-Verfahren entwickelt, mittels dessen 1388 genetische Manipulationen der Crz-Neurone durchgeführt und auf eine Änderung der Evidenzakkumulation getestet wurden. Nur ~30 genetische Manipulationen zeigten eine veränderte Evidenzakkumulation, wobei die meisten dieser Manipulationen den cAMP-Signalweg betrafen. Mittels der optogenetischen Photoadenylatzyklase bPAC, einer Reihe weiterer genetischer Manipulationen des cAMP-Signalwegs sowie der ex vivo Kalzium-Bildgebung und Fluoreszenzlebensdauer-Mikroskopie konnte bestätigt werden, dass cAMP das Äquivalent der in den Crz-Neuronen spannungsabhängig akkumulierten Evidenz darstellt, wobei die Kombination dieser Methoden nahelegte, dass der Schwellenwert der Evidenzakkumulation durch die cAMP-Bindungsaffinität der regulatorischen PKA-Untereinheiten festgelegt sein könnte. Mittels genetischer Mosaikexperimente sowie bildgebenden Verfahren konnte darüber hinaus gezeigt werden, dass innerhalb des Crz-Netzwerks eine positive Rückkopplungsschleife aus rekurrenter Aktivität sowie der cAMP-Akkumulation besteht, welche, sobald die cAMP-Spiegel den Schwellenwert erreichen, zu einem netzwerkweit synchronisierten massiven Kalziumeinstrom führt, was die Abgabe des Crz-Signals an nachgeschaltete Netzwerke triggert. Dieses Phänomen könnte ein Analogon des Aktionspotenzials auf Netzwerkebene sowie auf Intervallzeitskalen darstellen und wurde als „Eruption“ bezeichnet. Genetische, optogenetische sowie Bildgebungsexperimente konnten zeigen, dass die CaMKII derartige Eruptionen durch Niedrighalten der cAMP-Spiegel unterdrückt, was den Zeitmessmechanismus des ersten beschriebenen Intervallzeitmessers CaMKII offenlegt. N2 - The four Crz neurons of the ventral nervous system of Drosophila melanogaster collect evidence about when approximately 6 minutes have elapsed during a mating act. This decision is of importance for the male fly as the male would rather sacrifice his own life than terminate mating before the expiration of these ~6 minutes, which represent the time of ejaculation. After these ~6 minutes, however, the male's motivation drops dramatically. In this dissertation, optogenetic neuronal inhibition protocols as well as behavioral analyses were used to characterize the phenomenon of evidence accumulation in the Crz neurons in more detail. This showed that the accumulated evidence persisted during electrical inhibition of the Crz neurons. This result raised the hypothesis that the equivalent of accumulated evidence in the Crz neurons might be biochemical in nature. A high-throughput-screening-assay was developed using which 1388 genetic manipulations of the Crz neurons were performed and tested for a change in evidence accumulation. Only ~30 genetic manipulations showed altered evidence accumulation, with most of these manipulations involving the cAMP pathway. Using the optogenetic photoadenylyl cyclase bPAC, a number of other genetic manipulations of the cAMP pathway, as well as ex vivo calcium imaging and fluorescence lifetime microscopy techniques, it was confirmed that cAMP represents the equivalent of accumulated evidence in the Crz neurons, and the combination of these methods suggested that the evidence accumulation threshold may be set by the cAMP-binding affinity of regulatory PKA subunits. Using genetic mosaic experiments as well as imaging techniques, it was further shown that within the Crz network there is a positive feedback loop between the recurrent activity as well as the cAMP accumulation, which, once cAMP levels reach the threshold, leads to a network-wide synchronized massive calcium influx, triggering the delivery of the Crz signal to downstream networks. This phenomenon could represent an analog of the action potential at the network level as well as at interval time scales and has been termed an "eruption." Genetic, optogenetic as well as imaging experiments could show that CaMKII suppresses such eruptions by keeping cAMP levels low, revealing the timing mechanism of CaMKII, the first described interval timer. KW - Evidenz KW - Drosophila KW - Biologische Uhr KW - cAMP KW - Intervallzeitmessung Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-351292 ER - TY - THES A1 - Adhikari, Bikash T1 - Targeted degradation of Myc-interacting oncoproteins T1 - Gezielte Degradation von mit Myc interagierenden Onkoproteinen N2 - The hallmark oncoprotein Myc is a major driver of tumorigenesis in various human cancer entities. However, Myc’s structural features make it challenging to develop small molecules against it. A promising strategy to indirectly inhibit the function of Myc is by targeting its interactors. Many Myc-interacting proteins have reported scaffolding functions which are difficult to target using conventional occupancy- driven inhibitors. Thus, in this thesis, the proteolysis targeting chimera (PROTAC) approach was used to target two oncoproteins interacting with Myc which promote the oncogenicity of Myc, Aurora-A and WDR5. PROTACs are bifunctional small molecules that bind to the target protein with one ligand and recruit a cellular E3- ligase with the other ligand to induce target degradation via the ubiquitin- proteasome system. So far, the most widely used E3-ligases for PROTAC development are Cereblon (CRBN) and von Hippel–Lindau tumor suppressor (VHL). Furthermore, there are cases of incompatibility between some E3-ligases and proteins to bring about degradation. Hence there is a need to explore new E3- ligases and a demand for a tool to predict degradative E3-ligases for the target protein in the PROTAC field. In the first part, a highly specific mitotic kinase Aurora-A degrader, JB170, was developed. This compound utilized Aurora-A inhibitor alisertib as the target ligand and thalidomide as the E3-ligase CRBN harness. The specificity of JB170 and the ternary complex formation was supported by the interactions between Aurora-A and CRBN. The PROTAC-mediated degradation of Aurora-A induced a distinct S- phase defect rather than mitotic arrest, shown by its catalytic inhibition. The finding demonstrates that Aurora-A has a non-catalytic role in the S-phase. Furthermore, the degradation of Aurora-A led to apoptosis in various cancer cell lines. In the second part, two different series of WDR5 PROTACs based on two protein- protein inhibitors of WDR5 were evaluated. The most efficient degraders from both series recruited VHL as a E3-ligase and showed partial degradation of WDR5. In addition, the degradation efficiency of the PROTACs was significantly affected by the linker nature and length, highlighting the importance of linker length and composition in PROTAC design. The degraders showed modest proliferation defects at best in cancer cell lines. However, overexpression of VHL increased the degradation efficiency and the antiproliferative effect of the PROTACs. In the last part, a rapamycin-based assay was developed to predict the degradative E3-ligase for a target. The assay was validated using the WDR5/VHL and Aurora- A/CRBN pairs. The result that WDR5 is degraded by VHL but not CRBN and Aurora-A is degraded by CRBN, matches observations made with PROTACs. This technique will be used in the future to find effective tissue-specific and essential E3-ligases for targeted degradation of oncoproteins using PROTACs. Collectively, the work presented here provides a strategy to improve PROTAC development and a starting point for developing Aurora-A and WDR5 PROTACs for cancer therapy. N2 - Das Onkoprotein Myc ist ein wichtiger Faktor bei der Tumorentstehung in verschiedenen menschlichen Krebsarten. Die strukturellen Merkmale von Myc machen es jedoch schwierig, kleine Moleküle gegen dieses Protein zu entwickeln. Eine vielversprechende Strategie zur indirekten Hemmung der Funktion von Myc besteht darin, auf seine Interaktoren abzuzielen. Viele Proteine, die mit Myc interagieren, haben Gerüstfunktionen, die mit herkömmlichen Inhibitoren nur schwer zu hemmen sind. Daher wurde in dieser Arbeit der PROTAC-Ansatz (Proteolysis Targeting Chimera) verwendet, um zwei Onkoproteine, die mit Myc interagieren und die Onkogenität von Myc fördern, ins Visier zu nehmen: Aurora-A und WDR5. PROTACs sind bifunktionale kleine Moleküle, die mit einem Liganden an das Zielprotein binden und mit dem anderen Liganden eine zelluläre E3-Ligase rekrutieren, um den Abbau des Zielproteins über das Ubiquitin-Proteasom-System einzuleiten. Die bisher am häufigsten verwendeten E3-Ligasen für die Entwicklung von PROTACs sind Cereblon (CRBN) und der von Hippel-Lindau-Tumorsuppressor (VHL). Außerdem gibt es Fälle von Inkompatibilität zwischen einigen E3-Ligasen und Proteinen, die abgebaut werden sollen. Daher besteht die Notwendigkeit, neue E3-Ligasen zu erforschen und Werkzeuge zur Vorhersage abbauender E3-Ligasen für das Zielprotein zu entwickeln. Im ersten Teil wurde ein hochspezifischer Degrader der mitotischen Kinase Aurora-A, JB170, entwickelt. Bei dieser Verbindung wurde der Aurora-A-Inhibitor Alisertib als Zielligand und Thalidomid als Binder für die E3-Ligase CRBN verwendet. Die Spezifität von JB170 und die ternäre Komplexbildung wurden durch die Wechselwirkungen zwischen Aurora-A und CRBN unterstützt. Der durch PROTAC vermittelte Abbau von Aurora-A führte zu einem deutlichen Defekt in der S-Phase und nicht zu einem mitotischen Stillstand, wie es für dessen katalytische Hemmung beobachtet wurde. Dies zeigt, dass Aurora-A eine nicht-katalytische Funktion in der S-Phase hat. Außerdem führte der Abbau von Aurora-A in verschiedenen Krebszelllinien zur Apoptose. Im zweiten Teil wurden zwei verschiedene Serien von WDR5 PROTACs auf der Grundlage von zwei Protein-Protein-Inhibitoren von WDR5 untersucht. Die effizientesten Degrader aus beiden Serien rekrutierten VHL als E3-Ligase und zeigten einen teilweisen Abbau von WDR5. Darüber hinaus wurde die Abbaueffizienz der PROTACs erheblich von der Art und Länge des Linkers beeinflusst, was die Bedeutung der Linkerlänge und -zusammensetzung bei der Entwicklung von PROTACs unterstreicht. Die Abbauprodukte zeigten bestenfalls bescheidene Proliferationsdefekte in Krebszelllinien. Eine Überexpression von VHL erhöhte jedoch die Abbaueffizienz und den antiproliferativen Effekt der PROTACs. Im letzten Teil wurde ein auf Rapamycin basierender Assay entwickelt, um die abbauende E3-Ligase für ein Target vorherzusagen. Der Assay wurde anhand der Paare WDR5/VHL und Aurora-A/CRBN validiert. Das Ergebnis, dass WDR5 von VHL, aber nicht von CRBN abgebaut wird und Aurora-A von CRBN abgebaut wird, stimmt mit den Beobachtungen überein, die mit PROTACs gemacht wurden. Diese Technik wird in Zukunft eingesetzt werden, um wirksame gewebespezifische und essentielle E3-Ligasen für den gezielten Abbau von Onkoproteinen mit Hilfe von PROTACs zu finden. Insgesamt bieten die hier vorgestellten Arbeiten eine Strategie zur Verbesserung der PROTAC-Entwicklung und einen Ausgangspunkt für die Entwicklung von Aurora-A- und WDR5-PROTACs für die Krebstherapie. KW - Degradation KW - PROTACs KW - Oncoprotein KW - Cancer KW - Onkoprotein Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-317326 ER - TY - INPR A1 - Odenwald, Johanna A1 - Gabiatti, Bernardo A1 - Braune, Silke A1 - Shen, Siqi A1 - Zoltner, Martin A1 - Kramer, Susanne T1 - Beyond BioID: Streptavidin outcompetes antibody fluorescence signals in protein localization and readily visualises targets evading immunofluorescence detection T2 - eLife N2 - Immunofluorescence is a common method to localise proteins within their cellular context via fluorophore labelled antibodies and for some applications without alternative. However, some protein targets evade detection due to low protein abundance or accessibility issues. In addition, some imaging methods require a massive reduction in antigen density thus impeding detection of even medium-abundant proteins.Here, we show that the fusion of the target protein to TurboID, a biotin ligase labelling lysine residues in close proximity, and subsequent detection of biotinylation by fluorescent streptavidin offers an “all in one” solution to the above-mentioned restrictions. For a wide range of target proteins tested, the streptavidin signal was significantly stronger than an antibody signal, markedly improving the imaging sensitivity in expansion microscopy and correlative light and electron microscopy, with no loss in resolution. Importantly, proteins within phase-separated regions, such as the central channel of the nuclear pores, the nucleolus or RNA granules, were readily detected with streptavidin, while most antibodies fail to label proteins in these environments. When TurboID is used in tandem with an HA epitope tag, co-probing with streptavidin and anti-HA can be used to map antibody-accessibility to certain cellular regions. As a proof of principle, we mapped antibody access to all trypanosome nuclear pore proteins (NUPs) and found restricted antibody labelling of all FG NUPs of the central channel that are known to be phase-separated, while most non-FG Nups could be labelled. Lastly, we show that streptavidin imaging can resolve dynamic, temporally and spatially distinct sub-complexes and, in specific cases, reveal a history of dynamic protein interaction.In conclusion, streptavidin imaging has major advantages for the detection of lowly abundant or inaccessible proteins and in addition, can provide information on protein interactions and biophysical environment. KW - BioID KW - Streptavidin KW - antibody fluorescence signals KW - protein localization KW - immunofluorescence detection Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-360704 ER - TY - JOUR A1 - Osmanoglu, Özge A1 - Gupta, Shishir K. A1 - Almasi, Anna A1 - Yagci, Seray A1 - Srivastava, Mugdha A1 - Araujo, Gabriel H. M. A1 - Nagy, Zoltan A1 - Balkenhol, Johannes A1 - Dandekar, Thomas T1 - Signaling network analysis reveals fostamatinib as a potential drug to control platelet hyperactivation during SARS-CoV-2 infection JF - Frontiers in Immunology N2 - Introduction Pro-thrombotic events are one of the prevalent causes of intensive care unit (ICU) admissions among COVID-19 patients, although the signaling events in the stimulated platelets are still unclear. Methods We conducted a comparative analysis of platelet transcriptome data from healthy donors, ICU, and non-ICU COVID-19 patients to elucidate these mechanisms. To surpass previous analyses, we constructed models of involved networks and control cascades by integrating a global human signaling network with transcriptome data. We investigated the control of platelet hyperactivation and the specific proteins involved. Results Our study revealed that control of the platelet network in ICU patients is significantly higher than in non-ICU patients. Non-ICU patients require control over fewer proteins for managing platelet hyperactivity compared to ICU patients. Identification of indispensable proteins highlighted key subnetworks, that are targetable for system control in COVID-19-related platelet hyperactivity. We scrutinized FDA-approved drugs targeting indispensable proteins and identified fostamatinib as a potent candidate for preventing thrombosis in COVID-19 patients. Discussion Our findings shed light on how SARS-CoV-2 efficiently affects host platelets by targeting indispensable and critical proteins involved in the control of platelet activity. We evaluated several drugs for specific control of platelet hyperactivity in ICU patients suffering from platelet hyperactivation. The focus of our approach is repurposing existing drugs for optimal control over the signaling network responsible for platelet hyperactivity in COVID-19 patients. Our study offers specific pharmacological recommendations, with drug prioritization tailored to the distinct network states observed in each patient condition. Interactive networks and detailed results can be accessed at https://fostamatinib.bioinfo-wuerz.eu/. KW - signaling network KW - controllability KW - platelet KW - SARS-CoV-2 KW - fostamatinib KW - drug repurposing KW - COVID-19 Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-354158 VL - 14 ER - TY - THES A1 - Dehmer, Markus T1 - A novel USP11-TCEAL1-mediated mechanism protects transcriptional elongation by RNA Polymerase II T1 - Ein neuer USP11-TCEAL1 vermittelter Mechanismus schützt die transkriptionelle Elongation der RNA Polymerase II N2 - Deregulated expression of MYC oncoproteins is a driving event in many human cancers. Therefore, understanding and targeting MYC protein-driven mechanisms in tumor biology remain a major challenge. Oncogenic transcription in MYCN-amplified neuroblastoma leads to the formation of the MYCN-BRCA1-USP11 complex that terminates transcription by evicting stalling RNAPII from chromatin. This reduces cellular stress and allows reinitiation of new rounds of transcription. Basically, tumors with amplified MYC genes have a high demand on well orchestration of transcriptional processes-dependent and independent from MYC proteins functions in gene regulation. To date, the cooperation between promoter-proximal termination and transcriptional elongation in cancer cells remains still incomplete in its understanding. In this study the putative role of the dubiquitinase Ubiquitin Specific Protease 11 (USP11) in transcription regulation was further investigated. First, several USP11 interaction partners involved in transcriptional regulation in neuroblastoma cancer cells were identified. In particular, the transcription elongation factor A like 1 (TCEAL1) protein, which assists USP11 to engage protein-protein interactions in a MYCN-dependent manner, was characterized. The data clearly show that TCEAL1 acts as a pro-transcriptional factor for RNA polymerase II (RNAPII)-medi- ated transcription. In detail, TCEAL1 controls the transcription factor S-II (TFIIS), a factor that assists RNAPII to escape from paused sites. The findings claim that TCEAL1 outcompetes the transcription elongation factor TFIIS in a non-catalytic manner on chromatin of highly expressed genes. This is reasoned by the need regulating TFIIS function in transcription. TCEAL1 equili- brates excessive backtracking and premature termination of transcription caused by TFIIS. Collectively, the work shed light on the stoichiometric control of TFIIS demand in transcriptional regulation via the USP11-TCEAL1-USP7 complex. This complex protects RNAPII from TFIIS-mediated termination helping to regulate productive transcription of highly active genes in neuroblastoma. N2 - Die deregulierte Expression von MYC Onkoproteinen ist ein zentrales Event in vielen huma-nen Krebsarten. Aus diesem Grund sind das Verständnis und die gezielte Bekämpfung MYC-getriebener Mechanismen in der Tumorbiologie nach wie vor eine große Herausforderung. In MYCN-amplifizierten Neuroblastomen führt eine übermäßig hohe Transkriptionsrate zur stress-bedingten Rekrutierung des MYCN-BRCA1-USP11-Komplexes. Dieser Komplex be-endet vorzeitig die Transkription, indem er RNAPII Moleküle vom Chromatin wirft. Durch diesen Mechanismus wird zellulärer Stress reduziert und ermöglicht dadurch einen erneuten Start der Transkription. Grundsätzlich stellen Tumoren mit einer Amplifikation von einem der MYC Proteine hohe Anforderungen an eine feine Abstimmung der einzelnen Schritte in der Transkription. Dies ist sowohl abhängig als auch unabhängig von den bereits beschriebe-nen Funktionen der MYC-Proteine in der Genregulation. Bis heute ist das Zusammenspiel zwischen promoter-proximaler Termination und transkriptioneller Elongation noch nicht vollständig aufgeklärt. In dieser Studie wurde eine potenzielle Rolle von USP11 in der Regulation der Transkription weitergehend untersucht. Zunächst wurden mehrere Interaktionspartner von USP11, die an der Regulation der Transkription in Neuroblastom Krebszellen beteiligt sind, identifiziert. Es wurde insbesondere das Transcription Elongation Factor A Like 1 (TCEAL1) Protein charak-terisiert. Dieses Protein unterstützt USP11 dabei, Protein-Protein-Interaktionen MYCN-vermittelt einzugehen. Die Daten zeigen, dass TCEAL1 als pro-transkriptioneller Faktor für die RNA-Polymerase II (RNAPII) -vermittelte Transkription fungiert. Genauer, TCEAL1 kontrolliert den Transkriptionsfaktor S-II (TFIIS), einen Faktor, der der RNAPII dabei hilft, die Transkription nach einem kurzen Pausieren („pausing“) fortzusetzen. Die Ergebnisse zei-gen, dass TCEAL1 den Elongationsfaktor TFIIS auf nicht-katalytische Weise von dem Chromatin von hochexprimierten Genen verdrängt. Dies ist darin begründet, dass die Funkti-on von TFIIS bei der Transkription reguliert werden muss. TCEAL1 gleicht übermäßiges Zurückwandern der RNAPII und die vorzeitige Beendigung der Transkription, das durch TFIIS vermittelt wird, aus. Diese Arbeit gibt Aufschluss über die stöchiometrische Kontrolle des TFIIS-Bedarfs bei der Transkriptionsregulation durch den USP11-TCEAL1-USP7-Komplex. Dieser Komplex schützt die RNAPII vor der TFIIS-vermittelter Termination der Transkription und trägt zur Regulierung einer produktiven Transkription hochaktiver Gene im Neuroblastom bei. KW - Transkription KW - N-Myc KW - Transcription Regulation KW - Pause Release KW - Ubiquitin Specific Protease 11 KW - transcription elongation factor A (SII)-like 1 (TCEAL1) KW - RNA Polymerase II (RNAPII) KW - Transcriptional Stress Response Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-360544 ER - TY - THES A1 - Schwebs, Marie T1 - Structure and dynamics of the plasma membrane: a single-molecule study in \(Trypanosoma\) \(brucei\) T1 - Die Struktur und Dynamik der Plasmamembran: eine Einzelmolekülstudie in \(Trypanosoma\) \(brucei\) N2 - The unicellular, flagellated parasite Trypanosoma brucei is the causative agent of human African sleeping sickness and nagana in livestock. In the last decades, it has become an established eukaryotic model organism in the field of biology, as well as in the interdisciplinary field of biophysics. For instance, the dense variant surface glycoprotein (VSG) coat offers the