TY - THES A1 - Fink, Kristin T1 - Toxins in Renal Disease and Dialysis Therapy : Genotoxic Potential and Mechanisms T1 - Toxine in Nierenerkrankung und Dialyse Therapie : Genotoxisches Potential und Mechanismus N2 - In patients suffering from end-stage renal disease who are treated by hemodialysis genomic damage as well as cancer incidence is elevated. One possible cause for the increased genomic damage could be the accumulation of genotoxic substances in the blood of patients. Two possible sources for those toxins have to be considered. The first possibility is that substances from dialysers, the blood tubing system or even contaminated dialysis solutions may leach into the blood of the patients during dialysis. Secondly, the loss of renal filtration leads to an accumulation of substances which are normally excreted by the kidney. If those substances possess toxic potential, they are called uremic toxins. Several of these uremic toxins are potentially genotoxic. Within this thesis several exemplary uremic toxins have been tested for genotoxic effects (homocysteine, homocysteine-thiolactone,leptine, advanced glycated end-products). Additionally, it was analysed whether substances are leaching from dialysers or blood tubing and whether they cause effects in in vitrotoxicity testing. The focus of chemical analytisis was on bisphenol A (BPA), the main component of plastics used in dialysers and dialyser membranes. N2 - Patienten, die an terminaler Niereninsuffizienz leiden und mittels Hämodialyse behandelt werden, weisen einen erhöhten Genomschaden auf. Dieser könnte ursächlich für die erhöhte Krebsinzidenz dieser Patientengruppe sein. Eine der möglichen Ursachen für den erhöhten Genomschaden stellt die Akkumulation genotoxischer Substanzen im Blut der Patienten dar. Diese Substanzen können prinzipiell aus zwei unterschiedlichen Quellen stammen. Erstens besteht die Möglichkeit, dass während der Dialyse Substanzen aus den Dialysatoren, dem Blutschlauchsystem oder gar aus verunreinigtem Dialysat in das Blut der Patienten übertreten. Zweitens führt der Verlust der Nierenfunktion zu einer stark verminderten Exkretion harnpflichtiger Substanzen. Diese Substanzen akkumulieren im Blut und bilden, sofern sie ein toxisches Potential besitzen, die Gruppe der so genannten urämischen Toxine. Einige dieser urämischen Toxine sind potentiell auch genotoxisch. Im Rahmen der vorliegenden Dissertation wurden exemplarische Vertreter der urämischen Toxine auf ihre genotoxische Wirkung hin untersucht (Homocstein, Homocystein-Thiolacton, Leptin, Advanced Glycation End-Products). Außerdem wurde analysiert, ob Substanzen aus Dialysatormembranen oder dem Blutschlauchsystem austreten und in in vitro-Toxizitätstests Effekte zeigen. Der Fokus der Analytik lag hierbei auf dem Nachweis von Bisphenol A, dem Hauptbestandteil verschiedener Kunststoffe die für Dialysatoren und Dialysatormembranen verwendet werden. KW - Bisphenol A KW - Homocystein KW - Extrakorporale Dialyse KW - Genomschaden KW - Urämische Toxine KW - bisphenol a KW - homocysteine KW - dialysis KW - genomic damage KW - uremic toxins Y1 - 2008 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-31082 ER - TY - JOUR A1 - Figueiredo, Ludmilla A1 - Krauss, Jochen A1 - Steffan-Dewenter, Ingolf A1 - Cabral, Juliano Sarmento T1 - Understanding extinction debts: spatio-temporal scales, mechanisms and a roadmap for future research JF - Ecography N2 - Extinction debt refers to delayed species extinctions expected as a consequence of ecosystem perturbation. Quantifying such extinctions and investigating long‐term consequences of perturbations has proven challenging, because perturbations are not isolated and occur across various spatial and temporal scales, from local habitat losses to global warming. Additionally, the relative importance of eco‐evolutionary processes varies across scales, because levels of ecological organization, i.e. individuals, (meta)populations and (meta)communities, respond hierarchically to perturbations. To summarize our current knowledge of the scales and mechanisms influencing extinction debts, we reviewed recent empirical, theoretical and methodological studies addressing either the spatio–temporal scales of extinction debts or the eco‐evolutionary mechanisms delaying extinctions. Extinction debts were detected across a range of ecosystems and taxonomic groups, with estimates ranging from 9 to 90% of current species richness. The duration over which debts have been sustained varies from 5 to 570 yr, and projections of the total period required to settle a debt can extend to 1000 yr. Reported causes of delayed extinctions are 1) life‐history traits that prolong individual survival, and 2) population and metapopulation dynamics that maintain populations under deteriorated conditions. Other potential factors that may extend survival time such as microevolutionary dynamics, or delayed extinctions of interaction partners, have rarely been analyzed. Therefore, we propose a roadmap for future research with three key avenues: 1) the microevolutionary dynamics of extinction processes, 2) the disjunctive loss of interacting species and 3) the impact of multiple regimes of perturbation on the payment of debts. For their ability to integrate processes occurring at different levels of ecological organization, we highlight mechanistic simulation models as tools to address these knowledge gaps and to deepen our understanding of extinction dynamics. KW - Anthropocene KW - biotic interaction KW - extinction dynamics KW - mechanistic modelling KW - time lag KW - transient dynamics Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-204859 VL - 42 IS - 12 ER - TY - CHAP A1 - Fiala, Brigitte A1 - Rabenstein, R. A1 - Maschwitz, Ulrich T1 - Ant-attracting plant-structures: Food bodies of SE Asian Vitaceae N2 - No abstract available KW - Pflanzen Y1 - 1994 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-55177 ER - TY - JOUR A1 - Fiala, Brigitte A1 - Maschwitz, Ulrich A1 - Pong, Tho, Yow A1 - Helbig, Andreas J. T1 - Studies of a South East Asian ant-plant association : protection of Macaranga trees by Crematogaster borneensis N2 - In the humid tropics of SE Asia there are some 14 myrmecophytic species of the pioneer tree genus Macaranga (Euphorbiaceae). In Peninsular Malaysia a close association exists between the trees and the small, non-stinging myrmicine Crema togas ter borneensis. These ants feed mainly on food bodies provided by the plants and have their colonies inside the hollow intemodes. In a ten months field study we were able to demonstrate for four Macaranga species (M. triloba, M. hypoleuca, M. hosei, M. hulletti) that host plants also benefit considerably from ant-occupation. Ants do not contribute to the nutrient demands of their host plant, they do, however, protect it against herbivores and plant competition. Cleaning behaviour of the ants results in the removal of potential herbivores already in their earliest developmental stages. Strong aggressiveness and a mass recruiting system enable the ants to defend the host plant against many herbivorous insects. This results in a significant decrease in leaf damage due to herbivores on ant-occupied compared to ant-free myrmecophytes as well as compared to non-myrmecophytic Macaranga species. Most important is the ants' defense of the host plant against plant competitors, especially vines, which are abundant in the well-lit pioneer habitats where Macaranga grows. Ants