possibility to study the dynamics of GPI-anchored proteins in the plasma membrane of living cells. The fluidity of the VSG coat is not only an interesting object of study for its own sake, but is critically important for the survival of the parasite in the mammalian host. In order to maintain the integrity of the coat, the entire VSG coat is recycled within a few minutes. This is surprisingly fast for a purely diffusive process with the flagellar pocket (FP) as the sole site for endo- and exocytosis. Previous studies characterising VSG dynamics using FRAP reported diffusion coefficients that were not sufficient to to enable fast turnover based on passive VSG randomisation on the trypanosome surface. In this thesis, live-cell single-molecule fluorescence microscopy (SMFM) was employed to elucidate whether VSG diffusion coefficients were priorly underestimated or whether directed forces could be involved to bias VSGs towards the entrance of the FP. Embedding the highly motile trypanosomes in thermo-stable hydrogels facilitated the investigation of VSG dynamics on living trypanosomes at the mammalian host's temperature of 37°C. To allow for a spatial correlation of the VSG dynamics to the FP entrance, a cell line was employed harbouring a fluorescently labelled structure as a reference. Sequential two-colour SMFM was then established to allow for recording and registration of the dynamic and static single-molecule information. In order to characterise VSG dynamics, an algorithm to obtain reliable information from short trajectories was adapted (shortTrAn). It allowed for the quantification of the local dynamics in two distinct scenarios: diffusion and directed motion. The adaptation of the algorithm to the VSG data sets required the introduction of an additional projection filter. The algorithm was further extended to take into account the localisation errors inherent to single-particle tracking. The results of the quantification of diffusion and directed motion were presented in maps of the trypanosome surface, including an outline generated from a super-resolved static structure as a reference. Information on diffusion was displayed in one map, an ellipse plot. The colour code represented the local diffusion coefficient, while the shape of the ellipses provided an indication of the diffusion behaviour (aniso- or isotropic diffusion). The eccentricity of the ellipses was used to quantify deviations from isotropic diffusion. Information on directed motion was shown in three maps: A velocity map, representing the amplitude of the local velocities in a colour code. A quiver plot, illustrating the orientation of directed motion, and a third map which indicated the relative standard error of the local velocities colour-coded. Finally, a guideline based on random walk simulations was used to identify which of the two motion scenarios dominated locally. Application of the guideline to the VSG dynamics analysed by shortTrAn yielded supermaps that showed the locally dominant motion mode colour-coded. I found that VSG dynamics are dominated by diffusion, but several times faster than previously determined. The diffusion behaviour was additionally characterised by spatial heterogeneity. Moreover, isolated regions exhibiting the characteristics of round and elongated traps were observed on the cell surface. Additionally, VSG dynamics were studied with respect to the entrance of the FP. VSG dynamics in this region displayed similar characteristics compared to the remainder of the cell surface and forces biasing VSGs into the FP were not found. Furthermore, I investigated a potential interference of the attachment of the cytoskeleton to the plasma membrane with the dynamics of VSGs which are anchored to the outer leaflet of the membrane. Preliminary experiments were conducted on osmotically swollen trypanosomes and trypanosomes depleted for a microtubule-associated protein anchoring the subpellicular microtubule cytoskeleton to the plasma membrane. The measurements revealed a trend that detachment of the cytoskeleton could be associated with a reduction in the VSG diffusion coefficient and a loss of elongated traps. The latter could be an indication that these isolated regions were caused by underlying structures associated with the cytoskeleton. The measurements on cells with an intact cytoskeleton were complemented by random walk simulations of VSG dynamics with the newly determined diffusion coefficient on long time scales not accessible in experiments. Simulations showed that passive VSG randomisation is fast enough to allow for a turnover of the full VSG coat within a few minutes. According to an estimate based on the known rate of endocytosis and the newly determined VSG diffusion coefficient, the majority of exocytosed VSGs could escape from the FP to the cell surface without being immediately re-endocytosed. N2 - Der einzellige, begeißelte Parasit Trypanosoma brucei ist der Erreger der humanen Afrikanischen Schlafkrankheit und Nagana bei Nutztieren. In den vergangenen Jahrzehnten hat er sich sowohl in der Biologie als auch im interdisziplinären Bereich der Biophysik als eukaryotischer Modellorganismus etabliert. So bietet der dichte variant surface glycoprotein (VSG) Mantel beispielsweise die Möglichkeit, die Dynamik von GPI-verankerten Proteinen in der Plasmamembran von lebenden Zellen zu untersuchen. Die Fluidität des VSG-Mantels ist nicht nur um ihrer selbst Willen ein interessantes Studienobjekt, sondern auch von entscheidender Bedeutung für das Überleben des Parasiten im Säugetierwirt. Damit die Integrität des Mantels erhalten bleibt, wird der gesamte VSG Mantel kontinuierlich innerhalb weniger Minuten ausgetauscht. Dies ist erstaunlich schnell für einen rein diffusiven Prozess, bei welchem die Geißeltasche (GT) der einzige Ort für Endo- und Exozytose ist. Bisherige Studien zur Charakterisierung der VSG Dynamik mit FRAP ermittelten Diffusionskoeffizienten, welche nicht ausreichten, um einen schnellen Austausch durch eine passive Randomisierung der VSG auf der Trypanosomenoberfläche zu ermöglichen. In dieser Arbeit wurde die Einzelmolekül-Fluoreszenzmikroskopie (EMFM) an lebenden Zellen eingesetzt, um herauszufinden, ob die VSG Diffusionskoeffizienten zuvor unterschätzt wurden oder ob gerichtete Kräfte beteiligt sein könnten, um VSGs zum Eingang der GT zu leiten. Die Einbettung der hochmotilen Trypanosomen in thermostabilen Hydrogelen erlaubte die Analyse der VSG Dynamik auf lebenden Trypanosomen bei einer Temperatur des Säugetierwirts von 37°C. Um eine räumliche Korrelation der VSG Dynamik mit dem Eingang zur GT zu ermöglichen, wurde eine Zelllinie verwendet, die eine fluoreszenzmarkierte Struktur als Referenz besaß. Anschließend wurde die sequenzielle EMFM in zwei Farben etabliert, um sowohl die Aufzeichnung als auch die Registrierung der dynamischen und statischen Einzelmolekülinformationen zu gewährleisten. Um die VSG Dynamik zu charakterisieren, wurde ein Algorithmus zur Gewinnung von zuverlässigen Informationen aus kurzen Trajektorien adaptiert (shortTrAn). Dieser ließ die Quantifizierung der lokalen Dynamik anhand zweier unterschiedlicher Szenarien zu: Diffusion und gerichtete Bewegung. Die Anpassung des Algorithmus an die VSG Datensätze erforderte die Einführung eines zusätzlichen Projektionsfilters. Darüber hinaus wurde der Algorithmus erweitert, um die Lokalisierungsfehler zu berücksichtigen, die bei der Verfolgung von Einzelpartikeln unvermeidbar auftreten. Anschließend wurden die Ergebnisse der Quantifizierung von Diffusion und gerichteter Bewegung in Karten präsentiert, die die Trypanosomenoberfläche abbildeten, einschließlich eines Umrisses, der als Referenz aus einer hochaufgelösten statischen Struktur generiert wurde. Die Informationen zur Diffusion wurden in einer Karte, einem Ellipsenplot, dargestellt. Dabei repräsentierte eine Farbkodierung die lokalen Diffusionskoeffizienten, während die Form der Ellipsen einen Hinweis auf das Diffusionsverhalten (aniso- oder isotrope Diffusion) gab. Die Exzentrizität der Ellipsen wurde hierbei genutzt, um die Abweichung von isotroper Diffusion zu quantifizieren. Die Informationen zur gerichteten Bewegung wurden in drei Karten wiedergegeben: Eine Karte für die Geschwindigkeit zeigte die Amplitude der lokalen Geschwindigkeiten farbkodiert. Ein Köcherplot veranschaulichte die Richtung der Geschwindigkeit und eine dritte Karte zeigte den relativen Standardfehler der lokalen Geschwindigkeiten farblich kodiert an. Abschließend wurde ein auf Random-Walk-Simulationen basierender Leitfaden herangezogen, um zu entscheiden, welches der beiden Szenarien lokal dominierte. Die Anwendung des Leitfadens auf die mit shortTrAn analysierte VSG Dynamik ergab Übersichtskarten, in denen der lokal dominierende Bewegungsmodus farblich kodiert war. Ich konnte zeigen, dass die VSG Dynamik von der Diffusion dominiert wird. Jedoch war diese um ein Vielfaches schneller als bisher angenommen. Das Diffusionsverhalten war zudem durch eine räumliche Heterogenität charakterisiert. Des Weiteren wurden auf der Zelloberfläche isolierte Regionen beobachtet, die die Eigenschaften von runden und länglichen Fallen aufwiesen. Zusätzlich wurde die VSG Dynamik in Bezug auf den Eingang der GT untersucht. Die VSG Dynamik in dieser Region wies ähnliche Kennwerte auf wie die restliche Zelloberfläche, und es konnten keine Kräfte festgestellt werden, welche die VSGs in die GT dirigieren. Des Weiteren habe ich den potenziellen Einfluss der Verankerung des Zytoskeletts an der Plasmamembran auf die Dynamik der VSGs untersucht, die in der äußeren Membranschicht verankert sind. Hierzu wurden vorläufige Experimente auf osmotisch geschwollenen Trypanosomen und Trypanosomen durchgeführt, denen ein Mikrotubuli assoziiertes Protein fehlte, welches das subpellikuläre Mikrotubuli-Zytoskelett an der Plasmamembran verankert. Bei den Messungen wurde ein Trend festgestellt, wonach die Ablösung des Zytoskeletts mit einer Verringerung des VSG Diffusionskoeffizienten und dem Verlust der länglichen Fallen korrelieren könnte. Letzteres könnte ein Hinweis darauf sein, dass diese isolierten Regionen durch darunter liegende, mit dem Zytoskelett verbundene Strukturen verursacht wurden. Die Messungen auf Zellen mit intaktem Zytoskelett wurden durch Random-Walk-Simulationen von VSG Trajektorien mit dem neu ermittelten Diffusionskoeffizienten auf langen, experimentell nicht zugänglichen Zeitskalen ergänzt. Die Simulationen zeigten, dass die passive Randomisierung der VSGs schnell genug ist, um einen Austausch des gesamten VSG Mantels innerhalb weniger Minuten zu ermöglichen. Einer Schätzung zufolge, die auf der bekannten Endozytoserate und dem neu ermittelten VSG Diffusionskoeffizienten basierte, könnte der Großteil der exozytierten VSGs aus der GT zur Zelloberfläche gelangen, ohne unmittelbar wieder endozytiert zu werden. KW - Trypanosoma brucei KW - Einzelmolekülmikroskopie KW - Membranproteine KW - Diffusionskoeffizient KW - Single-molecule fluorescence microscopy KW - Single-molecule tracking KW - Variant surface glycoprotein KW - GPI-anchored protein KW - Diffusion coefficient KW - Zellskelett KW - Zytoskelett Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-275699 ER - TY - JOUR A1 - Meiser, Elisabeth A1 - Mohammadi, Reza A1 - Vogel, Nicolas A1 - Holcman, David A1 - Fenz, Susanne F. T1 - Experiments in micro-patterned model membranes support the narrow escape theory JF - Communications Physics N2 - The narrow escape theory (NET) predicts the escape time distribution of Brownian particles confined to a domain with reflecting borders except for one small window. Applications include molecular activation events in cell biology and biophysics. Specifically, the mean first passage time τ can be analytically calculated from the size of the domain, the escape window, and the diffusion coefficient of the particles. In this study, we systematically tested the NET in a disc by variation of the escape opening. Our model system consisted of micro-patterned lipid bilayers. For the measurement of τ, we imaged diffusing fluorescently-labeled lipids using single-molecule fluorescence microscopy. We overcame the lifetime limitation of fluorescent probes by re-scaling the measured time with the fraction of escaped particles. Experiments were complemented by matching stochastic numerical simulations. To conclude, we confirmed the NET prediction in vitro and in silico for the disc geometry in the limit of small escape openings, and we provide a straightforward solution to determine τ from incomplete experimental traces. KW - membrane biophysics KW - single-molecule biophysics Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-358121 VL - 6 ER - TY - JOUR A1 - Munawar, Umair A1 - Zhou, Xiang A1 - Prommersberger, Sabrina A1 - Nerreter, Silvia A1 - Vogt, Cornelia A1 - Steinhardt, Maximilian J. A1 - Truger, Marietta A1 - Mersi, Julia A1 - Teufel, Eva A1 - Han, Seungbin A1 - Haertle, Larissa A1 - Banholzer, Nicole A1 - Eiring, Patrick A1 - Danhof, Sophia A1 - Navarro-Aguadero, Miguel Angel A1 - Fernandez-Martin, Adrian A1 - Ortiz-Ruiz, Alejandra A1 - Barrio, Santiago A1 - Gallardo, Miguel A1 - Valeri, Antonio A1 - Castellano, Eva A1 - Raab, Peter A1 - Rudert, Maximilian A1 - Haferlach, Claudia A1 - Sauer, Markus A1 - Hudecek, Michael A1 - Martinez-Lopez, J. A1 - Waldschmidt, Johannes A1 - Einsele, Hermann A1 - Rasche, Leo A1 - Kortüm, K. Martin T1 - Impaired FADD/BID signaling mediates cross-resistance to immunotherapy in Multiple Myeloma JF - Communications Biology N2 - The treatment landscape in multiple myeloma (MM) is shifting from genotoxic drugs to immunotherapies. Monoclonal antibodies, immunoconjugates, T-cell engaging antibodies and CART cells have been incorporated into routine treatment algorithms, resulting in improved response rates. Nevertheless, patients continue to relapse and the underlying mechanisms of resistance remain poorly understood. While Impaired death receptor signaling has been reported to mediate resistance to CART in acute lymphoblastic leukemia, this mechanism yet remains to be elucidated in context of novel immunotherapies for MM. Here, we describe impaired death receptor signaling as a novel mechanism of resistance to T-cell mediated immunotherapies in MM. This resistance seems exclusive to novel immunotherapies while sensitivity to conventional anti-tumor therapies being preserved in vitro. As a proof of concept, we present a confirmatory clinical case indicating that the FADD/BID axis is required for meaningful responses to novel immunotherapies thus we report impaired death receptor signaling as a novel resistance mechanism to T-cell mediated immunotherapy in MM. KW - immunotherapy KW - translational research Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-357609 VL - 6 ER - TY - JOUR A1 - Albrecht, Jörg A1 - Classen, Alice A1 - Vollstädt, Maximilian G.R. A1 - Mayr, Antonia A1 - Mollel, Neduvoto P. A1 - Schellenberger Costa, David A1 - Dulle, Hamadi I. A1 - Fischer, Markus A1 - Hemp, Andreas A1 - Howell, Kim M. A1 - Kleyer, Michael A1 - Nauss, Thomas A1 - Peters, Marcell K. A1 - Tschapka, Marco A1 - Steffan-Dewenter, Ingolf A1 - Böhning-Gaese, Katrin A1 - Schleuning, Matthias T1 - Plant and animal functional diversity drive mutualistic network assembly across an elevational gradient JF - Nature Communications N2 - Species' functional traits set the blueprint for pair-wise interactions in ecological networks. Yet, it is unknown to what extent the functional diversity of plant and animal communities controls network assembly along environmental gradients in real-world ecosystems. Here we address this question with a unique dataset of mutualistic bird-fruit, bird-flower and insect-flower interaction networks and associated functional traits of 200 plant and 282 animal species sampled along broad climate and land-use gradients on Mt. Kilimanjaro. We show that plant functional diversity is mainly limited by precipitation, while animal functional diversity is primarily limited by temperature. Furthermore, shifts in plant and animal functional diversity along the elevational gradient control the niche breadth and partitioning of the respective other trophic level. These findings reveal that climatic constraints on the functional diversity of either plants or animals determine the relative importance of bottom-up and top-down control in plant-animal interaction networks. KW - Traits-Environment Relationships KW - Species Traits KW - Ecological Networks KW - 4TH-Corner Problem KW - Multiple Traits KW - Bottom-up KW - Biodiversity KW - Community ecology KW - Ecological networks KW - Ecology KW - Ecosystem ecology Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-221056 VL - 9 ER - TY - JOUR A1 - Annunziata, Ida A1 - van de Vlekkert, Diantha A1 - Wolf, Elmar A1 - Finkelstein, David A1 - Neale, Geoffrey A1 - Machado, Eda A1 - Mosca, Rosario A1 - Campos, Yvan A1 - Tillman, Heather A1 - Roussel, Martine F. A1 - Weesner, Jason Andrew A1 - Fremuth, Leigh Ellen A1 - Qiu, Xiaohui A1 - Han, Min-Joon A1 - Grosveld, Gerard C. A1 - d'Azzo, Alessandra T1 - MYC competes with MiT/TFE in regulating lysosomal biogenesis and autophagy through an epigenetic rheostat JF - Nature Communications N2 - Coordinated regulation of the lysosomal and autophagic systems ensures basal catabolism and normal cell physiology, and failure of either system causes disease. Here we describe an epigenetic rheostat orchestrated by c-MYC and histone deacetylases that inhibits lysosomal and autophagic biogenesis by concomitantly repressing the expression of the transcription factors MiT/TFE and FOXH1, and that of lysosomal and autophagy genes. Inhibition of histone deacetylases abates c-MYC binding to the promoters of lysosomal and autophagy genes, granting promoter occupancy to the MiT/TFE members, TFEB and TFE3, and/or the autophagy regulator FOXH1. In pluripotent stem cells and cancer, suppression of lysosomal and autophagic function is directly downstream of c-MYC overexpression and may represent a hallmark of malignant transformation. We propose that, by determining the fate of these catabolic systems, this hierarchical switch regulates the adaptive response of cells to pathological and physiological cues that could be exploited therapeutically. KW - autophagy KW - cancer KW - cancer metabolism KW - cell biology KW - mechanisms of disease Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-221189 VL - 10 ER - TY - JOUR A1 - Carradec, Quentin A1 - Pelletier, Eric A1 - Da Silva, Corinne A1 - Alberti, Adriana A1 - Seeleuthner, Yoann A1 - Blanc-Mathieu, Romain A1 - Lima-Mendez, Gipsi A1 - Rocha, Fabio A1 - Tirichine, Leila A1 - Labadie, Karine A1 - Kirilovsky, Amos A1 - Bertrand, Alexis A1 - Engelen, Stefan A1 - Madoui, Mohammed-Amin A1 - Méheust, Raphaël A1 - Poulain, Julie A1 - Romac, Sarah A1 - Richter, Daniel J. A1 - Yoshikawa, Genki A1 - Dimier, Céline A1 - Kandels-Lewis, Stefanie A1 - Picheral, Marc A1 - Searson, Sarah A1 - Jaillon, Olivier A1 - Aury, Jean-Marc A1 - Karsenti, Eric A1 - Sullivan, Matthew B. A1 - Sunagawa, Shinichi A1 - Bork, Peer A1 - Not, Fabrice A1 - Hingamp, Pascal A1 - Raes, Jeroen A1 - Guidi, Lionel A1 - Ogata, Hiroyuki A1 - de Vargas, Colomban A1 - Iudicone, Daniele A1 - Bowler, Chris A1 - Wincker, Patrick T1 - A global ocean atlas of eukaryotic gene JF - Nature Communications N2 - While our knowledge about the roles of microbes and viruses in the ocean has increased tremendously due to recent advances in genomics and metagenomics, research on marine microbial eukaryotes and zooplankton has benefited much less from these new technologies because of their larger genomes, their enormous diversity, and largely unexplored physiologies. Here, we use a metatranscriptomics approach to capture expressed genes in open ocean Tara Oceans stations across four organismal size fractions. The individual sequence reads cluster into 116 million unigenes representing the largest reference collection of eukaryotic transcripts from any single biome. The catalog is used to unveil functions expressed by eukaryotic marine plankton, and to assess their functional biogeography. Almost half of the sequences have no similarity with known proteins, and a great number belong to new gene families with a restricted distribution in the ocean. Overall, the resource provides the foundations for exploring the roles of marine eukaryotes in ocean ecology and biogeochemistry. KW - genomics KW - marine biology KW - microbial ecology KW - water microbiology Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-222250 VL - 9 ER - TY - JOUR A1 - Brunk, Michael A1 - Sputh, Sebastian A1 - Doose, Sören A1 - van de Linde, Sebastian A1 - Terpitz, Ulrich T1 - HyphaTracker: An ImageJ toolbox for time-resolved analysis of spore germination in filamentous fungi JF - Scientific Reports N2 - The dynamics of early fungal development and its interference with physiological signals and environmental factors is yet poorly understood. Especially computational analysis tools for the evaluation of the process of early spore germination and germ tube formation are still lacking. For the time-resolved analysis of conidia germination of the filamentous ascomycete Fusarium fujikuroi we developed a straightforward toolbox implemented in ImageJ. It allows for processing of microscopic acquisitions (movies) of conidial germination starting with drift correction and data reduction prior to germling analysis. From the image time series germling related region of interests (ROIs) are extracted, which are analysed for their area, circularity, and timing. ROIs originating from germlings crossing other hyphae or the image boundaries are omitted during analysis. Each conidium/hypha is identified and related to its origin, thus allowing subsequent categorization. The efficiency of HyphaTracker was proofed and the accuracy was tested on simulated germlings at different signal-to-noise ratios. Bright-field microscopic images of conidial germination of rhodopsin-deficient F. fujikuroi mutants and their respective control strains were analysed with HyphaTracker. Consistent with our observation in earlier studies the CarO deficient mutant germinated earlier and grew faster than other, CarO expressing strains. KW - bioinformatics KW - cell growth KW - fungal biology KW - microscopy Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-221691 VL - 8 ER - TY - INPR A1 - Dandekar, Thomas T1 - How do qubits interact? Implications for fundamental physics N2 - Proteins fold in water and achieve a clear structure despite a huge parameter space. Inside a (protein) crystal you have everywhere the same symmetries as there is everywhere the same unit cell. We apply this to qubit interactions to do fundamental physics: We modify cosmological inflation: we replace the big bang by a condensation event in an eternal all-encompassing ocean of free qubits. Rare interactions of qubits in the ocean provide a nucleus or seed for a new universe (domain), as the qubits become decoherent and freeze-out into defined bit ensembles. Next, we replace inflation by a crystallization event triggered by the nucleus of interacting qubits to which rapidly more and more qubits attach (like in everyday crystal growth). The crystal unit cell guarantees same symmetries (and laws of nature) everywhere inside the crystal, no inflation scenario is needed. Interacting qubits solidify, quantum entropy decreases in the crystal, but increases outside in the ocean. The interacting qubits form a rapidly growing domain where the n**m states become separated ensemble states, rising long-range forces stop ultimately further growth. After this very early modified steps, standard cosmology with the hot fireball model takes over. Our theory agrees well with lack of inflation traces in cosmic background measurements. Applying the Hurwitz theorem to qubits we prove that initiation of qubit interactions can only be 1,2,4 or 8-dimensional (agrees with E8 symmetry of our universe). Repulsive forces at ultrashort distances result from quantization, long-range forces limit crystal growth. The phase space of the crystal agrees with the standard model of the basic four forces for n quanta. It includes all possible ensemble combinations of their quantum states m, a total of n**m states. We describe a six-bit-ensemble toy model of qubit interaction and the repulsive forces of qubits for ultra-short distances. Neighbor states reach according to transition possibilities (S-matrix) with emergent time from entropic ensemble gradients. However, in our four dimensions there is only one bit overlap to neighbor states left (almost solid, only below Planck´s quantum is liquidity left). The E8 symmetry of heterotic string theory has six curled-up, small dimensions. These keep the qubit crystal together and never expand. We give energy estimates for free qubits vs bound qubits, misplacements in the qubit crystal and entropy increase during qubit crystal formation. Implications are fundamental answers, e.g. why there is fine-tuning for life-friendliness, why there is string theory with rolled-up dimension and so many free parameters. We explain by cosmological crystallization instead of inflation the early creation of large-scale structure of voids and filaments, supercluster formation, galaxy formation, and the dominance of matter: the unit cell of our crystal universe has a matter handedness avoiding anti-matter. Importantly, crystals come and go in the qubit ocean. This selects for the ability to lay seeds for new crystals, for self-organization and life-friendliness. Vacuum energy gets appropriate low inside the crystal by its qubit binding energy, outside it is 10**20 higher. Scalar fields for color interaction/confinement and gravity could be derived from the qubit-interaction field. KW - protein folding KW - qubit interaction KW - early cosmology KW - qubit KW - modified inflation KW - crystallization KW - decoherence Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-357435 ER - TY - JOUR A1 - Schwarz, Jessica Denise A1 - Lukassen, Sören A1 - Bhandare, Pranjali A1 - Eing, Lorenz A1 - Snaebjörnsson, Marteinn Thor A1 - García, Yiliam Cruz A1 - Kisker, Jan Philipp A1 - Schulze, Almut A1 - Wolf, Elmar T1 - The glycolytic enzyme ALDOA and the exon junction complex protein RBM8A are regulators of ribosomal biogenesis JF - Frontiers in Cell and Developmental Biology N2 - Cellular growth is a fundamental process of life and must be precisely controlled in multicellular organisms. Growth is crucially controlled by the number of functional ribosomes available in cells. The production of new ribosomes depends critically on the activity of RNA polymerase (RNAP) II in addition to the activity of RNAP I and III, which produce ribosomal RNAs. Indeed, the expression of both, ribosomal proteins and proteins required for ribosome assembly (ribosomal biogenesis factors), is considered rate-limiting for ribosome synthesis. Here, we used genetic screening to identify novel transcriptional regulators of cell growth genes by fusing promoters from a ribosomal protein gene (Rpl18) and from a ribosomal biogenesis factor (Fbl) with fluorescent protein genes (RFP, GFP) as reporters. Subsequently, both reporters were stably integrated into immortalized mouse fibroblasts, which were then transduced with a genome-wide sgRNA-CRISPR knockout library. Subsequently, cells with altered reporter activity were isolated by FACS and the causative sgRNAs were identified. Interestingly, we identified two novel regulators of growth genes. Firstly, the exon junction complex protein RBM8A controls transcript levels of the intronless reporters used here. By acute depletion of RBM8A protein using the auxin degron system combined with the genome-wide analysis of nascent transcription, we showed that RBM8A is an important global regulator of ribosomal protein transcripts. Secondly, we unexpectedly observed that the glycolytic enzyme aldolase A (ALDOA) regulates the expression of ribosomal biogenesis factors. Consistent with published observations that a fraction of this protein is located in the nucleus, this may be a mechanism linking transcription of growth genes to metabolic processes and possibly to metabolite availability. KW - ribosome biogenesis KW - Ribosomal protein gene KW - genetic screen KW - genome-wide screen KW - RBM8A KW - Y14 KW - AldoA KW - aldolase A Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-290875 SN - 2296-634X VL - 10 ER - TY - THES A1 - Gabel, Martin Sebastian T1 - Behavioural resistance to \(Varroa\) \(destructor\) in the Western honeybee \(Apis\) \(mellifera\) - Mechanisms leading to decreased mite reproduction T1 - Resistenzverhalten der Westlichen Honigbiene \(Apis\) \(mellifera\) gegen \(Varroa\) \(destructor\) - Zu verringerter Milbenreproduktion führende Mechanismen N2 - The Western Honeybee (Apis mellifera) is among the most versatile species in the world. Its adaptability is rooted in thousands of the differently specialized individuals acting jointly together. Thus, bees that are able to handle a certain task or condition well can back up other individuals less capable to do so on the colony level. Vice versa, the latter individuals might perform better in other situations. This evolutionary recipe for success ensures the survival of colonies despite challenging habitat conditions. In this context, the ectoparasitic mite Varroa destructor reflects the most pronounced biotic challenge to honeybees worldwide. Without proper treatment, infested colonies rapidly dwindle and ultimately die. Nevertheless, resistance behaviours against this parasite have evolved in some populations through natural selection, enabling colonies to survive untreated. In this, different behaviours appear to be adapted to the respective habitat conditions and may complement each other. Yet, the why and how of this behavioural response to the mite remains largely unknown. My thesis focuses on the biological background of Varroa-resistance traits in honeybees and presents important findings for the comprehension of this complex host-parasite interaction. Based on this, I draw implications for both, applied bee breeding and scientific investigations in the field of Varroa-resistance. Specifically, I focus on two traits commonly found in resistant and, to a lower degree, also mite-susceptible colonies: decreased mite reproduction and the uncapping and subsequent recapping of sealed brood cells. Examining failures in the reproductive success of mites as a primary mechanism of Varroa-resistance, I was able to link them to specific bee behaviours and external factors. Since mite reproduction and the brood rearing of bees are inevitably connected, I first investigated the effects of brood interruption on the reproductive success of mites. Brood interruption decreased the reproductive success of mites both immediately and in the long term. By examining the causes of reproductive failure, I could show that this was mainly due to an increased share of infertile mites. Furthermore, I proved that interruption in brood rearing significantly increased the expression of recapping behaviour. These findings consequently showed a dynamic modulation of mite reproduction and recapping, as well as a direct effect of brood interruption on both traits. To further elucidate the plasticity in the expression of both traits, I studied mite reproduction, recapping behaviour and infestation levels over the course of three years. The resulting extensive dataset unveiled a significant seasonal variation in mite reproduction and recapping. In addition, I show that recapping decreases the reproductive success of mites by increasing delayed developing female offspring and cells lacking male offspring. By establishing a novel picture-based brood investigation method, I could furthermore show that both the removal of brood cells and recapping activity specifically target brood ages in which mite offspring would be expected. Recapping, however, did not cause infertility of mites. Considering the findings of my first study, this points towards complementary mechanisms. This underlines the importance of increased recapping behaviour and decreased mite reproduction as resistance traits, while at the same time emphasising the challenges of reliable data acquisition. To pave the way for a practical application of these findings in breeding, we then investigated the heritability (i.e., the share of genotypic variation on the observed phenotypic variation) of the accounted traits. By elaborating comparable test protocols and compiling data from over 4,000 colonies, we could, for the first time, demonstrate that recapping of infested cells and decreased reproductive success of mites are heritable (and thus selectable) traits in managed honeybee populations. My thesis proves the importance of recapping and decreased mite reproduction as resistance traits and therefore valuable goals for breeding efforts. In this regard, I shed light on the underlying mechanisms of both traits, and present clear evidence for their interaction and heritability. N2 - Die Westliche Honigbiene (Apis mellifera) zählt zu den anpassungsfähigsten Arten der Welt. Diese Anpassungsfähigkeit liegt in der Zusammenarbeit tausender unterschiedlich spezialisierter Individuen begründet. Auf Volksebene können Bienen, die mit einer bestimmten Aufgabe oder Situation gut umgehen können, andere Individuen, die dies weniger gut können, absichern. Andererseits können Letztere womöglich mit anderen Situationen besser umgehen. Dieses evolutionäre Erfolgskonzept sichert das Überleben der Völker selbst unter herausfordernden Habitatbedingungen. Die ektoparasitäre Milbe Varroa destructor stellt in diesem Zusammenhang weltweit die größte biotische Herausforderung dar. Ohne entsprechende Behandlung siechen die Völker rasch dahin und sterben schlussendlich. In einigen Populationen haben sich jedoch Resistenzmechanismen durch natürliche Selektion herausgebildet, die es den Völkern ermöglichen, ohne Behandlung zu überleben. Die verschiedenen Verhaltensweisen scheinen dabei an die jeweiligen Habitatbedingungen angepasst zu sein und sich gegenseitig zu ergänzen. Was diese Reaktion auf die Milben auslöst und wie sie funktioniert ist allerdings noch weitestgehend unbekannt. Meine Dissertation fokussiert den biologischen Hintergrund von Varroa-resistenzmechanismen bei Honigbienen und stellt dabei wichtige Erkenntnisse zum Verständnis dieser komplexen Parasit-Wirt-Beziehung vor. Darauf aufbauend leite ich Implikationen für die angewandte Bienenzucht und wissenschaftliche Untersuchungen auf dem Gebiet der Varroa-resistenz ab. Hierbei konzentriere ich mich insbesondere auf zwei Merkmale, die häufig in resistenten Völkern zu finden sind: die reduzierte Milbenreproduktion und das Entdeckeln und Wiederverdeckeln bereits verschlossener Brutzellen. Beide Merkmale treten in geringerem Umfang auch in milbenanfälligen Populationen auf und sind daher von besonderem Interesse für jedwede Zuchtbemühung mit dem Ziel der Varroa-resistenz. Durch die Untersuchung von Fehlern in der Reproduktion der Milben, konnte ich diesen Hauptmechanismus der Varroa-resistenz mit Verhaltensweisen der Bienen, sowie äußeren Faktoren in Verbindung setzen. Da die Milbenvermehrung untrennbar mit der Brutaufzucht der Bienen verbunden ist, habe ich zunächst die Einflüsse von Brutunterbrechungen auf den Vermehrungserfolg der Milben untersucht. Diese Untersuchung zeigte auf, dass Brutunterbrechungen den Vermehrungserfolg der Milben sowohl kurzfristig, als auch langfristig herabsetzen. Durch die Untersuchung der jeweils zugrundeliegenden Ursachen gescheiterter Milbenreproduktion konnte ich zeigen, dass dies vor Allem auf einen gesteigerten Anteil infertiler Milben zurückzuführen war. Des Weiteren konnte ich beweisen, dass die Unterbrechung der Brutaufzucht die Ausprägung des Wiederverdeckelns signifikant verstärkte. Folglich zeigten diese Ergebnisse eine dynamische Anpassung der Milbenreproduktion und des Wiederverdeckelns, sowie einen direkten Einfluss der Brutunterbrechungen auf beide Eigenschaften. Um die Plastizität der Ausprägung beider Merkmale genauer zu erklären, untersuchte ich daraufhin drei Jahre lang die Milbenvermehrung, das Verhalten des Wiederverdeckelns, sowie die Befallsentwicklung. Daraus resultierte ein umfangreicher Datensatz, der eine signifikante saisonale Variation der Milbenvermehrung und des Wiederverdeckelns belegte. Ich konnte außerdem eindeutig beweisen, dass das Wiederverdeckeln den Reproduktionserfolg der Milben herabsetzt, indem es die Anteile von verzögert heranwachsenden weiblichen Nachkommen und fehlenden Männchen steigert. Durch Anwendung einer neuartigen Bild-basierten Methode der Brutuntersuchung, konnte ich darüber hinaus zeigen, dass sich sowohl das Ausräumen, als auch das Wiederverdeckeln von Brutzellen auf Brutalter konzentriert, in denen Milbennachwuchs erwartet werden würde. Das Wiederverdeckeln trug jedoch nicht zur Infertilität der Milben bei, was zusammen mit den Ergebnissen meiner ersten Untersuchung auf komplementäre Mechanismen hinweist. Dies unterstreicht die Bedeutung des Wiederverdeckelns und der verminderten Milbenreproduktion als Resistenzmechanismen, hebt aber gleichzeitig auch die Herausforderungen einer verlässlichen Datenerhebung hervor. Um den Weg für die praktische Anwendung dieser Erkenntnisse in der Zuchtarbeit zu ebnen, untersuchten wir daraufhin die Erblichkeit (den Anteil der genotypischen Variation an der beobachteten phänotypischen Variation) der betrachteten Merkmale. Durch das Erarbeiten vergleichbarer Prüfprotokolle und Zusammenführen von Daten aus über 4000 Völkern, konnten wir erstmalig zeigen, dass das Wiederverdeckeln befallener Zellen und der verminderte Vermehrungserfolg der Milben erbliche und damit selektierbare Merkmale in bewirtschafteten Honigbienenpopulationen sind. Meine Dissertation beweist die Relevanz des Wiederverdeckelns und der verminderten Milbenreproduktion als Resistenzmerkmale und damit lohnende Ziele für Zuchtbemühungen. In diesem Zusammenhang beleuchtete ich verschiedene Mechanismen, die der Ausprägung beider Merkmale zugrunde liegen und lieferte eindeutige Beweise für deren Interaktion und Erblichkeit. KW - Varroa destructor KW - Resistenz KW - Biene KW - mite non-reproduction KW - recapping KW - Varroa resistance KW - biotechnical Varroa control KW - heritability KW - selection KW - honeybees KW - Varroa mites KW - Züchtung KW - Apis mellifera KW - Breeding Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-360536 ER - TY - THES A1 - Gaballa, Abdallah Hatem Hassan Hosny Ahmed T1 - PAF1c drives MYC-mediated immune evasion in pancreatic ductal adenocarcinoma T1 - PAF1c treibt die MYC-vermittelte Immunevasion im duktalen Adenokarzinom der Bauchspeicheldrüse an N2 - The expression of the MYC proto-oncogene is elevated in a large proportion of patients with pancreatic ductal adenocarcinoma (PDAC). Previous findings in PDAC have shown that this increased MYC expression mediates immune evasion and promotes S-phase progression. How these functions are mediated and whether a downstream factor of MYC mediates these functions has remained elusive. Recent studies identifying the MYC interactome revealed a complex network of interaction partners, highlighting the need to identify the oncogenic pathway of MYC in an unbiased manner. In this work, we have shown that MYC ensures genomic stability during S-phase and prevents transcription-replication conflicts. Depletion of MYC and inhibition of ATR kinase showed a synergistic effect to induce DNA damage. A targeted siRNA screen targeting downstream factors of MYC revealed that PAF1c is required for DNA repair and S-phase progression. Recruitment of PAF1c to RNAPII was shown to be MYC dependent. PAF1c was shown to be largely dispensable for cell proliferation and regulation of MYC target genes. Depletion of CTR9, a subunit of PAF1c, caused strong tumor regression in a pancreatic ductal adenocarcinoma model, with long-term survival in a subset of mice. This effect was not due to induction of DNA damage, but to restoration of tumor immune surveillance. Depletion of PAF1c resulted in the release of RNAPII with transcription elongation factors, including SPT6, from the bodies of long genes, promoting full-length transcription of short genes. This resulted in the downregulation of long DNA repair genes and the concomitant upregulation of short genes, including MHC class I genes. These data demonstrate that a balance between long and short gene transcription is essential for tumor progression and that interference with PAF1c levels shifts this balance toward a tumor-suppressive transcriptional program. It also directly links MYC-mediated S-phase progression to immune evasion. Unlike MYC, PAF1c has a stable, known folded structure; therefore, the development of a small molecule targeting PAF1c may disrupt the immune evasive function of MYC while sparing its physiological functions in cellular growth. N2 - Die Expression des MYC-Proto-Onkogens ist bei einem großen Teil der Patienten mit duktalem Adenokarzinom der Bauchspeicheldrüse (PDAC) erhöht. Bisherige Erkenntnisse in der Erforschung des ankreaskarzinoms zeigen, dass die erhöhte MYCExpression die Umgehung des Immunsystems bewirkt und die Progression der S-Phase fördert. Wie diese Funktionen vermittelt werden und ob ein nachgeschalteter Faktor von MYC für diese Funktion verantwortlich ist, blieb jedoch bisher ungeklärt. Jüngste Studien zur Identifizierung des MYC-Interaktoms haben ein sehr komplexes Netzwerk an Interaktionspartnern von MYC aufgedeckt, was die Notwendigkeit unterstreicht, die onkogenen Eigenschaften von MYC und seinen Interaktionspartnern unvoreingenommen und genau zu untersuchen. In dieser Arbeit konnte gezeigt werden, dass MYC die genomische Stabilität während der S-Phase herstellt und Konflikte zwischen Transkription und Replikation verhindert. Die Depletion von MYC und die Hemmung der ATR-Kinase zeigten bei der Induktion von DNA Schäden eine synergistische Wirkung. Ein siRNA-Screen, der Gene beinhaltete, die MYC nachgeschaltet sind, ergab, dass PAF1c für die DNA-Reparatur und die S-PhasenProgression erforderlich ist. Es zeigte sich außerdem, dass die Rekrutierung von PAF1c an RNAPII von MYC abhängig ist. Für die Zellproliferation und die Regulierung von MYCZielgenen ist PAF1c jedoch weitgehend entbehrlich. Es konnte gezeigt werden, dass die Depletion von CTR9, einer Untereinheit von PAF1c, in einem murinen Modell des duktalen Adenokarzinoms der Bauchspeicheldrüse zu einer starken Tumorregression mit langfristigem Überleben einiger Mäuse führte. Diese Wirkung war nicht auf die Induktion von DNA-Schäden zurückzuführen, sondern auf die Wiederherstellung der Immunüberwachung des Tumors. Die Deletion von PAF1c führte zu einer Umverteilung von RNAPII und Trankriptionselongationsfaktoren wie SPT6, von langen Genen hin zu kurzen Genen. Dadurch wurden lange Gene wie zum Beispiel DNA Reparaturgene nicht vollständig transkribiert, kurze Gene wie MHC-Klasse-I-Gene hingegen schon. Diese Daten zeigen, dass ein Gleichgewicht zwischen der Transkription langer und kurzer Gene für die Tumorprogression wichtig ist und dass eine Verminderung der PAF1c-Konzentration dieses Gleichgewicht in Richtung eines tumorsuppressiven Transkriptionsprogramms verschiebt. Außerdem besteht ein direkter Zusammenhang zwischen der MYCvermittelten S-Phasen-Progression und der Umgehung des Immunsystems. Im Gegensatz zu MYC verfügt PAF1c über eine stabile und gut bekannte gefaltete Struktur. Daher könnte die Entwicklung eines kleinen Moleküls, das PAF1c hemmt, die Funktion von MYC zur Umgehung des Immunsystems stören und gleichzeitig seine physiologischen Funktionen für das Zellwachstum nicht beeinträchtigen. KW - Myc KW - Transkription KW - PAF1c KW - Transcription elongation KW - Immune evasion KW - Immunevasion Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-360459 ER - TY - THES A1 - Amini, Emad T1 - How central and peripheral clocks and the neuroendocrine system interact to time eclosion behavior in \(Drosophila\) \(melanogaster\) T1 - Wie zentrale und periphere Uhren und das neuroendokrine System zusammenwirken, um das Schlupfverhalten von \(Drosophila\) \(melanogaster\) zeitlich festzulegen N2 - To grow larger, insects must shed their old rigid exoskeleton and replace it with a new one. This process is called molting and the motor behavior that sheds the old cuticle is called ecdysis. Holometabolic insects have pupal stages in between their larval and adult forms, during which they perform metamorphosis. The pupal stage ends with eclosion, i.e., the emergence of the adult from the pupal shell. Insects typically eclose at a specific time during the day, likely when abiotic conditions are at their optimum. A newly eclosed insect is fragile and needs time to harden its exoskeleton. Hence, eclosion is regulated by sophisticated developmental and circadian timing mechanisms. In Drosophila melanogaster, eclosion is limited to a daily time window in the morning, regarded as the “eclosion gate”. In a population of laboratory flies entrained by light/dark cycles, most of the flies eclose around lights on. This rhythmic eclosion pattern is controlled by the circadian clock and persists even under constant conditions. Developmental timing is under the control of complex hormonal signaling, including the steroid ecdysone, insulin-like peptides, and prothoracicotropic hormone (PTTH). The interactions of the central circadian clock in the brain and a peripheral clock in the prothoracic gland (PG) that produces ecdysone are important for the circadian timing of eclosion. These two clocks are connected by a bilateral pair of peptidergic PTTH neurons (PTTHn) that project to the PG. Before each molt, the ecdysone level rises and then falls shortly before ecdysis. The falling ecdysone level must fall below a certain threshold value for the eclosion gate to open. The activity of PTTHn is inhibited by short neuropeptide F (sNPF) from the small ventrolateral neurons (sLNvs) and inhibition is thought to lead to a decrease in ecdysone production. The general aim of this thesis is to further the understanding of how the circadian clock and neuroendocrinal pathways are coordinated to drive eclosion rhythmicity and to identify when these endocrinal signaling pathways are active. In Chapter I, a series of conditional PTTHn silencing-based behavioral assays, combined with neuronal activity imaging techniques such as non-invasive ARG-Luc show that PTTH signaling is active and required shortly before eclosion and may serve to phase-adjust the activity of the PG at the end of pupal development. Trans-synaptic anatomical stainings identified the sLNvs, dorsal neurons 1 (DN1), dorsal neurons 2 (DN2), and lateral posterior neurons (LPNs) clock neurons as directly upstream of the PTTHn. Eclosion motor behavior is initiated by Ecdysis triggering hormone (ETH) which activates a pair of ventromedial (Vm) neurons to release eclosion hormone (EH) which positively feeds back to the source of ETH, the endocrine Inka cells. In Chapter II trans-synaptic tracing showed that most clock neurons provide input to the Vm and non-canonical EH neurons. Hence, clock can potentially influence the ETH/EH feedback loop. The activity profile of the Inka cells and Vm neurons before eclosion is described. Vm and Inka cells are active around seven hours before eclosion. Interestingly, all EH neurons appear to be exclusively peptidergic. In Chapter III, using chemoconnectomics, PTTHns were found to express receptors for sNPF, allatostatin A (AstA), allatostatin C (AstC), and myosuppressin (Ms), while EH neurons expressed only Ms and AstA receptors. Eclosion assays of flies with impaired AstA, AstC, or Ms signaling do not show arrhythmicity under constant conditions. However, optogenetic activation of the AstA neurons strongly suppresses eclosion. Chapter IV focuses on peripheral ventral’ Tracheal dendrite (v’Td) and class IV dendritic arborization (C4da) neurons. The C4da neurons mediate larval light avoidance through endocrine PTTH signaling. The v’Td neurons mainly receive O2/CO2 input from the trachea and are upstream of Vm neurons but are not required for eclosion rhythmicity. Conditional ablation of the C4da neurons or torso (receptor of PTTH) knock-out in the C4da neurons impaired eclosion rhythmicity. Six to seven hours before eclosion, PTTHn, C4da, and Vm neurons are active based on ARG-Luc imaging. Thus, C4da neurons may indirectly connect the PTTHn to the Vm neurons. In summary, this thesis advances our knowledge of the temporal activity and role of PTTH signaling during pupal development and rhythmic eclosion. It further provides a comprehensive characterization of the synaptic and peptidergic inputs from clock neurons to PTTHn and EH neurons. AstA, AstC, and Ms are identified as potential modulators of eclosion circuits and suggest an indirect effect of PTTH signaling on EH signaling via the peripheral sensory C4da neurons. N2 - Um zu wachsen, müssen Insekten ihr altes, starres Exoskelett abwerfen und durch ein neues ersetzen. Dieser Vorgang wird als Häutung bezeichnet, und das motorische Verhalten, bei dem die alte Kutikula abgestoßen wird, heißt Ekdysis. Holometabole Insekten haben zwischen ihrer Larven- und Erwachsenenform ein Puppenstadium, in welchem sie eine Metamorphose durchlaufen. Das Puppenstadium endet mit dem Schlüpfen des erwachsenen Tieres aus der Puppenhülle. Die Insekten schlüpfen in der Regel zu einem bestimmten Zeitpunkt am Tag, wenn die abiotischen Bedingungen optimal sind, da das frisch geschlüpfte Insekt zerbrechlich ist und Zeit braucht, um sein Exoskelett auszuhärten. Daher wird der Schlupf durch ausgeklügelte Mechanismen der Entwicklung und der inneren Uhr gesteuert. Bei Drosophila melanogaster ist der Sclupf auf ein tägliches Zeitfenster am Morgen beschränkt, das als "Schlupffenster" bezeichnet wird. In einer Population von Laborfliegen, die durch Licht/Dunkel-Zyklen gesteuert wird, schlüpfen die meisten Fliegen in etwa um das Einschalten der Beleuchtung. Dieses rhythmische Schlupfmuster wird von der inneren Uhr gesteuert und bleibt auch unter konstanten Bedingungen bestehen. Das Timing der Entwicklung wird von komplexen hormonellen Signalen gesteuert, darunter das Steroid Ecdyson, insulinähnliche Peptide und das prothorakotrope Hormon (PTTH). Die Wechselwirkungen zwischen der zentralen zirkadianen Uhr im Gehirn und einer peripheren Uhr in der Prothorakaldrüse (PG), die Ecdyson produziert, sind wichtig für die zirkadiane Zeitsteuerung des Schlupfs. Diese beiden Uhren sind durch ein bilaterales Paar peptiderger PTTH-Neuronen (PTTHn) verbunden, die in die PG projizieren. Vor jeder Häutung steigt der Ecdysonspiegel an und fällt dann kurz vor danach wieder ab. Der fallende Ecdysonspiegel muss einen bestimmten Schwellenwert unterschreiten, damit sich das Schlupffenster öffnen kann. Die Aktivität der PTTHn wird durch das kurze Neuropeptid F (sNPF) aus den kleinen ventrolateralen Neuronen (sLNvs) gehemmt, und es wird angenommen, dass die Hemmung zu einer Abnahme der Ecdysonproduktion führt. Das allgemeine Ziel dieser Thesis besteht darin, die Koordination zwischen der zirkadianen Uhr und den neuroendokrinen Signalwegen zur Steuerung der Eklosionsrhythmik weiter zu charakterisieren und zu ermitteln, wann diese endokrinen Signalwege aktiv sind. In Kapitel I zeigen eine Reihe von Verhaltenstests, die auf der konditionalen Ausschaltung von PTTHn basieren, in Kombination mit Techniken zur Darstellung neuronaler Aktivität, wie z. B. nicht-invasives ARG-Luc imaging, dass PTTH-Signale kurz vor dem Schlupf aktiv und erforderlich sind und zur Phasenanpassung der Aktivität der PG am Ende der Puppenentwicklung dienen könnten. Trans-synaptische anatomische Färbungen identifizierten die sLNvs, die dorsalen Neuronen 1 (DN1), die dorsalen Neuronen 2 (DN2) und die lateralen posterioren Neuronen (LPNs) als Uhrneuronen, die dem PTTHn direkt vorgeschaltet sind. Das motorische Schlupfverhalten wird durch das Ecdysis-auslösende Hormon (ETH) ausgelöst, das ein Paar ventromedialer (Vm) Neuronen zur Freisetzung des Eklosionshormons (EH) anregt, welches positiv an die Quelle des ETH, die endokrinen Inka-Zellen, zurückkoppelt. In Kapitel II zeigte die trans-synaptische Nachverfolgung, dass die meisten Uhrneuronen Input für die Vm- und nicht-kanonischen EH-Neuronen liefern, sodass die Uhr möglicherweise die ETH/EH-Rückkopplungsschleife beeinflussen kann. Das Aktivitätsprofil der Inka-Zellen und Vm-Neuronen vor dem Schlupf wird beschrieben. Vm- und Inka-Zellen sind etwa sieben Stunden vor dem Schlupf aktiv. Interessanterweise scheinen alle EH-Neuronen ausschließlich peptiderg zu sein. In Kapitel III wurde mit Hilfe von Chemoconnectomics festgestellt, dass PTTH-Neuronen Rezeptoren für sNPF, Allatostatin A (AstA), Allatostatin C (AstC) und Myosuppressin (Ms) exprimieren, während EH nur Ms- und AstA-Rezeptoren exprimieren. Eklosionsversuche mit Fliegen, deren AstA-, AstC- oder Ms-Signalübertragung beeinträchtigt ist, zeigen unter konstanten Bedingungen keine Arrhythmie. Eine optogenetische Aktivierung der AstA-Neuronen führt jedoch zu einer starken Unterdrückung des Schlupfs. Kapitel IV konzentriert sich auf die peripheren ventralen Trachealdendritischen Neurone (v'Td) und dendritische Verzweigungsneurone der Klasse IV (C4da). Die C4da-Neuronen vermitteln die Lichtvermeidung der Larven durch endokrine PTTH-Signale. Die v'Td-Neuronen erhalten hauptsächlich O2/CO2-Input aus den Tracheen und sind den Vm-Neuronen vorgeschaltet, werden aber für die Schlupfrhythmik nicht benötigt. Die bedingte Ablation der C4da-Neuronen und das Knock-out von torso (Rezeptor für PTTH) in den C4da-Neuronen beeinträchtigten die Schlupfrhythmik. Sechs bis sieben Stunden vor dem Schlupf sind die PTTHn-, C4da- und Vm-Neuronen aktiv. Somit könnten C4da-Neuronen indirekt die PTTHn mit den Vm-Neuronen verbinden. Zusammenfassend lässt sich sagen, dass diese Arbeit unser Wissen über das zeitliche Aktivitätsmuster und der Rolle des PTTH signalling während der Puppenentwicklung und dem rhythmisches Schlupf erweitert. Sie liefert auch eine umfassende Charakterisierung der synaptischen und peptidergen Eingänge von Uhrneuronen zu PTTHn- und EH-Neuronen. AstA, AstC und Ms wurden als potenzielle Modulatoren der neuronalen Schlupfschaltkreise identifiziert und deuten auf einen indirekten Effekt der PTTH-Signalgebung auf das EH signalling über die peripheren sensorischen C4da-Neuronen hin. KW - Prothoracicotropic hormone KW - Prothoracic gland KW - Eclosion KW - Eclosion hormone KW - C4da KW - v’Td KW - Neuropeptide KW - Neuroendokrines System KW - Taufliege Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-361309 ER - TY - JOUR A1 - Dammert, Marcel A. A1 - Brägelmann, Johannes A1 - Olsen, Rachelle R. A1 - Böhm, Stefanie A1 - Monhasery, Niloufar A1 - Whitney, Christopher P. A1 - Chalishazar, Milind D. A1 - Tumbrink, Hannah L. A1 - Guthrie, Matthew R. A1 - Klein, Sebastian A1 - Ireland, Abbie S. A1 - Ryan, Jeremy A1 - Schmitt, Anna A1 - Marx, Annika A1 - Ozretić, Luka A1 - Castiglione, Roberta A1 - Lorenz, Carina A1 - Jachimowicz, Ron D. A1 - Wolf, Elmar A1 - Thomas, Roman K. A1 - Poirier, John T. A1 - Büttner, Reinhard A1 - Sen, Triparna A1 - Byers, Lauren A. A1 - Reinhardt, H. Christian A1 - Letai, Anthony A1 - Oliver, Trudy G. A1 - Sos, Martin L. T1 - MYC paralog-dependent apoptotic priming orchestrates a spectrum of vulnerabilities in small cell lung cancer JF - Nature Communications N2 - MYC paralogs are frequently activated in small cell lung cancer (SCLC) but represent poor drug targets. Thus, a detailed mapping of MYC-paralog-specific vulnerabilities may help to develop effective therapies for SCLC patients. Using a unique cellular CRISPR activation model, we uncover that, in contrast to MYCN and MYCL, MYC represses BCL2 transcription via interaction with MIZ1 and DNMT3a. The resulting lack of BCL2 expression promotes sensitivity to cell cycle control inhibition and dependency on MCL1. Furthermore, MYC activation leads to heightened apoptotic priming, intrinsic genotoxic stress and susceptibility to DNA damage checkpoint inhibitors. Finally, combined AURK and CHK1 inhibition substantially prolongs the survival of mice bearing MYC-driven SCLC beyond that of combination chemotherapy. These analyses uncover MYC-paralog-specific regulation of the apoptotic machinery with implications for genotype-based selection of targeted therapeutics in SCLC patients. KW - genetic engineering KW - oncogenes KW - small-cell lung cancer KW - targeted therapies Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-223569 VL - 10 ER - TY - JOUR A1 - Dörk, Thilo A1 - Peterlongo, Peter A1 - Mannermaa, Arto A1 - Bolla, Manjeet K. A1 - Wang, Qin A1 - Dennis, Joe A1 - Ahearn, Thomas A1 - Andrulis, Irene L. A1 - Anton-Culver, Hoda A1 - Arndt, Volker A1 - Aronson, Kristan J. A1 - Augustinsson, Annelie A1 - Beane Freeman, Laura E. A1 - Beckmann, Matthias W. A1 - Beeghly-Fadiel, Alicia A1 - Behrens, Sabine A1 - Bermisheva, Marina A1 - Blomqvist, Carl A1 - Bogdanova, Natalia V. A1 - Bojesen, Stig E. A1 - Brauch, Hiltrud A1 - Brenner, Hermann A1 - Burwinkel, Barbara A1 - Canzian, Federico A1 - Chan, Tsun L. A1 - Chang-Claude, Jenny A1 - Chanock, Stephen J. A1 - Choi, Ji-Yeob A1 - Christiansen, Hans A1 - Clarke, Christine L. A1 - Couch, Fergus J. A1 - Czene, Kamila A1 - Daly, Mary B. A1 - dos-Santos-Silva, Isabel A1 - Dwek, Miriam A1 - Eccles, Diana M. A1 - Ekici, Arif B. A1 - Eriksson, Mikael A1 - Evans, D. Gareth A1 - Fasching, Peter A. A1 - Figueroa, Jonine A1 - Flyger, Henrik A1 - Fritschi, Lin A1 - Gabrielson, Marike A1 - Gago-Dominguez, Manuela A1 - Gao, Chi A1 - Gapstur, Susan M. A1 - García-Closas, Montserrat A1 - García-Sáenz, José A. A1 - Gaudet, Mia M. A1 - Giles, Graham G. A1 - Goldberg, Mark S. A1 - Goldgar, David E. A1 - Guenél, Pascal A1 - Haeberle, Lothar A1 - Haimann, Christopher A. A1 - Håkansson, Niclas A1 - Hall, Per A1 - Hamann, Ute A1 - Hartman, Mikael A1 - Hauke, Jan A1 - Hein, Alexander A1 - Hillemanns, Peter A1 - Hogervorst, Frans B. L. A1 - Hooning, Maartje J. A1 - Hopper, John L. A1 - Howell, Tony A1 - Huo, Dezheng A1 - Ito, Hidemi A1 - Iwasaki, Motoki A1 - Jakubowska, Anna A1 - Janni, Wolfgang A1 - John, Esther M. A1 - Jung, Audrey A1 - Kaaks, Rudolf A1 - Kang, Daehee A1 - Kapoor, Pooja Middha A1 - Khusnutdinova, Elza A1 - Kim, Sung-Won A1 - Kitahara, Cari M. A1 - Koutros, Stella A1 - Kraft, Peter A1 - Kristensen, Vessela N. A1 - Kwong, Ava A1 - Lambrechts, Diether A1 - Le Marchand, Loic A1 - Li, Jingmei A1 - Lindström, Sara A1 - Linet, Martha A1 - Lo, Wing-Yee A1 - Long, Jirong A1 - Lophatananon, Artitaya A1 - Lubiński, Jan A1 - Manoochehri, Mehdi A1 - Manoukian, Siranoush A1 - Margolin, Sara A1 - Martinez, Elena A1 - Matsuo, Keitaro A1 - Mavroudis, Dimitris A1 - Meindl, Alfons A1 - Menon, Usha A1 - Milne, Roger L. A1 - Mohd Taib, Nur Aishah A1 - Muir, Kenneth A1 - Mulligan, Anna Marie A1 - Neuhausen, Susan L. A1 - Nevanlinna, Heli A1 - Neven, Patrick A1 - Newman, William G. A1 - Offit, Kenneth A1 - Olopade, Olufunmilayo I. A1 - Olshan, Andrew F. A1 - Olson, Janet E. A1 - Olsson, Håkan A1 - Park, Sue K. A1 - Park-Simon, Tjoung-Won A1 - Peto, Julian A1 - Plaseska-Karanfilska, Dijana A1 - Pohl-Rescigno, Esther A1 - Presneau, Nadege A1 - Rack, Brigitte A1 - Radice, Paolo A1 - Rashid, Muhammad U. A1 - Rennert, Gad A1 - Rennert, Hedy S. A1 - Romero, Atocha A1 - Ruebner, Matthias A1 - Saloustros, Emmanouil A1 - Schmidt, Marjanka K. A1 - Schmutzler, Rita K. A1 - Schneider, Michael O. A1 - Schoemaker, Minouk J. A1 - Scott, Christopher A1 - Shen, Chen-Yang A1 - Shu, Xiao-Ou A1 - Simard, Jaques A1 - Slager, Susan A1 - Smichkoska, Snezhana A1 - Southey, Melissa C. A1 - Spinelli, John J. A1 - Stone, Jennifer A1 - Surowy, Harald A1 - Swerdlow, Anthony J. A1 - Tamimi, Rulla M. A1 - Tapper, William J. A1 - Teo, Soo H. A1 - Terry, Mary Beth A1 - Toland, Amanda E. A1 - Tollenaar, Rob A. E. M. A1 - Torres, Diana A1 - Torres-Mejía, Gabriela A1 - Troester, Melissa A. A1 - Truong, Thérèse A1 - Tsugane, Shoichiro A1 - Untch, Michael A1 - Vachon, Celine M. A1 - van den Ouweland, Ans M. W. A1 - van Veen, Elke M. A1 - Vijai, Joseph A1 - Wendt, Camilla A1 - Wolk, Alicja A1 - Yu, Jyh-Cherng A1 - Zheng, Wei A1 - Ziogas, Argyrios A1 - Ziv, Elad A1 - Dunnig, Alison A1 - Pharaoh, Paul D. P. A1 - Schindler, Detlev A1 - Devilee, Peter A1 - Easton, Douglas F. T1 - Two truncating variants in FANCC and breast cancer risk JF - Scientific Reports N2 - Fanconi anemia (FA) is a genetically heterogeneous disorder with 22 disease-causing genes reported to date. In some FA genes, monoallelic mutations have been found to be associated with breast cancer risk, while the risk associations of others remain unknown. The gene for FA type C, FANCC, has been proposed as a breast cancer susceptibility gene based on epidemiological and sequencing studies. We used the Oncoarray project to genotype two truncating FANCC variants (p.R185X and p.R548X) in 64,760 breast cancer cases and 49,793 controls of European descent. FANCC mutations were observed in 25 cases (14 with p.R185X, 11 with p.R548X) and 26 controls (18 with p.R185X, 8 with p.R548X). There was no evidence of an association with the risk of breast cancer, neither overall (odds ratio 0.77, 95%CI 0.44–1.33, p = 0.4) nor by histology, hormone receptor status, age or family history. We conclude that the breast cancer risk association of these two FANCC variants, if any, is much smaller than for BRCA1, BRCA2 or PALB2 mutations. If this applies to all truncating variants in FANCC it would suggest there are differences between FA genes in their roles on breast cancer risk and demonstrates the merit of large consortia for clarifying risk associations of rare variants. KW - oncology KW - risk factors Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-222838 VL - 9 ER - TY - JOUR A1 - Dunce, James M. A1 - Milburn, Amy E. A1 - Gurusaran, Manickam A1 - da Cruz, Irene A1 - Sen, Lee T. A1 - Benavente, Ricardo A1 - Davies, Owen R. T1 - Structural basis of meiotic telomere attachment to the nuclear envelope by MAJIN-TERB2-TERB1 JF - Nature Communications N2 - Meiotic chromosomes undergo rapid prophase movements, which are thought to facilitate the formation of inter-homologue recombination intermediates that underlie synapsis, crossing over and segregation. The meiotic telomere complex (MAJIN, TERB1, TERB2) tethers telomere ends to the nuclear envelope and transmits cytoskeletal forces via the LINC complex to drive these rapid movements. Here, we report the molecular architecture of the meiotic telomere complex through the crystal structure of MAJIN-TERB2, together with light and X-ray scattering studies of wider complexes. The MAJIN-TERB2 2:2 hetero-tetramer binds strongly to DNA and is tethered through long flexible linkers to the inner nuclear membrane and two TRF1-binding 1:1 TERB2-TERB1 complexes. Our complementary structured illumination microscopy studies and biochemical findings reveal a telomere attachment mechanism in which MAJIN-TERB2-TERB1 recruits telomere-bound TRF1, which is then displaced during pachytene, allowing MAJIN-TERB2-TERB1 to bind telomeric DNA and form a mature attachment plate. KW - DNA KW - meiosis KW - proteins KW - super-resolution microscopy KW - X-ray crystallography Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-226416 VL - 9 ER - TY - JOUR A1 - Steuer Costa, Wagner A1 - Van der Auwera, Petrus A1 - Glock, Caspar A1 - Liewald, Jana F. A1 - Bach, Maximilian A1 - Schüler, Christina A1 - Wabnig, Sebastian A1 - Oranth, Alexandra A1 - Masurat, Florentin A1 - Bringmann, Henrik A1 - Schoofs, Liliane A1 - Stelzer, Ernst H. K. A1 - Fischer, Sabine C. A1 - Gottschalk, Alexander T1 - A GABAergic and peptidergic sleep neuron as a locomotion stop neuron with compartmentalized Ca2+ dynamics JF - Nature Communications N2 - Animals must slow or halt locomotion to integrate sensory inputs or to change direction. In Caenorhabditis elegans, the GABAergic and peptidergic neuron RIS mediates developmentally timed quiescence. Here, we show RIS functions additionally as a locomotion stop neuron. RIS optogenetic stimulation caused acute and persistent inhibition of locomotion and pharyngeal pumping, phenotypes requiring FLP-11 neuropeptides and GABA. RIS photoactivation allows the animal to maintain its body posture by sustaining muscle tone, yet inactivating motor neuron oscillatory activity. During locomotion, RIS axonal Ca2+ signals revealed functional compartmentalization: Activity in the nerve ring process correlated with locomotion stop, while activity in a branch correlated with induced reversals. GABA was required to induce, and FLP-11 neuropeptides were required to sustain locomotion stop. RIS attenuates neuronal activity and inhibits movement, possibly enabling sensory integration and decision making, and exemplifies dual use of one cell across development in a compact nervous system. KW - Cellular neuroscience KW - Neural circuits Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-223273 VL - 10 ER - TY - THES A1 - Nirchal, Naveen Kumar T1 - Mechanistische Regulierung des gastroösophagealen Übergangs und die Rolle der Retinsäure bei der Entwicklung des Barrett-Ösophagus T1 - Mechanistic regulation of gastroesophageal junction and role of retinoic acid in the development of Barrett's esophagus N2 - Der gastroösophageale Übergang (GEJ), der die Region abgrenzt, in der der distale Ösophagus auf die proximale Magenregion trifft, ist bekannt für die Entwicklung pathologischer Zustände, wie Metaplasie und Adenokarzinom des Ösophagus (EAC). Es ist wichtig, die Mechanismen der Entwicklungsstadien zu verstehen, die zu EAC führen, da die Inzidenzrate von EAC in den letzten 4 Jahrzehnten um das 7-fache gestiegen ist und die Gesamtüberlebensrate von 5 Jahren 18,4 % beträgt. In den meisten Fällenwird die Diagnose im fortgeschrittenen Stadium ohne vorherige Symptome erstellt. Der Hauptvorläufer für die Entwicklung von EAC ist eine prämaligne Vorstufe namens Barrett-Ösophagus (BE). BE ist der metaplastische Zustand, bei dem das mehrschichtige Plattenepithel des nativen Ösophagus durch ein spezialisiertes einschichtiges Säulenepithel ersetzt wird, das die molekularen Eigenschaften des Magen- sowie des Darmepithels aufweist. Zu den wichtigsten Risikofaktoren für die Entwicklung von BE gehören die chronische gastroösophageale Refluxkrankheit (GERD), eine veränderte Mikrobiota und veränderte Retinsäure-Signalwege (RA). Es ist unklar, welche Zelle der Ursprung für BE ist, da es keine eindeutigen Beweisen für den Prozess der BE-Initiation gibt. In dieser Arbeit habe ich untersucht, wie die GEJ-Homöostase in gesundem Gewebe durch stammzellregulatorische Morphogene aufrechterhalten wird, welche Rolle der Vitamin-A (RA-Signalübertragung) spieltund wie ihre Veränderung zur BE-Entwicklung beiträgt. Im ersten Teil meiner Dissertation habe ich anhand von Einzelmolekül-RNA in situ-Hybridisierung und Immunhistochemie eindeutig das Vorhandensein von zwei Arten von Epithelzellen nachweisen können, dem Plattenepithel in der Speiseröhre und dem Säulenepithel imMagenbereich des GEJ. Mittels Abstammungsanalysen im Mausmodell konnte ich zeigen, dass die Epithelzellen des Ösophagus und des Magens von zwei verschiedenen epithelialen Stammzelllinien imGEJ abstammen. Die Grenze zwischen Plattenepithel und Säulenepithelzellen im SCJ des GEJ wirddurch gegensätzliche Wnt-Mikroumgebungen streng reguliert. Plattenepithelstammzellen des Ösophagus werden durch das Wnt-hemmende Mikroumgebungssignal aufrechterhalten, während Magensäulenepithelzellen durch das Wnt-aktivierende Signal aus dem Stromakompartiment erhalten werden. Ich habe die in vivo Erhaltung der Epithelstammzellen des GEJ mit Hilfe eines in vitro Epithel-3D-Organoidkulturmodells rekonstruiert. Das Wachstum und die Vermehrung von Magensäulenepithel-Organoiden hängen von Wnt-Wachstumsfaktoren ab, während das Wachstum von Plattenepithel-Organoiden von Wnt-defizienten Kulturbedingungen abhängt. Darüber hinaus zeigte die Einzelzell-RNA-Sequenzanalyse (scRNA-seq) der aus Organoiden gewonnenenEpithelzellen, dass der nicht-kanonische Wnt/ planar cell polarity (PCP) Signalweg an der Regulierung der Plattenepithelzellen beteiligt ist. Im Gegensatz dazu werden säulenförmige Magenepithelzellen durch den kanonischen Wnt/beta-Catenin- und den nicht-kanonischen Wnt/Ca2+-Weg reguliert. Meine Daten zeigen, dass die SCJ-Epithelzellen, die am GEJ verschmelzen, durch entgegengesetzte stromale Wnt-Faktoren und unterschiedliche Wnt-Weg-Signalee in den Epithelzellen reguliert werden. Im zweiten Teil der Dissertation untersuchte ich die Rolle der bioaktiven Vitamin A Verbindung RA auf Ösophagus- und Magenepithelstammzellen. Die In-vitro-Behandlung von epithelialen Organoiden der Speiseröhre und des Magens mitRA oder seinem pharmakologischen Inhibitors BMS 493 zeigte, dass jeder Zelltyp unterschiedlich reguliert wurde. Ich beobachtete, dass eine verstärkte RA die Differenzierung von Stammzellen und den Verlust der Schichtung förderte, während die RA-Hemmung zu einer verstärkten Stammzellbildung und Regeneration im mehrschichtigen Epithel der Speiseröhre führte. Im Gegensatz zur Speiseröhre ist der RA-Signalweg in Magen-Organoiden aktiv, und die Hemmung von RA hat ein reduziertes Wachstum von Magen-Organoiden. Globale transkriptomische Daten und scRNA-seq-Daten zeigten, dass derRA-Signalweg einen Ruhephänotyp in den Ösophaguszellen induziert. Dagegen führt das Fehlen von RA in Magenepithelzellen zur Expression von Genen, die mit BE assoziiert sind. Daher isteine räumlich definierte Regulation der Wnt- und Retinsäure-Signalgebung amGEJ entscheidend für eine gesunde Homöostase, und ihre Störung führt zur Entwicklung von Krankheiten. N2 - Gastroesophageal junction (GEJ), demarcating the region where the distal esophagus meets with the proximal stomach region, is known for developing pathological conditions, including metaplasia and esophageal adenocarcinoma (EAC). It is essential to understand the mechanisms of developmental stages which lead to EAC since the incidence rate of EAC increased over 7-fold during the past four decades, and the overall five years survival rate is 18.4%. In most cases, patients are diagnosed in the advanced stage without prior symptoms. The main precursor for the development of EAC is a pre-malignant condition called Barrett's esophagus (BE). BE is the metaplastic condition where the multilayered squamous epithelium of the native esophagus is replaced by specialized single-layered columnar epithelium, which shows the molecular characteristics of the gastric as well as intestinal epithelium. The main risk factors for BE development include chronic gastro-esophageal acid reflux disease (GERD), altered microbiota, and altered retinoic acid signaling (RA). The cell of origin of BE is under debate due to a lack of clear evidence demonstrating the process of BE initiation. Here, I investigated how GEJ homeostasis is maintained in healthy tissue by stem cell regulatory morphogens, the role of vitamin A (RA signaling), and how its alteration contributes to BE development. In the first part of my thesis, I showed the presence of two types of epithelial cells, the squamous type in the esophagus and the columnar type in the stomach region in the GEJ, using single-molecule RNA in situ hybridization (smRNA-ISH) and immunohistochemistry. Employing lineage tracing in the mouse model, I have demonstrated that the esophageal epithelial and stomach epithelial cells derived from two distinct epithelial stem cell lineages in the GEJ. The border between squamous and columnar epithelial cells in the Squamo-columnar junction (SCJ) of GEJ is regulated by opposing Wnt microenvironments. The regeneration of stomach columnar epithelial stem cells is maintained by Wnt activating signal from the stromal compartment while squamous epithelial stem cells of the esophagus are maintained by the Wnt inhibitory signals. I recapitulated the in vivo GEJ epithelial stem cell maintenance by using in vitro epithelial 3D organoid culture model. The growth and propagation of stomach columnar epithelial organoids depend on Wnt growth factors, while squamous epithelial organoids' development needs Wnt-deficient culture conditions. Further, single-cell RNA sequence (scRNA-seq) analysis of organoid-derived epithelial cells revealed the non-canonical Wnt/ planar cell polarity (PCP) pathway involvement in regulating the squamous epithelial cells. In contrast, columnar stomach epithelial cells are regulated by the canonical Wnt/ beta-catenin and non-canonical Wnt/Ca2+ pathways. My data indicate that the SCJ epithelial cells that merge at the GEJ are regulated by opposing stromal Wnt factors and distinct Wnt pathway signaling in the epithelial cells. In the second part of the thesis, I investigated the role of Vitamin A-derived bioactive compound RA on esophageal and stomach epithelial stem cells. In vitro treatment of esophageal and stomach, epithelial organoids with RA or its pharmacological inhibitor BMS 493 revealed that each cell type was regulated distinctly. I observed that enhanced RA promoted esophageal stem cell differentiation and loss of stratification, while RA inhibition led to enhanced stemness and regeneration of the esophagus stratified epithelium. As opposed to the esophagus, RA signaling is active in the stomach organoids, and inhibition of RA reduces the growth of stomach organoids. Global transcriptomic data and scRNA-seq data revealed that RA signaling induces dormancy phenotype in the esophageal cells. In contrast, the absence of RA in stomach epithelial cells induces the expression of genes associated with BE. Thus, spatially defined regulation of Wnt and RA signaling at GEJ is critical for healthy homeostasis, and its perturbation leads to disease development. KW - Retinoesäure KW - Esophageal adenocarcinoma KW - Intestinal metaplasia KW - Epithelial lineage KW - Organoid KW - Retinoic acid KW - Gastroesophageal reflux KW - Endobrachyösophagus KW - Esophageal disease Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-311556 ER - TY - INPR A1 - Hennig, Thomas A1 - Prusty, Archana B. A1 - Kaufer, Benedikt A1 - Whisnant, Adam W. A1 - Lodha, Manivel A1 - Enders, Antje A1 - Thomas, Julius A1 - Kasimir, Francesca A1 - Grothey, Arnhild A1 - Herb, Stefanie A1 - Jürges, Christopher A1 - Meister, Gunter A1 - Erhard, Florian A1 - Dölken, Lars A1 - Prusty, Bhupesh K. T1 - Selective inhibition of miRNA 1 processing by a herpesvirus encoded miRNA N2 - Herpesviruses have mastered host cell modulation and immune evasion to augment productive infection, life-long latency and reactivation thereof 1,2. A long appreciated, yet elusively defined relationship exists between the lytic-latent switch and viral non-coding RNAs 3,4. Here, we identify miRNA-mediated inhibition of miRNA processing as a thus far unknown cellular mechanism that human herpesvirus 6A (HHV-6A) exploits to disrupt mitochondrial architecture, evade intrinsic host defense and drive the lytic-latent switch. We demonstrate that virus-encoded miR-aU14 selectively inhibits the processing of multiple miR-30 family members by direct interaction with the respective pri-miRNA hairpin loops. Subsequent loss of miR-30 and activation of the miR-30/p53/Drp1 axis triggers a profound disruption of mitochondrial architecture. This impairs induction of type I interferons and is necessary for both productive infection and virus reactivation. Ectopic expression of miR-aU14 triggered virus reactivation from latency, identifying viral miR-aU14 as a readily drugable master regulator of the herpesvirus lytic-latent switch. Our results show that miRNA-mediated inhibition of miRNA processing represents a generalized cellular mechanism that can be exploited to selectively target individual members of miRNA families. We anticipate that targeting miR-aU14 provides exciting therapeutic options for preventing herpesvirus reactivations in HHV-6-associated disorders. KW - Herpesvirus KW - HHV-6A KW - miRNA processing KW - miR-30 KW - mitochondria KW - fusion and fission KW - type I interferon KW - latency KW - virus reactivation Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-267862 ET - accepted version ER - TY - JOUR A1 - Eckert, Johanna A1 - Bohn, Manuel A1 - Spaethe, Johannes T1 - Does quantity matter to a stingless bee? JF - Animal Cognition N2 - Quantitative information is omnipresent in the world and a wide range of species has been shown to use quantities to optimize their decisions. While most studies have focused on vertebrates, a growing body of research demonstrates that also insects such as honeybees possess basic quantitative abilities that might aid them in finding profitable flower patches. However, it remains unclear if for insects, quantity is a salient feature relative to other stimulus dimensions, or if it is only used as a “last resort” strategy in case other stimulus dimensions are inconclusive. Here, we tested the stingless bee Trigona fuscipennis, a species representative of a vastly understudied group of tropical pollinators, in a quantity discrimination task. In four experiments, we trained wild, free-flying bees on stimuli that depicted either one or four elements. Subsequently, bees were confronted with a choice between stimuli that matched the training stimulus either in terms of quantity or another stimulus dimension. We found that bees were able to discriminate between the two quantities, but performance differed depending on which quantity was rewarded. Furthermore, quantity was more salient than was shape. However, quantity did not measurably influence the bees' decisions when contrasted with color or surface area. Our results demonstrate that just as honeybees, small-brained stingless bees also possess basic quantitative abilities. Moreover, invertebrate pollinators seem to utilize quantity not only as "last resort" but as a salient stimulus dimension. Our study contributes to the growing body of knowledge on quantitative cognition in invertebrate species and adds to our understanding of the evolution of numerical cognition. KW - numerical cognition KW - insects KW - Trigona fuscipennis KW - associative learning KW - quantity discrimination KW - behavioral experiments Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-307696 SN - 1435-9448 SN - 1435-9456 VL - 25 IS - 3 ER - TY - JOUR A1 - Loos, Jacqueline A1 - Krauss, Jochen A1 - Lyons, Ashley A1 - Föst, Stephanie A1 - Ohlendorf, Constanze A1 - Racky, Severin A1 - Röder, Marina A1 - Hudel, Lennart A1 - Herfert, Volker A1 - Tscharntke, Teja T1 - Local and landscape responses of biodiversity in calcareous grasslands JF - Biodiversity and Conservation N2 - Across Europe, calcareous grasslands become increasingly fragmented and their quality deteriorates through abandonment and land use intensification, both affecting biodiversity. Here, we investigated local and landscape effects on diversity patterns of several taxonomic groups in a landscape of highly fragmented calcareous grassland remnants. We surveyed 31 grassland fragments near Göttingen, Germany, in spring and summer 2017 for vascular plants, butterflies and birds, with sampling effort adapted to fragment area. Through regression modelling, we tested relationships between species richness and fragment size (from 314 to 51,395 m\(^2\)), successional stage, habitat connectivity and the per cent cover of arable land in the landscape at several radii. We detected 283 plant species, 53 butterfly species and 70 bird species. Of these, 59 plant species, 19 butterfly species and 9 bird species were grassland specialists. Larger fragments supported twice the species richness of plants than small ones, and hosted more species of butterflies, but not of birds. Larger grassland fragments contained more grassland specialist plants, but not butterfly or bird specialists. Increasing amounts of arable land in the landscape from 20 to 90% was related to the loss of a third of species of plants, and less so, of butterflies, but not of birds. Per cent cover of arable land negatively correlated to richness of grassland specialist plants and butterflies, but positively to grassland specialist birds. We found no effect by successional stages and habitat connectivity. Our multi-taxa approach highlights the need for conservation management at the local scale, complemented by measures at the landscape scale. KW - abandonment KW - birds KW - butterflies KW - land use intensification KW - nature conservation KW - vascular plants Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-308595 SN - 0960-3115 SN - 1572-9710 VL - 30 IS - 8-9 ER - TY - THES A1 - König, Sebastian Thomas T1 - Temperature-driven assembly processes of Orthoptera communities: Lessons on diversity, species traits, feeding interactions, and associated faecal microorganisms from elevational gradients in Southern Germany (Berchtesgaden Alps) T1 - Temperaturabhängige Zusammensetzungsprozesse von Heuschreckengemeinschaften: Lektionen über die Diversität, Artmerkmale, Fraßinteraktionen, und Kot-Mikroorganismen von Höhengradienten in Süddeutschland (Berchtesgadener Alpen) N2 - Chapter I: Introduction Temperature is a major driver of biodiversity and abundance patterns on our planet, which becomes particularly relevant facing the entanglement of an imminent biodiversity and climate crisis. Climate shapes the composition of species assemblages either directly via abiotic filtering mechanisms or indirectly through alterations in biotic interactions. Insects - integral elements of Earth’s ecosystems - are affected by climatic variation such as warming, yet responses vary among species. While species’ traits, antagonistic biotic interactions, and even species’ microbial mutualists may determine temperature-dependent assembly processes, the lion’s share of these complex relationships remains poorly understood due to methodological constraints. Mountains, recognized as hotspots of diversity and threatened by rapidly changing climatic conditions, can serve as natural experimental settings to study the response of insect assemblages and their trophic interactions to temperature variation, instrumentalizing the high regional heterogeneity of micro- and macroclimate. With this thesis, we aim to enhance our mechanistic understanding of temperature-driven assembly processes within insect communities, exemplified by Orthoptera, that are significant herbivores in temperate mountain grassland ecosystems. Therefore, we combined field surveys of Orthoptera assemblages on grassland sites with molecular tools for foodweb reconstruction, primarily leveraging the elevational gradients offered by the complex topography within the Berchtesgaden Alpine region (Bavaria, Germany) as surrogate for temperature variation (space-for-time substitution approach). In this framework, we studied the effects of temperature variation on (1) species richness, abundance, community composition, and interspecific as well as intraspecific trait patterns, (2) ecological feeding specialisation, and (3) previously neglected links to microbial associates found in the faeces. Chapter II: Temperature-driven assembly processes Climate varies at multiple scales. Since microclimate is often overlooked, we assessed effects of local temperature deviations on species and trait compositions of insect communities along macroclimatic temperature gradients in Chapter II. Therefore, we employed joint species distribution modelling to explore how traits drive variation in the climatic niches of Orthoptera species at grassland sites characterized by contrasting micro- and macroclimatic conditions. Our findings revealed two key insights: (1) additive effects of micro- and macroclimate on the diversity, but (2) interactive effects on the abundance of several species, resulting in turnover and indicating that species possess narrower climatic niches than their elevational distributions might imply. This chapter suggests positive effects of warming on Orthoptera, but also highlights that the interplay of macro- and microclimate plays a pivotal role in structuring insect communities. Thus, it underscores the importance of considering both elements when predicting the responses of species to climate change. Additionally, this chapter revealed inter- and intraspecific effects of traits on the niches and distribution of species. Chapter III: Dietary specialisation along climatic gradients A crucial trait linked to the position of climatic niches is dietary specialisation. According to the ‘altitudinal niche-breadth hypothesis’, species of high-elevation habitats should be less specialized compared to their low-elevation counterparts. However, empirical evidence on shifts in specialization is scarce for generalist insect herbivores and existing studies often fail to control for the phylogeny and abundance of interaction partners. In Chapter III, we used a combination of field observations and amplicon sequencing to reconstruct dietary relationships between Orthoptera and plants along an extensive temperature gradient. We did not find close but flexible links between individual grasshopper and plant taxa in space. While interaction network specialisation increased with temperature, the corrected dietary specialisation pattern peaked at intermediate elevations on assemblage level. These nuanced findings demonstrate that (1) resource availability, (2) phylogenetic relationships, and (3) climate can affect empirical foodwebs intra- and interspecifically and, hence, the dietary specialisation of herbivorous insects. In this context, we discuss that the underlying mechanisms involved in shaping the specialisation of herbivore assemblages may switch along temperature clines. Chapter IV: Links between faecal microbe communities, feeding habits, and climate Since gut microbes affect the fitness and digestion of insects, studying their diversity could provide novel insights into specialisation patterns. However, their association with insect hosts that differ in feeding habits and specialisation has never been investigated along elevational climatic gradients. In Chapter IV, we utilized the dietary information gathered in Chapter III to characterize links between insects with distinct feeding behaviour and the microbial communities present in their faeces, using amplicon sequencing. Both, feeding and climate affected the bacterial communities. However, the large overlap of microbes at site level suggests that common bacteria are acquired from the shared feeding environment, such as the plants consumed by the insects. These findings emphasize the influence of a broader environmental context on the composition of insect gut microbial communities. Chapter V: Discussion & Conclusions Cumulatively, the sections of this dissertation provide support for the hypothesis that climatic conditions play a role in shaping plant–herbivore systems. The detected variation of taxonomic and functional compositions contributes to our understanding of assembly processes and resulting diversity patterns within Orthoptera communities, shedding light on the mechanisms that structure their trophic interactions in diverse climates. The combined results presented suggest that a warmer climate could foster an increase of Orthoptera species richness in Central European semi-natural grasslands, also because the weak links observed between insect herbivores and plants are unlikely to limit decoupled range shifts. However, the restructuring of Orthoptera communities in response to warmer temperatures depends on species' traits such as moisture preferences or phenology. Notably, we were able to demonstrate a crucial role of microclimate for many species, partly unravelling narrower climatic niches than their elevational ranges suggest. We found evidence that not only Orthoptera community composition, specialisation, and traits varied along elevational gradients, but even microbial communities in the faeces of Orthoptera changed, which is a novel finding. This complex restructuring and reassembly of communities, coupled with the nonlinear specialisation of trophic interactions and a high diversity of associated bacteria, emphasize our currently incomplete comprehension of how ecosystems will develop under future climatic conditions, demanding caution in making simplified predictions for biodiversity change under climate warming. Since these predictions may benefit from including biotic interactions and both, micro- and macroclimate based on our findings, conservation authorities and practitioners must not neglect improving microclimatic conditions to ensure local survival of a diverse set of threatened and demanding species. In this context, mountains can play a pivotal role for biodiversity conservation since these offer heterogeneous microclimatic conditions in proximity that can be utilized by species with distinct niches. N2 - Kapitel I: Einleitung Die Temperatur ist eine wichtige Triebkraft hinter den Artenvielfalts- und Abundanzmustern auf unserem Planeten, was angesichts der Verflechtung der unmittelbar bevorstehenden Biodiversitäts- und Klimakrise besonders relevant ist. Das Klima strukturiert die Artenvielfalt direkt durch abiotische Filtermechanismen oder indirekt durch Veränderungen biotischer Wechselwirkungen. Insekten - wesentliche Bestandteile der Ökosysteme der Erde - sind von klimatischen Veränderungen wie der Erwärmung betroffen, reagieren aber je nach Art unterschiedlich. Während die Merkmale der Arten, antagonistische biotische Interaktionen und sogar die mikrobiellen Partner der Arten temperaturabhängige Zusammensetzungsprozesse bestimmen können, bleibt ein Großteil dieser komplexen Beziehungen aufgrund methodischer Einschränkungen nach wie vor schlecht verstanden. Gebirge, die als Hotspots der Diversität gelten und von sich rasch verändernden klimatischen Bedingungen bedroht sind, können durch Nutzung der großen regionalen Heterogenität der Klein- und Großklimate als natürliche Experimente dienen, um die Reaktion von Insektengemeinschaften und deren trophischen Interaktionen auf Temperaturänderungen zu untersuchen. Mit dieser Arbeit möchten wir einen Beitrag zum mechanistischen Verständnis der temperaturbedingten Zusammensetzungsprozesse von Insektengemeinschaften leisten, am Beispiel von Heuschrecken, die bedeutende Pflanzenfresser in Grünlandökosystemen der gemäßigten Breiten sind. Hierfür kombinierten wir Felduntersuchungen von Heuschreckengemeinschaften in Grünlandstandorten mit molekularen Methoden zur Rekonstruktion von Nahrungsbeziehungen, wobei wir hauptsächlich die Höhengradienten, die die komplexe Topografie der Berchtesgadener Alpenregion (Bayern, Deutschland) bietet, stellvertretend für Temperaturveränderungen verwendeten (Raum-Zeit-Substitutionsansatz). In diesem Rahmen untersuchten wir die Auswirkungen von Temperaturvariation auf (1) den Artenreichtum, die Abundanz, die Zusammensetzung der Gemeinschaft und die inter- und intraspezifischen Merkmalsmuster, (2) die ökologische Nahrungsspezialisierung und (3) die bis dato vernachlässigte Verbindung zu den mikrobiellen Begleitarten im Kot. Kapitel II: Temperaturabhängige Zusammensetzungsprozesse Das Klima variiert auf verschiedenen Ebenen. Da Veränderungen im Kleinklima oft vernachlässigt werden, haben wir in Kapitel II die Auswirkungen der lokalen Temperaturunterschiede auf die Arten- und Merkmalszusammensetzung von Insektengemeinschaften entlang makroklimatischer Temperaturgradienten untersucht. Hierfür haben wir die Methode der gemeinsamen Artenverteilungsmodellierung verwendet, um zu untersuchen, wie Artmerkmale die Unterschiede in klimatischen Nischen von Heuschreckenarten auf Grünlandstandorten mit gegensätzlichen mikro- und makroklimatischen Bedingungen beeinflussen. Unsere Ergebnisse brachten zwei wichtige Erkenntnisse zutage: (1) additive Auswirkungen des Mikro- und Makroklimas auf die Vielfalt, aber (2) interaktive Effekte auf die Häufigkeit mehrerer Arten, die sich in Zusammensetzungsunterschieden niederschlagen und auf engere klimatische Nischen hinweisen, als es die Höhenverbreitung vermuten lässt. Dieses Kapitel deutet auf positive Auswirkungen einer Erwärmung auf Orthoptera hin, zeigt aber auch, dass das Zusammenspiel von Makro- und Mikroklima eine Schlüsselrolle bei der Strukturierung von Insektengemeinschaften spielt und beide Elemente bei der Vorhersage der Reaktionen von Arten auf den Klimawandel berücksichtigt werden sollten. Darüber hinaus wurden in diesem Kapitel die inter- und intraspezifischen Auswirkungen von Merkmalen auf die Nischen und die Verbreitung von Arten aufgezeigt. Kapitel III: Nahrungsspezialisierung entlang von Klimagradienten Ein entscheidendes Merkmal für die Lage der klimatischen Nische einer Art ist die Nahrungsspezialisierung. Nach der "Hypothese der Höhenlagen-abhängigen Nischenbreite" sollten Arten in hoch gelegenen Lebensräumen weniger spezialisiert sein als ihre Pendants in niedrigen Lagen. Empirische Belege für Verschiebungen in der Spezialisierung von generalistischen, herbivoren Insekten sind jedoch rar und es fehlt eine Berücksichtigung der Häufigkeit und Phylogenie von Interaktionspartnern. In Kapitel III haben wir eine Kombination aus Feldbeobachtungen und Amplikonsequenzierung verwendet, um die Nahrungsbeziehungen von Heuschrecken und Pflanzen entlang eines ausgedehnten Temperaturgradienten zu rekonstruieren. Wir konnten keine engen, sondern flexible Beziehungen zwischen einzelnen Herbivoren- und Pflanzentaxa feststellen. Während die Spezialisierung der Interaktionsnetzwerke mit der Temperatur zunahm, erreichte das korrigierte Muster der Nahrungsspezialisierung auf Gemeinschaftsebene seinen Höhepunkt in mittleren Höhenlagen. Diese differenzierten Ergebnisse zeigen, dass (1) die Verfügbarkeit von Ressourcen, (2) phylogenetische Beziehungen und (3) das Klima intra- und interspezifische empirische Nahrungsbeziehungen und damit die Nahrungsspezialisierung pflanzenfressender Insekten beeinflussen können. In diesem Kontext diskutieren wir, dass die zugrundeliegenden Mechanismen hinter der Nahrungsspezialisierung von herbivoren Insekten entlang von Temperaturgradienten wechseln könnten. Kapitel IV: Verbindungen zwischen Kotbakteriengemeinschaften, Ernährungsgewohnheiten und Klima. Da Darmbakterien die Fitness und Verdauung von Insekten beeinflussen, könnte die Untersuchung deren Vielfalt neue Erkenntnisse über Spezialisierungsmuster liefern. Ihre Verbindung mit Insekten, die sich in ihren Ernährungsgewohnheiten und ihrer Spezialisierung unterscheiden, wurde jedoch noch nie entlang klimatischer Höhengradienten untersucht. In Kapitel IV verwendeten wir Nahrungsinformationen aus Kapitel III, um mit Hilfe von Amplikonsequenzierung Verbindungen zwischen Insekten mit unterschiedlichem Ernährungsverhalten und mikrobiellen Gemeinschaften in deren Kot zu charakterisieren. Sowohl die Nahrung als auch das Klima hatten Auswirkungen auf die bakteriellen Gemeinschaften. Die große Überschneidung der Mikrobengemeinschaften auf Standortebene deutet jedoch darauf hin, dass gemeinsame Bakterien aus der geteilten Nahrungsumgebung, wie z.B. den von den Insekten verzehrten Pflanzen, stammen. Diese Ergebnisse unterstreichen den Einfluss eines breiteren Umweltkontextes auf die Zusammensetzung der mikrobiellen Gemeinschaften im Insektendarm. Kapitel V: Diskussion & Schlussfolgerungen Insgesamt stützen die Kapitel dieser Dissertation die Hypothese, dass klimatische Verhältnisse Pflanzen-Pflanzenfresser-Systeme prägen. Die festgestellten Unterschiede in der taxonomischen und funktionellen Zusammensetzung tragen zu unserem Verständnis der Zusammensetzungsprozesse und daraus resultierenden Diversitätsmustern von Heuschreckengemeinschaften sowie der Mechanismen bei, die deren trophische Interaktionen in verschiedenen Klimazonen strukturieren. Die Kombination der Ergebnisse deutet darauf hin, dass wärmeres Klima eine Zunahme des Heuschreckenartenreichtums in naturnahen Grünlandgebieten Mitteleuropas begünstigen könnte, auch weil die schwachen Verbindungen zwischen den herbivoren Insekten und Pflanzen entkoppelte Arealverschiebungen wahrscheinlich nicht limitieren. Jedoch könnten höhere Temperaturen die Zusammensetzung von Heuschreckengemeinschaften je nach den Merkmalen der Arten wie deren Feuchtigkeitsvorlieben oder der Schlupfphänologie verändern. Darüber hinaus konnten wir nachweisen, dass das Mikroklima für viele Arten eine entscheidende Rolle spielt, da es teilweise engere klimatische Nischen aufdeckt, als ihre Höhenverbreitung vermuten lassen. Wir fanden Hinweise darauf, dass sich nicht nur die Zusammensetzung, Spezialisierung und Merkmale der Heuschreckengemeinschaften entlang der Höhengradienten ändern, sondern dass sogar die mikrobiellen Gemeinschaften im Kot variieren, was eine neue Erkenntnis darstellt. Diese komplexe Umstrukturierung und Neuzusammensetzung von Gemeinschaften in Kombination mit der nichtlinearen Spezialisierung von Interaktionen und einer hohen Vielfalt an assoziierten Bakterien unterstreichen unser noch immer begrenztes Verständnis davon, wie sich Ökosysteme unter zukünftigen Klimabedingungen entwickeln werden, und mahnen zur Vorsicht bei vereinfachten Vorhersagen über die Veränderung der biologischen Vielfalt im Zuge der Klimaerwärmung. Da solche Vorhersagen auf Grundlage unserer Ergebnisse vom Einbezug biotischer Wechselwirkungen und des Mikro- und Makroklimas profitieren können, dürfen Naturschutzverantwortliche eine Verbesserung der mikroklimatischen Bedingungen nicht vernachlässigen, um das lokale Überleben einer Vielzahl bedrohter und anspruchsvoller Arten zu sichern. In diesem Zusammenhang können Berge eine entscheidende Rolle für den Erhalt der biologischen Vielfalt spielen, da sie in räumlicher Nähe heterogene mikroklimatische Bedingungen bieten, die von Arten mit unterschiedlichen Nischen genutzt werden können. KW - Heuschrecken KW - Mikroklima KW - Bayerische Alpen KW - Nahrung KW - Mikrobiom KW - biotic interactions KW - plant-herbivore-interactions KW - elevational gradients Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-354608 ER - TY - THES A1 - Weisert, Nadine T1 - Characterization of telomere-associated proteins in \(Trypanosoma\) \(brucei\) T1 - Charakterisierung Telomer-assoziierter Proteine in \(Trypanosoma\) \(brucei\) N2 - The unicellular pathogen Trypanosoma brucei is the causative agent of African trypanosomiasis, an endemic disease prevalent in sub-Saharan Africa. Trypanosoma brucei alternates between a mammalian host and the tsetse fly vector. The extracellular parasite survives in the mammalian bloodstream by periodically exchanging their ˈvariant surface glycoproteinˈ (VSG) coat to evade the host immune response. This antigenic variation is achieved through monoallelic expression of one VSG variant from subtelomeric ˈbloodstream form expression sitesˈ (BES) at a given timepoint. During the differentiation from the bloodstream form (BSF) to the procyclic form (PCF) in the tsetse fly midgut, the stage specific surface protein is transcriptionally silenced and replaced by procyclins. Due to their subtelomeric localization on the chromosomes, VSG transcription and silencing is partly regulated by homologues of the mammalian telomere complex such as TbTRF, TbTIF2 and TbRAP1 as well as by ˈtelomere-associated proteinsˈ (TelAPs) like TelAP1. To gain more insights into transcription regulation of VSG genes, the identification and characterization of other TelAPs is critical and has not yet been achieved. In a previous study, two biochemical approaches were used to identify other novel TelAPs. By using ˈco-immunoprecipitationˈ (co-IP) to enrich possible interaction partners of TbTRF and by affinity chromatography using telomeric repeat oligonucleotides, a listing of TelAP candidates has been conducted. With this approach TelAP1 was identified as a novel component of the telomere complex, involved in the kinetics of transcriptional BES silencing during BSF to PCF differentiation. To gain further insights into the telomere complex composition, other previously enriched proteins were characterized through a screening process using RNA interference to deplete potential candidates. VSG expression profile changes and overall proteomic changes after depletion were analyzed by mass spectrometry. With this method, one can gain insights into the functions of the proteins and their involvement in VSG expression site regulation. To validate the interaction of proteins enriched by co-IP with TbTRF and TelAP1 and to identify novel interaction proteins, I performed reciprocal affinity purifications of the four most promising candidates (TelAP2, TelAP3, PPL2 and PolIE) and additionally confirmed colocalization of two candidates with TbTRF via immunofluorescence (TelAP2, TelAP3). TelAP3 colocalizes with TbTRF and potentially interacts with TbTRF, TbTIF2, TelAP1 and TelAP2, as well as with two translesion polymerases PPL2 and PolIE in BSF. PPL2 and PolIE seem to be in close contact to each other at the telomeric ends and fulfill different roles as only PolIE is involved in VSG regulation while PPL2 is not. TelAP2 was previously characterized to be associated with telomeres by partially colocalizing with TbTRF and cells show a VSG derepression phenotype when the protein was depleted. Here I show that TelAP2 interacts with the telomere-binding proteins TbTRF and TbTIF2 as well as with the telomere-associated protein TelAP1 in BSF and that TelAP2 depletion results in a loss of TelAP1 colocalization with TbTRF in BSF. In conclusion, this study demonstrates that characterizing potential TelAPs is effective in gaining insights into the telomeric complex's composition and its role in VSG regulation in Trypanosoma brucei. Understanding these interactions could potentially lead to new therapeutic targets for combatting African trypanosomiasis. N2 - Der einzellige Pathogen Trypanosoma brucei ist der Erreger der afrikanischen Trypanosomiasis, eine endemische Krankheit vertreten in der Sub-Sahara Zone Afrikas. Trypanosoma brucei wechselt zwischen einem Säugerwirt und dem Insektenvektor, der Tsetse-Fliege. Der im Blutstrom des Säugers vorkommende, extrazelluläre Parasit ändert seinen Oberflächenmantel bestehend aus dem ˈvariablen Oberflächenproteinˈ (VSG) in periodischen Abständen, um der Immunantwort des Wirtes auszuweichen. Diese antigenetische Variation wird durch die monoallelische Expression einer einzelnen VSG-Variante, lokalisiert auf den ˈBlutstromform Expressionsseitenˈ (BES), zu einem bestimmten Zeitpunkt erreicht. Diese stadienspezifischen Oberflächenproteine werden während der Differenzierung der ˈBlutstromformˈ (BSF) zur ˈprozyklischen Formˈ (PCF) im Mitteldarm der Tsetse-Fliege stillgelegt und durch Prozykline ersetzt. Wegen der subtelomeren Lokalisation wird die VSG Transkription und Stilllegung teilweise durch Homologe des Säuger Telomerkomplexes TbTRF, TbTIF2 und TbRAP1 als auch durch Telomer-assoziierte Proteine (TelAPs) wie TelAP1 reguliert. Um Einblicke in die Transkriptionsregulation der VSG Gene zu erhalten, ist die Identifikation und Charakterisierung anderer Telomer-assoziierter Proteine von großem Interesse. In einer vorherigen Studie wurden zwei komplementäre biochemische Versuchsansätze verwendet, um weitere neue TelAPs zu identifizieren. Es wurde eine ko-Immunpräzipitation (co-IP) durchgeführt, um mögliche Interaktionspartner von TbTRF zu identifizieren, sowie eine Affinitätschromatographie unter Verwendung telomerischen Wiederholungseinheiten. Hierdurch wurde eine Liste von potenziellen Kandidaten generiert. Mit diesem Ansatz wurde TelAP1 als neue Komponente des Telomerkomplexes identifiziert, welches an der Kinetik der transkriptionellen BES-Stilllegung während der Differenzierung von BSF zu PCF beteiligt ist. Um weitere Einblicke in die Zusammensetzung des Telomerkomplexes zu erhalten, wurden zuvor angereicherte Proteine durch einen Screening-Prozess unter Verwendung von RNA-Interferenz charakterisiert. Nach der Depletion von 21 Proteinen wurden massenspektrometrische Analysen der VSG Expressionsprofiländerungen sowie allgemeine Veränderungen des Proteomenprofils analysiert. Mit dieser Methode können Erkenntnisse über die Funktion der jeweiligen Proteine und ihrer Beteiligung an der Regulierung der antigenetischen Variation von T. brucei gewonnen werden. Um die Interaktionen von Proteinen zu validieren, welche bei den Co-Immunpräzipitationen mit TbTRF und TelAP1 angereichert wurden, habe ich eine reziproke Affinitätschromatographie mit vier der vielversprechendsten Kandidaten durchgeführt (TelAP2, TelAP3, PPL2 und PolIE). Zusätzlich bestätigte ich die Co-lokalisation von zwei Kandidaten mit TbTRF via Immunfluoreszenzaufnahmen (TelAP2, TelAP3). TelAP3 ko-lokalisiert mit TbTRF und TelAP1 und interagiert potenziell mit TbTRF, TbTIF2, TelAP1 und TelAP2 als auch mit den zwei Transläsionspolymerasen PPL2 und PolIE in BSF. PPL2 und PolIE stehen in engem Kontakt zueinander und nehmen an den Telomerenden unterschiedliche Funktionen ein, da nur PolIE an der VSG Regulation beteiligt ist. TelAP2 wurde in einer vorherigen Publikation als Telomer-assoziiertes Protein durch partielle Co-Lokalisation mit TbTRF identifiziert und Zellen zeigen nach der Depletion von TelAP2 eine Derepression von zuvor stillgelegten VSGs. In dieser Studie zeige ich, dass TelAP2 mit den Telomer-bindenden Proteinen TbTRF und TbTIF2 sowie mit dem telomerassoziierten Protein TelAP1 in BSF interagiert und dass die Depletion von TelAP2 zu dem Verlust der Co-Lokalisation von TelAP1 mit TbTRF in BSF führt. Zusammenfassend zeigt diese Studie, dass die Charakterisierung potenzieller TelAPs dazu beiträgt, Einblicke in die Zusammensetzung des Telomerkomplexes und dessen Rolle bei der VSG-Regulation in Trypanosoma brucei zu gewinnen. Das Verständnis dieser Interaktionen könnte möglicherweise zu neuen therapeutischen Ansatzpunkten zur Bekämpfung der afrikanischen Trypanosomiasis führen. KW - Telomer KW - Trypanosoma brucei KW - telomere-associated protein Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-352732 ER - TY - JOUR A1 - Franchini, Paolo A1 - Jones, Julia C. A1 - Xiong, Peiwen A1 - Kneitz, Susanne A1 - Gompert, Zachariah A1 - Warren, Wesley C. A1 - Walter, Ronald B. A1 - Meyer, Axel A1 - Schartl, Manfred T1 - Long-term experimental hybridisation results in the evolution of a new sex chromosome in swordtail fish JF - Nature Communications N2 - The remarkable diversity of sex determination mechanisms known in fish may be fuelled by exceptionally high rates of sex chromosome turnovers or transitions. However, the evolutionary causes and genomic mechanisms underlying this variation and instability are yet to be understood. Here we report on an over 30-year evolutionary experiment in which we tested the genomic consequences of hybridisation and selection between two Xiphophorus fish species with different sex chromosome systems. We find that introgression and imposing selection for pigmentation phenotypes results in the retention of an unexpectedly large maternally derived genomic region. During the hybridisation process, the sex-determining region of the X chromosome from one parental species was translocated to an autosome in the hybrids leading to the evolution of a new sex chromosome. Our results highlight the complexity of factors contributing to patterns observed in hybrid genomes, and we experimentally demonstrate that hybridisation can catalyze rapid evolution of a new sex chromosome. KW - evolutionary genetics KW - experimental evolution KW - genome evolution Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-228396 VL - 9 ER - TY - THES A1 - Kuklovsky [former Finke], Valerie T1 - Are some bees smarter than others? An examination of consistent individual differences in the cognitive abilities of honey bees T1 - Sind manche Bienen schlauer als andere? Eine Untersuchung von konsistenten individuellen Unterschieden in den kognitiven Fähigkeiten von Honigbienen N2 - Cognition refers to the ability to of animals to acquire, process, store and use vital information from the environment. Cognitive processes are necessary to predict the future and reduce the uncertainty of the ever-changing environment. Classically, research on animal cognition focuses on decisive cognitive tests to determine the capacity of a species by the testing the ability of a few individuals. This approach views variability between these tested key individuals as unwanted noise and is thus often neglected. However, inter-individual variability provides important insights to behavioral plasticity, cognitive specialization and brain modularity. Honey bees Apis mellifera are a robust and traditional model for the study of learning, memory and cognition due to their impressive capabilities and rich behavioral repertoire. In this thesis I have applied a novel view on the learning abilities of honey bees by looking explicitly at individual differences in a variety of learning tasks. Are some individual bees consistently smarter than some of her sisters? If so, will a smart individual always perform good independent of the time, the context and the cognitive requirements or do bees show distinct isolated ‘cognitive modules’? My thesis presents the first comprehensive investigation of consistent individual differences in the cognitive abilities of honey bees. To speak of an individual as behaving consistently, a crucial step is to test the individual multiple times to examine the repeatability of a behavior. I show that free-flying bees remain consistent in a visual discrimination task for three consecutive days. Successively, I explored individual consistency in cognitive proficiency across tasks involving different sensory modalities, contexts and cognitive requirements. I found that free-flying bees show a cognitive specialization between visual and olfactory learning but remained consistent across a simple discrimination task and a complex concept learning task. I wished to further explore individual consistency with respect to tasks of different cognitive complexity, a question that has never been tackled before in an insect. I thus performed a series of four experiments using either visual or olfactory stimuli and a different training context (free-flying and restrained) and tested bees in a discrimination task, reversal learning and negative patterning. Intriguingly, across all these experiments I evidenced the same results: The bees’ performances were consistent across the discrimination task and reversal learning and negative patterning respectively. No association was evidenced between reversal learning and negative patterning. After establishing the existence of consistent individual differences in the cognitive proficiency of honey bees I wished to determine factors which could underlie these differences. Since genetic components are known to underlie inter-individual variability in learning abilities, I studied the effects of genetics on consistency in cognitive proficiency by contrasting bees originating from either from a hive with a single patriline (low genetic diversity) or with multiple patrilines (high genetic diversity). These two groups of bees showed differences in the patterns of individually correlated performances, indicating a genetic component accounts for consistent cognitive individuality. Another major factor underlying variability in learning performances is the individual responsiveness to sucrose solution and to visual stimuli, as evidenced by many studies on restrained bees showing a positive correlation between responsiveness to task relevant stimuli and learning performances. I thus tested whether these relationships between sucrose/visual responsiveness and learning performances are applicable for free-flying bees. Free-flying bees were again subjected to reversal learning and negative patterning and subsequently tested in the laboratory for their responsiveness to sucrose and to light. There was no evidence of a positive relationship between sucrose/visual responsiveness and neither performances of free-flying bees in an elemental discrimination, reversal learning and negative patterning. These findings indicate that relationships established between responsiveness to task relevant stimuli and learning proficiency established in the laboratory with restrained bees might not hold true for a completely different behavioral context i.e. for free-flying bees in their natural environment. These results show that the honey bee is an excellent insect model to study consistency in cognitive proficiency and to identify the underlying factors. I mainly discuss the results with respect to the question of brain modularity in insects and the adaptive significance of individuality in cognitive abilities for honey bee colonies. I also provide a proposition of research questions which tie in this theme of consistent cognitive proficiency and could provide fruitful areas for future research. N2 - Unter Kognition versteht man die Fähigkeit von Tieren, essenzielle Informationen aus der Umwelt zu erfassen, zu verarbeiten, zu speichern und zu nutzen. Kognitive Prozesse sind notwendig, um die Zukunft vorherzusagen und die Unvorhersehbarkeit der sich ständig verändernden Umwelt zu verringern. Die Forschung der Kognition von Tieren konzentriert sich klassischerweise auf entscheidende kognitive Tests, um die Fähigkeit einer Spezies anhand der Leistungen einiger weniger Individuen zu bestimmen. Bei diesem Ansatz wird die Variabilität zwischen Individuen als unerwünschtes Rauschen betrachtet und daher vernachlässigt. Die interindividuelle Variabilität liefert jedoch wichtige Erkenntnisse über die Plastizität des Verhaltens, die kognitive Spezialisierung und die Modularität des Gehirns. Die Honigbiene Apis mellifera ist aufgrund ihrer eindrucksvollen Fähigkeiten und ihres reichen Verhaltensrepertoires ein robuster und traditioneller Modellorganismus für die Untersuchung von Lernen, Gedächtnis und Kognition. In dieser Arbeit habe ich das Lernverhalten von Honigbienen in einem neuen Blickwinkel betrachtet, indem ich explizit die individuellen Unterschiede bei diversen Lernaufgaben untersucht habe. Zeigen manche Bienen durchweg eine erhöhte Lernleistung im Vergleich zu ihren Schwestern? Wenn ja, erbringt ein Individuum unabhängig von der Zeit, dem Kontext und den kognitiven Anforderungen der Lernaufgaben immer gute Leistungen, oder zeigen Bienen ausgeprägte unabhängige "kognitive Module"? Die vorliegende Doktorarbeit stellt die erste umfassende Untersuchung konsistenter individueller Unterschiede in den kognitiven Fähigkeiten von Honigbienen dar. Um von einem konsistenten Verhalten sprechen zu können, ist es entscheidend das Individuum mehrfach zu testen, um die Wiederholbarkeit eines Verhaltens zu untersuchen. Ich konnte zeigen, dass frei fliegende Bienen bei einer visuellen Unterscheidungsaufgabe an drei aufeinanderfolgenden Tagen eine konsistente Lernleistung zeigen. Im Anschluss untersuchte ich die individuelle Konsistenz der kognitiven Fähigkeiten bei Lernaufgaben mit unterschiedlichen sensorischen Modalitäten, Kontexten und kognitiven Anforderungen. Frei fliegende Bienen zeigten eine kognitive Spezialisierung zwischen visuellem und olfaktorischem Lernen, während sie bei einer einfachen Unterscheidungsaufgabe und einer komplexen Konzeptlernaufgabe konsistent im Lernverhalten blieben. Anschließend wollte ich die individuelle Konsistenz im Lernverhalten bei Aufgaben unterschiedlicher kognitiver Komplexität weiter erforschen, eine Frage, die bisher noch nie bei einem Insekt behandelt wurde. Ich führte dazu eine Reihe von vier Experimenten durch, bei denen entweder visuelle oder olfaktorische Stimuli und ein unterschiedlicher Trainingskontext (frei fliegend oder eingespannt) verwendet wurden. Die Bienen wurden in einer Unterscheidungsaufgabe, einer Umlernaufgabe und in Negative Patterning getestet. Erstaunlicherweise wurden bei diesen Experimenten die gleichen Ergebnisse festgestellt: Die Lernleitung der Bienen in der Unterscheidungsaufgabe zeigte eine positive Korrelation mit der Lernleistung im Umlernen und Negative Patterning. Zwischen dem Umkehrlernen und Negative Patterning konnte jedoch kein Zusammenhang festgestellt werden. Nachdem ich festgestellt hatte, dass es konsistente individuelle Unterschiede in den kognitiven Fähigkeiten von Bienen gibt, wollte ich die Faktoren ermitteln, die diesen Unterschieden zugrunde liegen könnten. Es war bereits bekannt, dass genetische Komponenten der interindividuellen Variabilität im Lernverhalten zugrunde liegen. Deshalb untersuchte ich den Einfluss von genetischer Vielfalt auf die Beständigkeit von kognitiven Fähigkeiten, indem ich Bienen gegenüberstellte, die entweder aus einem Bienenstock mit einer einzigen Patriline (geringe genetische Vielfalt) oder mit mehreren Patrilinen (hohe genetische Vielfalt) stammten. Diese beiden Gruppen von Bienen wiesen Unterschiede in den Mustern der individuellen korrelierten Lernleistungen auf, was darauf hindeutet, dass eine genetische Komponente für kognitive Individualität verantwortlich ist. Ein weiterer wichtiger Faktor, welcher der Variabilität im Lernverhalten zugrunde liegt, ist die individuelle Reaktionsfähigkeit auf Saccharose Lösungen und auf visuelle Stimuli. Dies wurde durch viele Studien an eingespannten Bienen gezeigt, die eine positive Korrelation zwischen der Reaktionsfähigkeit auf aufgabenrelevante Reize und den Lernfähigkeiten feststellten. Ich habe daher untersucht, ob diese Beziehungen zwischen der Reaktionsfähigkeit auf Saccharose und visuellen Stimuli und den Lernleistungen auch für frei fliegende Bienen zutreffen. Die individuellen Lernleistungen im Umlernen und Negative patterning von frei fliegenden Bienen wurden erneut ermittelt und anschließend wurde im Labor die Reaktionsfähigkeit auf Saccharose und Licht getestet. Es gab keine Hinweise auf eine positive Korrelation zwischen der Reaktionsfähigkeit auf Saccharose und Licht und den Lernleistungen von frei fliegenden Bienen. Diese Ergebnisse deuten darauf hin, dass Beziehungen zwischen der Reaktionsfähigkeit auf aufgabenrelevante Stimuli und der Lernleistung, die im Labor mit eingespannten Bienen festgestellt wurden, möglicherweise nicht für einen anderen Verhaltenskontext gelten, d. h. für frei fliegende Bienen in ihrer natürlichen Umgebung. Diese Ergebnisse zeigen, dass die Honigbiene ein hervorragendes Insektenmodell ist, um die Konsistenz kognitiver Fähigkeiten zu untersuchen und die zugrunde liegenden Faktoren zu ermitteln. Ich diskutiere die Ergebnisse vor allem im Hinblick auf die Frage der Modularität des Gehirns bei Insekten und die adaptive Bedeutung von individuellen konsistenten kognitiven Fähigkeiten für Honigbienenvölker. Ich schlage auch Forschungsfragen vor, die mit individuellen konsistenten kognitiven Fähigkeiten zusammenhängen und wertvolle Bereiche für künftige Forschungen darstellen könnten. KW - Lernen KW - Biene KW - Kognition KW - Individual differences KW - Cognitive consistency KW - Cognitive profile KW - Learning KW - Honeybee KW - Cognition Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-323012 ER - TY - THES A1 - Hahn, Sarah T1 - Investigating non-canonical, 5' UTR-dependent translation of MYC and its impact on colorectal cancer development T1 - Untersuchung der nicht-kanonischen, 5' UTR-abhängigen Translation von MYC und ihres Einflusses auf die Entwicklung von Darmkrebs N2 - Colorectal cancer (CRC) is the second most common tumour disease in Germany, with the sequential accumulation of certain mutations playing a decisive role in the transition from adenoma to carcinoma. In particular, deregulation of the Wnt signalling pathway and the associated deregulated expression of the MYC oncoprotein play a crucial role. Targeting MYC thus represents an important therapeutic approach in the treatment of tumours. Since direct inhibition of MYC is challenging, various approaches have been pursued to date to target MYC indirectly. The MYC 5' UTR contains an internal ribosomal entry site (IRES), which has a particular role in the initiation of MYC translation, especially in multiple myeloma. As basis for this work, it was hypothesised on the basis of previous data that translation of MYC potentially occurs via its IRES in CRC as well. Based on this, two IRES inhibitors were tested for their potential to regulate MYC expression in CRC cells. In addition, alternative, 5’ UTR-dependent translation of MYC and interacting factors were investigated. EIF3D was identified as a MYC 5' UTR binding protein which has the potential to regulate MYC expression in CRC. The results of this work suggest that there is a link between eIF3D and MYC expression/translation, rendering eIF3D a potential therapeutic target for MYC-driven CRCs. N2 - Das kolorektale Karzinom (KRK) ist die zweithäufigste Tumorerkrankung in Deutschland, wobei die sequenzielle Akkumulation bestimmter Mutationen eine entscheidende Rolle beim Übergang vom Adenom zum Karzinom spielt. Insbesondere die Deregulation des Wnt-Signalweges und die damit verbundene deregulierte Expression des MYC-Onkoproteins spielen eine entscheidende Rolle. MYC ist ein zentraler Vermittler von Zellfunktionen und reguliert als Transkriptionsfaktor die Expression fast aller Gene sowie verschiedener RNA-Spezies. Selbst kleine Veränderungen der zellulären MYC-Konzentration können das Proliferationsverhalten beeinflussen und die Entstehung und das Fortschreiten von Tumoren fördern. Die gezielte Beeinflussung von MYC stellt daher einen wichtigen therapeutischen Ansatz für die Behandlung von Tumoren dar. Da eine direkte Hemmung von MYC aufgrund seiner Struktur herausfordernd ist, wurden bisher verschiedene Ansätze verfolgt, um MYC indirekt zu beeinflussen, etwa über seinen Interaktionspartner MAX oder auf Ebene der Stabilität, Transkription oder Translation. In unserer eigenen Forschungsgruppe lag der Schwerpunkt in den letzten Jahren speziell auf der Translation von MYC im KRK. Es konnte gezeigt werden, dass die Hemmung der kanonischen cap-abhängigen Translation nicht wie erwartet zu einer Verringerung der zellulären MYC-Level führt, was auf einen alternativen Mechanismus der MYC-Translation hindeutet, der unabhängig vom eIF4F-Komplex abläuft. Die 5'-UTR von MYC enthält eine interne ribosomale Eintrittsstelle (IRES), die eine besondere Rolle bei der Initiierung der MYC-Translation spielt, insbesondere im Multiplen Myelom. Als Grundlage für diese Arbeit wurde daher die Hypothese aufgestellt, dass die Translation von MYC im KRK möglicherweise ebenfalls über die IRES erfolgt. Auf dieser Grundlage wurden zunächst zwei publizierte IRES-Inhibitoren auf ihr Potenzial zur Regulierung der MYC-Expression in KRK-Zellen getestet. J007-IRES hatte keine Auswirkungen auf die MYC-Proteinmenge, und Cymarin scheint weitaus globalere Auswirkungen zu haben, die nicht ausschließlich auf die Verringerung der MYC-Proteinmenge zurückzuführen sind. Daher wurde weiter untersucht, inwieweit die alternative Translation von MYC generell von der 5'-UTR und damit interagierenden Faktoren abhängig ist. EIF3D wurde als MYC-5'-UTR-Bindungsprotein identifiziert, dessen Knockdown zu reduzierten MYC-Leveln, einem Proliferationsdefizit sowie einer Verringerung der globalen Proteinsynthese in KRK-Zellen führte. Darüber hinaus führte die Depletion von EIF3D zu ähnlichen Veränderungen im zellulären Genexpressionsmuster wie die Depletion von MYC, wobei viele tumorassoziierte Signalwege betroffen waren. Mittels eCLIP-seq wurde die Bindung von eIF3D an die MYC mRNA nachgewiesen, der genaue Mechanismus einer möglicherweise durch eIF3D vermittelten Translation von MYC muss jedoch weiter untersucht werden. Die Ergebnisse dieser Arbeit deuten darauf hin, dass eine Verbindung zwischen eIF3D und der MYC-Expression/Translation besteht, wodurch eIF3D zu einem potenziellen therapeutischen Ziel für MYC-getriebene KRKs wird. KW - Myc KW - Translation KW - Colorectal cancer KW - 5' UTR Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-364202 ER - TY - THES A1 - Hartmann, Oliver T1 - Development of somatic modified mouse models of Non-Small cell lung cancer T1 - Entwicklung von somatisch veränderten Mausmodellen für nichtkleinzelligen Lungenkrebs N2 - In 2020, cancer was the leading cause of death worldwide, accounting for nearly 10 million deaths. Lung cancer was the most common cancer, with 2.21 million cases per year in both sexes. This non-homogeneous disease is further subdivided into small cell lung cancer (SCLC, 15%) and non-small cell lung cancer (NSCLC, 85%). By 2023, the American Cancer Society estimates that NSCLC will account for 13% of all new cancer cases and 21% of all estimated cancer deaths. In recent years, the treatment of patients with NSCLC has improved with the development of new therapeutic interventions and the advent of targeted and personalised therapies. However, these advances have only marginally improved the five-year survival rate, which remains alarmingly low for patients with NSCLC. This observation highlights the importance of having more appropriate experimental and preclinical models to recapitulate, identify and test novel susceptibilities in NSCLC. In recent years, the Trp53fl/fl KRaslsl-G12D/wt mouse model developed by Tuveson, Jacks and Berns has been the main in vivo model used to study NSCLC. This model mimics ADC and SCC to a certain extent. However, it is limited in its ability to reflect the genetic complexity of NSCLC. In this work, we use CRISPR/Cas9 genome editing with targeted mutagenesis and gene deletions to recapitulate the conditional model. By comparing the Trp53fl/fl KRaslsl- G12D/wt with the CRISPR-mediated Trp53mut KRasG12D, we demonstrated that both showed no differences in histopathological features, morphology, and marker expression. Furthermore, next-generation sequencing revealed a very high similarity in their transcriptional profile. Adeno-associated virus-mediated tumour induction and the modular design of the viral vector allow us to introduce additional mutations in a timely manner. CRISPR-mediated mutation of commonly mutated tumour suppressors in NSCLC reliably recapitulated the phenotypes described in patients in the animal model. Lastly, the dual viral approach could induce the formation of lung tumours not only in constitutive Cas9 expressing animals, but also in wildtype animals. Thus, the implementation of CRISPR genome editing can rapidly advance the repertoire of in vivo models for NSCLC research. Furthermore, it can reduce the necessity of extensive breeding. N2 - Krebs war mit fast 10 Millionen Todesfällen weltweit die häufigste Todesursache in 2020. Mit 2,21 Millionen Fällen pro Jahr in beiden Geschlechtern kombiniert war Lungenkrebs die häufigste Unterart. Auszeichnend für dieses Krankheit ist die hohe Komplexität und Heterogenität. Daher wird diese weiter in kleinzelligen Lungenkrebs (SCLC, 15 %) und nicht-kleinzelligen Lungenkrebs (NSCLC, 85 %) unterteilt. Die American Cancer Society schätzt, dass bis 2023 13 % aller neuen Krebsfälle und 21 % aller geschätzten Krebstodesfälle auf das nicht-kleinzellige Lungenkarzinom entfallen werden. In den letzten Jahren hat sich die Behandlung von Patienten mit nicht-kleinzelligem Lungenkarzinom durch die Entwicklung neuer therapeutischer Maßnahmen und das Anwenden personalisierter Therapien verbessert. Allerdings haben diese Fortschritte die Fünfjahresüberlebensrate nur geringfügig verbessert, die für Patienten mit NSCLC nach wie vor alarmierend niedrig ist. Diese macht deutlich, wie wichtig es ist, über geeignetere experimentelle und präklinische Modelle zu verfügen, um neue Therapieansätze beim NSCLC zu rekapitulieren, zu identifizieren und zu testen. In der letzten Dekade war das von Tuveson, Jacks und Berns entwickelte Trp53fl/fl KRaslsl-G12D/wt-Mausmodell das wichtigste In-vivo-Modell zur Untersuchung von NSCLC. Dieses kann grundlegend das Krankheitsbild von NSCLC wiederspiegeln. Es ist jedoch nur begrenzt in der Lage, die genetische Komplexität von NSCLC im vollen Umfang zu refelktieren. In dieser Arbeit verwenden wir CRISPR/Cas9 Genome Editing mit gezielter Mutagenese und Gendeletionen, um das konditionale Modell zu rekapitulieren. Durch den Vergleich des Trp53fl/fl KRaslsl-G12D/wt mit dem CRISPR-vermittelten Trp53mut KRasG12D konnten wir zeigen, dass beide keine Unterschiede in Bezug auf histopathologische Merkmale, Morphologie und Markerexpression aufweisen. Darüber hinaus ergab die Analyse mittels Next Generation Sequencing 8Hochdruchsatz.Sequenzierung) eine sehr große Ähnlichkeit in ihrem Transkriptionsprofil. Die Adeno-assoziierte Virus-vermittelte Tumorinduktion und der modulare Aufbau des viralen Vektors ermöglichen es uns, zusätzliche Mutationen zeitnah einzuführen. Die CRISPR-vermittelte Mutation von häufig mutierten Tumorsuppressoren bei NSCLC rekapitulierte zuverlässig die bei Patienten beschriebenen Phänotypen im Tiermodell. Schließlich konnte der duale virale Ansatz die Bildung von Lungentumoren nicht nur in konstitutiv Cas9 exprimierenden Tieren, sondern auch in Wildtyp-Tieren induzieren. Somit kann die Anwendung von CRISPR-Genome Editing das Repertoire an In-vivo- Modellen für die NSCLC-Forschung rasch erweitern. Darüber hinaus kann es die Notwendigkeit umfangreicher Züchtungen verringern. KW - CRISPR/Cas-Methode KW - in vivo KW - Lung Cancer KW - CRISPR/Cas9 KW - in vivo genome editing KW - Immunohistochemistry KW - Nicht-kleinzelliges Bronchialkarzinom KW - NSCLC KW - Mouse Model KW - CRISPR Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-363401 ER - TY - THES A1 - Heimberger, Kevin T1 - Regulation pathways of c-MYC under glutamine-starving conditions in colon carcinoma cells T1 - Regulierungsmechanismen von c-MYC in Darmkrebszellen unter Glutaminmangelbedingungen N2 - Colon carcinomas (CRC) are statistically among the most fatal cancer types and hence one of the top reasons for premature mortality in the developed world. CRC cells are characterized by high proliferation rates caused by deregulation of gene transcription of proto-oncogenes and general chromosomal instability. On macroscopic level, CRC cells show a strongly altered nutrient and energy metabolism. This work presents research to understand general links between the metabolism and transcription alteration. Mainly focussing on glutamine dependency, shown in colon carcinoma cells and expression pathways of the pro-proliferation protein c-MYC. Previous studies showed that a depletion of glutamine in the cultivation medium of colon carcinoma cell lines caused a proliferation arrest and a strong decrease of overall c-MYC levels. Re-addition of glutamine quickly replenished c-MYC levels through an unknown mechanism. Several proteins altering this regulation mechanism were identified and proposed as possible starting point for further in detail studies to unveil the precise biochemical pathway controlling c-MYC translation repression and reactivation in a rapid manner. On a transcriptional level the formation of RNA:DNA hybrids, so called R-loops, was observed under glutamine depleted conditions. The introduction and overexpression of RNaseH1, a R-loop degrading enzyme, in combination with an ectopically expressed c-MYC variant, independent of cellular regulation mechanisms by deleting the regulatory 3’-UTR of the c-MYC gene, lead to a high rate of apoptotic cells in culture. Expression of a functionally inactive variant of RNaseH1 abolished this effect. This indicates a regulatory function of R-loops formed during glutamine starvation in the presence of c-MYC protein in a cell. Degradation of R-loops and high c-MYC levels in this stress condition had no imminent effect on the cell cycle progression is CRC cells but disturbed the nucleotide metabolism. Nucleotide triphosphates were strongly reduced in comparison to starving cells without R-loop degradation and proliferating cells. This study proposes a model of a terminal cycle of transcription termination, unregulated initiation and elongation of transcription leading to a depletion of energy resources of cells. This could finally lead to high apoptosis of the cells. Sequencing experiments to determine a coinciding of termination sites and R-loop formation sides failed so far but show a starting point for further studies in this essential survival mechanism involving R-loop formation and c-MYC downregulation. N2 - Darmkrebs gehört statistisch zu den Krebsarten mit den höchsten Sterblichkeitsraten und zählen somit zu den häufigsten Todesursachen der entwickelten Länder. Darmkrebszellen zeichnen sich durch chromosomale Instabilität und hohe Proliferationsraten aus, die durch eine Deregulierung der Expression verschiedener Proto-Onkogene zustande kommen. Generell besitzen diese Krebszellen einen stark veränderten Nährstoff- und Energiestoffwechsel im Vergleich zu gesunden somatischen Zellen. Diese Arbeit strebt ein besseres Verständnis der Verbindung zwischen dem Metabolismus und der Gen-Expression an. Das Hauptaugenmerk liegt hierbei auf dem Mechanismus der Expression des proliferationsfördernden Proteins c-MYC und der Abhängigkeit von Glutamin, die Darmkrebszellen charakterisiert. Frühere Studien haben gezeigt, dass der Entzug von Glutamin aus dem Kulturmedium von Darmkrebszelllinien eine Arretierung des Zellzyklus bewirkt sowie die Konzentration des Proteins c-MYC reduziert. Erneute Zugabe von Glutamin zum Medium stellt die MYC-Konzentration schnell wieder her. Die Hintergründe dieses Mechanismus sind bislang aber kaum verstanden. Einige Proteine wurden hier als potenzielle Kandidaten identifiziert, die einen Einfluss auf den biochemischen Prozess haben könnten, der die schnelle Wiederaufnahme der c-MYC Translation gewährleistet. Auf Translationsebene wurden RNA:DNA-Hybriden, sogenannte R-loops, gefunden, die sich unter anderem unter Glutamin-Mangelbedingungen im Genom bilden können. Ein gezielter Abbau dieser R-loops mithilfe des Enzyms RNaseH1, in Kombination mit der ektopischen Expression einer c-MYC-Variante, die unempfindlich gegenüber der zelleigenen Regulationsmechanismen ist, führte zu einer erhöhten Anzahl an apoptotischen Zellen in Kultur. Exprimiert man eine funktionell inaktive Variante der RNaseH1, statt der funktionellen, so kann dieser Apoptose-fördernde Prozess nicht beobachtet werden. Dies bestärkt die Hypothese, dass die R-loops, die sich während eines Glutamin-Mangels und hoher c-MYC-Konzentration bilden, eine regulatorische Funktion innehaben. Als Ursache für die Apoptose konnte ein Effekt der veränderten Expression auf das Fortschreiten des Zellzyklus ausgeschlossen werden. Jedoch zeigte sich eine Veränderung im Nukleotid-Metabolismus. Betroffene Zellen zeigten deutlich reduzierte Nuklotidtriphosphat-Konzentrationen im Vergleich zu Zellen unter Glutaminmangelbedingungen ohne R-loop-Abbau. In dieser Arbeit wurde ein Modell entwickelt, das einen sich selbst negativ verstärkenden Zyklus vorschlägt, der die Zellen zur Apoptose führt. Transkriptionstermination und eine unkontrollierte Initiation der Transkription im Wechsel führt zu einem Verbrauch der lebensnotwendigen Energieressourcen der Zellen. Sequenzierungsexperimente zur Lokalisierung der R-loops und Terminationsstellen sind bislang fehlgeschlagen, bieten jedoch Ansätze für künftige Forschung. KW - Myc KW - cMYC regulation KW - Colorectal Cancer KW - Glutamine KW - Translation regulation Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-363316 ER - TY - JOUR A1 - Hennrich, Marco L. A1 - Romanov, Natalie A1 - Horn, Patrick A1 - Jaeger, Samira A1 - Eckstein, Volker A1 - Steeples, Violetta A1 - Ye, Fei A1 - Ding, Ximing A1 - Poisa-Beiro, Laura A1 - Mang, Ching Lai A1 - Lang, Benjamin A1 - Boultwood, Jacqueline A1 - Luft, Thomas A1 - Zaugg, Judith B. A1 - Pellagatti, Andrea A1 - Bork, Peer A1 - Aloy, Patrick A1 - Gavin, Anne-Claude A1 - Ho, Anthony D. T1 - Cell-specific proteome analyses of human bone marrow reveal molecular features of age-dependent functional decline JF - Nature Communications N2 - Diminishing potential to replace damaged tissues is a hallmark for ageing of somatic stem cells, but the mechanisms remain elusive. Here, we present proteome-wide atlases of age-associated alterations in human haematopoietic stem and progenitor cells (HPCs) and five other cell populations that constitute the bone marrow niche. For each, the abundance of a large fraction of the ~12,000 proteins identified is assessed in 59 human subjects from different ages. As the HPCs become older, pathways in central carbon metabolism exhibit features reminiscent of the Warburg effect, where glycolytic intermediates are rerouted towards anabolism. Simultaneously, altered abundance of early regulators of HPC differentiation reveals a reduced functionality and a bias towards myeloid differentiation. Ageing causes alterations in the bone marrow niche too, and diminishes the functionality of the pathways involved in HPC homing. The data represent a valuable resource for further analyses, and for validation of knowledge gained from animal models. KW - ageing KW - haematopoietic stem cells KW - mesenchymal stem cells Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-319877 VL - 9 ER - TY - JOUR A1 - Hines, Rochelle M. A1 - Maric, Hans Michael A1 - Hines, Dustin J. A1 - Modgil, Amit A1 - Panzanelli, Patrizia A1 - Nakamura, Yasuko A1 - Nathanson, Anna J. A1 - Cross, Alan A1 - Deeb, Tarek A1 - Brandon, Nicholas J. A1 - Davies, Paul A1 - Fritschy, Jean-Marc A1 - Schindelin, Hermann A1 - Moss, Stephen J. T1 - Developmental seizures and mortality result from reducing GABAA receptor α2-subunit interaction with collybistin JF - Nature Communications N2 - Fast inhibitory synaptic transmission is mediated by γ-aminobutyric acid type A receptors (GABAARs) that are enriched at functionally diverse synapses via mechanisms that remain unclear. Using isothermal titration calorimetry and complementary methods we demonstrate an exclusive low micromolar binding of collybistin to the α2-subunit of GABAARs. To explore the biological relevance of collybistin-α2-subunit selectivity, we generate mice with a mutation in the α2-subunit-collybistin binding region (Gabra2-1). The mutation results in loss of a distinct subset of inhibitory synapses and decreased amplitude of inhibitory synaptic currents. Gabra2–1 mice have a striking phenotype characterized by increased susceptibility to seizures and early mortality. Surviving Gabra2-1 mice show anxiety and elevations in electroencephalogram δ power, which are ameliorated by treatment with the α2/α3-selective positive modulator, AZD7325. Taken together, our results demonstrate an α2-subunit selective binding of collybistin, which plays a key role in patterned brain activity, particularly during development. KW - cellular neuroscience KW - ion channels in the nervous system KW - neurotransmitters KW - synaptic development Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-320719 VL - 9 ER - TY - JOUR A1 - Gröbner, Susanne N. A1 - Worst, Barbara C. A1 - Weischenfeldt, Joachim A1 - Buchhalter, Ivo A1 - Kleinheinz, Kortine A1 - Rudneva, Vasilisa A. A1 - Johann, Pascal D. A1 - Balasubramanian, Gnana Prakash A1 - Segura-Wang, Maia A1 - Brabetz, Sebastian A1 - Bender, Sebastian A1 - Hutter, Barbara A1 - Sturm, Dominik A1 - Pfaff, Elke A1 - Hübschmann, Daniel A1 - Zipprich, Gideon A1 - Heinold, Michael A1 - Eils, Jürgen A1 - Lawerenz, Christian A1 - Erkek, Serap A1 - Lambo, Sander A1 - Waszak, Sebastian A1 - Blattmann, Claudia A1 - Borkhardt, Arndt A1 - Kuhlen, Michaela A1 - Eggert, Angelika A1 - Fulda, Simone A1 - Gessler, Manfred A1 - Wegert, Jenny A1 - Kappler, Roland A1 - Baumhoer, Daniel A1 - Stefan, Burdach A1 - Kirschner-Schwabe, Renate A1 - Kontny, Udo A1 - Kulozik, Andreas E. A1 - Lohmann, Dietmar A1 - Hettmer, Simone A1 - Eckert, Cornelia A1 - Bielack, Stefan A1 - Nathrath, Michaela A1 - Niemeyer, Charlotte A1 - Richter, Günther H. A1 - Schulte, Johannes A1 - Siebert, Reiner A1 - Westermann, Frank A1 - Molenaar, Jan J. A1 - Vassal, Gilles A1 - Witt, Hendrik A1 - Burkhardt, Birgit A1 - Kratz, Christian P. A1 - Witt, Olaf A1 - van Tilburg, Cornelis M. A1 - Kramm, Christof M. A1 - Fleischhack, Gudrun A1 - Dirksen, Uta A1 - Rutkowski, Stefan A1 - Frühwald, Michael A1 - Hoff, Katja von A1 - Wolf, Stephan A1 - Klingebeil, Thomas A1 - Koscielniak, Ewa A1 - Landgraf, Pablo A1 - Koster, Jan A1 - Resnick, Adam C. A1 - Zhang, Jinghui A1 - Liu, Yanling A1 - Zhou, Xin A1 - Waanders, Angela J. A1 - Zwijnenburg, Danny A. A1 - Raman, Pichai A1 - Brors, Benedikt A1 - Weber, Ursula D. A1 - Northcott, Paul A. A1 - Pajtler, Kristian W. A1 - Kool, Marcel A1 - Piro, Rosario M. A1 - Korbel, Jan O. A1 - Schlesner, Matthias A1 - Eils, Roland A1 - Jones, David T. W. A1 - Lichter, Peter A1 - Chavez, Lukas A1 - Zapatka, Marc A1 - Pfister, Stefan M. T1 - The landscape of genomic alterations across childhood cancers JF - Nature N2 - Pan-cancer analyses that examine commonalities and differences among various cancer types have emerged as a powerful way to obtain novel insights into cancer biology. Here we present a comprehensive analysis of genetic alterations in a pan-cancer cohort including 961 tumours from children, adolescents, and young adults, comprising 24 distinct molecular types of cancer. Using a standardized workflow, we identified marked differences in terms of mutation frequency and significantly mutated genes in comparison to previously analysed adult cancers. Genetic alterations in 149 putative cancer driver genes separate the tumours into two classes: small mutation and structural/copy-number variant (correlating with germline variants). Structural variants, hyperdiploidy, and chromothripsis are linked to TP53 mutation status and mutational signatures. Our data suggest that 7–8% of the children in this cohort carry an unambiguous predisposing germline variant and that nearly 50% of paediatric neoplasms harbour a potentially druggable event, which is highly relevant for the design of future clinical trials. KW - cancer genomics KW - oncogenesis KW - paediatric cancer KW - predictive markers KW - translational research Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-229579 VL - 555 ER - TY - JOUR A1 - Letunic, Ivica A1 - Khedkar, Supriya A1 - Bork, Peer T1 - SMART: recent updates, new developments and status in 2020 JF - Nucleic Acids Research N2 - SMART (Simple Modular Architecture Research Tool) is a web resource (https://smart.embl.de) for the identification and annotation of protein domains and the analysis of protein domain architectures. SMART version 9 contains manually curatedmodels formore than 1300 protein domains, with a topical set of 68 new models added since our last update article (1). All the new models are for diverse recombinase families and subfamilies and as a set they provide a comprehensive overview of mobile element recombinases namely transposase, integrase, relaxase, resolvase, cas1 casposase and Xer like cellular recombinase. Further updates include the synchronization of the underlying protein databases with UniProt (2), Ensembl (3) and STRING (4), greatly increasing the total number of annotated domains and other protein features available in architecture analysis mode. Furthermore, SMART's vector-based protein display engine has been extended and updated to use the latest web technologies and the domain architecture analysis components have been optimized to handle the increased number of protein features available. KW - SMART KW - SMART version 9 KW - protein domains KW - protein domain architectures Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-363816 VL - 49 IS - D1 ER - TY - THES A1 - Aroko, Erick Onyango T1 - Trans-regulation of \(Trypanosoma\) \(brucei\) variant surface glycoprotein (VSG) mRNA and structural analysis of a \(Trypanosoma\) \(vivax\) VSG using X-ray crystallography T1 - Trans-regulierung der mRNA des variablen Oberflächenglykoprotein (VSG) von \(Trypanosoma\) \(brucei\) und strukturelle Analyse eines \(Trypanosoma\) \(vivax\) VSG mittels Kristallstrukturanalyse N2 - African trypanosomes are unicellular parasites that cause nagana and sleeping sickness in livestock and man, respectively. The major pathogens for the animal disease include Trypanosoma vivax, T. congolense, and T. brucei brucei, whereas T. b. gambiense and T. b. rhodesiense are responsible for human infections. Given that the bloodstream form (BSF) of African trypanosomes is exclusively extracellular, its cell surface forms a critical boundary with the host environment. The cell surface of the BSF African trypanosomes is covered by a dense coat of immunogenic variant surface glycoproteins (VSGs). This surface protein acts as an impenetrable shield that protects the cells from host immune factors and is also involved in antibody clearance and antigenic variation, which collectively ensure that the parasite stays ahead of the host immune system. Gene expression in T. brucei is markedly different from other eukaryotes: most genes are transcribed as long polycistronic units, processed by trans-splicing a 39-nucleotide mini exon at the 5′ and polyadenylation at the 3′ ends of individual genes to generate the mature mRNA. Therefore, gene expression in T. brucei is regulated post-transcriptionally, mainly by the action of RNA binding proteins (RBPs) and conserved elements in the 3′ untranslated regions (UTR) of transcripts. The expression of VSGs is highly regulated, and only a single VSG gene is expressed at a time from one of the ~15 subtelomeric domains termed bloodstream expression sites (BES). When cells are engineered to simultaneously express two VSGs, the total VSG mRNA do not exceed the wild type amounts. This suggests that a robust VSG mRNA balancing mechanism exists in T. brucei. The present study uses inducible and constitutive expression of ectopic VSG genes to show that the endogenous VSG mRNA is regulated only if the second VSG is properly targeted to the ER. Additionally, the endogenous VSG mRNA response is triggered when high amounts of the GFP reporter with a VSG 3′UTR is targeted to the ER. Further evidence that non-VSG ER import signals can efficiently target VSGs to the ER is presented. This study suggests that a robust trans-regulation of the VSG mRNA is elicited at the ER through a feedback loop to keep the VSG transcripts in check and avoid overshooting the secretory pathway capacity. Further, it was shown that induction of expression of the T. vivax VSG ILDat1.2 in T. brucei causes a dual cell cycle arrest, with concomitant upregulation of the protein associated with differentiation (PAD1) expression. It could be shown that T. vivax VSG ILDat1.2 can only be sufficiently expressed in T. brucei after replacing its native GPI signal peptide with that of a T. brucei VSG. Taken together, these data indicate that inefficient VSG GPI anchoring and expression of low levels of the VSG protein can trigger differentiation from slender BSF to stumpy forms. However, a second T. vivax VSG, ILDat2.1, is not expressed in T. brucei even after similar modifications to its GPI signals. An X-ray crystallography approach was utilized to solve the N-terminal domain (NTD) structure of VSG ILDat1.2. This is first structure of a non-T. brucei VSG, and the first of a surface protein of T. vivax to be solved. VSG ILDat1.2 NTD maintains the three-helical bundle scaffold conserved in T. brucei surface proteins. However, it is likely that there are variations in the architecture of the membrane proximal region of the ILDat1.2 NTD and its CTD from T. brucei VSGs. The tractable T. brucei system is presented as a model that can be used to study surface proteins of related trypanosome species, thus creating avenues for further characterization of trypanosome surface coats. N2 - Afrikanische Trypanosomen sind einzellige Parasiten, die Nagana in Nutzvieh und die Schlafkrankheit im Menschen verursachen. Zu den Hauptverursachern der Tierkrankheit gehören Trypanosoma vivax, T. congolense und T. brucei brucei, während T. b. gambiense und T. b. rhodesiense für Infektionen im Menschen verantwortlich sind. Da die Blutstromform (BSF) der afrikanischen Trypanosomen rein extrazellulär vorkommt, bildet die Zelloberfläche eine kritische Grenzregion mit der Wirtsumgebung. Die Zelloberoberfläche der BSF afrikanischer Trypanosomen ist mit einem dichten Mantel an immunogenen variablen Oberflächenglykoproteinen (variant surface glycoprotein, VSG) umgeben. Dieses Oberflächenprotein dient als Barriere zum Schutz gegen Faktoren des Wirtsimmunsystems und spielt ebenfalls eine Rolle in Antikörper-Clearance und antigener Variation, welche gemeinsam dafür sorgen, dass der Parasit dem Wirtsimmunsystem stets einen Schritt voraus bleibt. Die Genexpression von T. brucei weist dezidierte Unterschiede im Vergleich zu anderen Eukaryoten auf: Die meisten Gene werden als lange polyzystronische Einheiten transkribiert, die durch trans-Splicing eines Miniexons aus 39 Nukleotiden am 5′ und Polyadenylierung am 3′ Ende der individuellen Gene prozessiert wird. Daher wird die Genexpression in T. brucei posttranskriptionell reguliert, zumeist durch RNA Bindeproteine (RBPs) und konservierte Elemente in der 3′ untranslatierten Region (UTR). Die Expression der VSGs ist stark reguliert, so wird zu einer gegebenen Zeit stets nur ein VSG Gen aus einer von ~15 Subtelomerregionen, die Blutstrom Expressionsorte (bloodstream expression sites, BES) genannt werden, exprimiert. Zellen, die gentechnisch manipuliert wurden um zwei VSGs zu exprimieren, produzieren die gleiche Menge an VSG mRNA wie Wildtyp Zellen. Dies deutet auf die Existenz eines robusten Mechanismus zur Regulierung der Gesamt-VSG mRNA Menge in T. brucei hin. Diese Arbeit verwendet induzierbare sowie konstitutive Expression eines ektopischen VSG Gens um zu zeigen, dass die endogene VSG mRNA nur reguliert wird, wenn das zweite VSG zum ER gelangt. Außerdem wird die endogene VSG mRNA Antwort auch ausgelöst, wenn hohe Mengen eines GFP Reporters, der eine VSG 3′UTR enthält, zum ER geleitet wird. Weiterhin, wird gezeigt, dass ER Importsignale anderer Proteine VSGs effizient zum ER dirigieren können. Das Ergebnis dieser Studie deutet darauf hin, dass eine Rückkopplungsschleife am ER eine robuste trans-Regulation der VSG mRNA auslöst, die die VSG Transkripte limitiert und somit eine Überlastung des sekretorischen Wegs verhindert. Weiterhin konnte gezeigt werden, dass es nach Induktion der Expression des T. vivax VSGs ILDat1.2 in T. brucei zu einem doppelten Zellzyklusarrest mit gleichzeitiger Hochregulation der Expression des protein associated with differentation (PAD1) kam und dass dieses T. vivax VSG nur nach Austausch des GPI Signalpeptids durch das eines T. brucei VSGs effizient exprimiert werden konnte. Zusammengenommen suggerieren diese Daten, dass eine ineffiziente GPI-Verankerung und wenig abundante Expression des VSGs die Differenzierung der sogenannten slender BSF zur sogenannten stumpy Form einleiten kann. Ein zweites T. vivax VSG, ILDat2.1, konnte hingegen auch nach Austausch des GPI Signals nicht in T. brucei exprimiert werden. Mit Hilfe der Röntgenstrukturanalyse wurde die Struktur der N-terminalen Domäne (NTD) des ILDat1.2 VSGs gelöst. Es handelt sich hierbei um die erste Proteinstruktur eines VSGs, welches nicht aus T. brucei stammt und die erste Struktur eines Oberflächenproteins von T. vivax. Das in T. brucei Oberflächenproteinen konservierte drei-Helix Grundgerüst ist auch in der NTD des ILDat1.2 VSGs enthalten. Die Architektur der Membranproximalen Gegend der IlDat1.2 NTD und CTD unterscheiden sich aber vermutlich von der der T. brucei VSGs. Das leicht handhabbare T. brucei System bietet somit ein geeignetes Modell um die Oberflächenproteine anderer afrikanischer Trypanosomen Spezies zu untersuchen und eröffnet neue Wege zur Charakterisierung ihrer Oberflächenmäntel. KW - Trypanosoma vivax KW - Trypanosoma brucei KW - Variant surface glycoprotein KW - messenger RNA KW - Regulation of expression KW - messenger RNA regulation KW - VSG structure Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-241773 ER - TY - JOUR A1 - Kraus, Amelie J. A1 - Brink, Benedikt G. A1 - Siegel, T. Nicolai T1 - Efficient and specific oligo-based depletion of rRNA JF - Scientific Reports N2 - In most organisms, ribosomal RNA (rRNA) contributes to >85% of total RNA. Thus, to obtain useful information from RNA-sequencing (RNA-seq) analyses at reasonable sequencing depth, typically, mature polyadenylated transcripts are enriched or rRNA molecules are depleted. Targeted depletion of rRNA is particularly useful when studying transcripts lacking a poly(A) tail, such as some non-coding RNAs (ncRNAs), most bacterial RNAs and partially degraded or immature transcripts. While several commercially available kits allow effective rRNA depletion, their efficiency relies on a high degree of sequence homology between oligonucleotide probes and the target RNA. This restricts the use of such kits to a limited number of organisms with conserved rRNA sequences. In this study we describe the use of biotinylated oligos and streptavidin-coated paramagnetic beads for the efficient and specific depletion of trypanosomal rRNA. Our approach reduces the levels of the most abundant rRNA transcripts to less than 5% with minimal off-target effects. By adjusting the sequence of the oligonucleotide probes, our approach can be used to deplete rRNAs or other abundant transcripts independent of species. Thus, our protocol provides a useful alternative for rRNA removal where enrichment of polyadenylated transcripts is not an option and commercial kits for rRNA are not available. KW - parasite biology KW - RNA sequencing KW - transcriptomics Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-224829 VL - 9 ER -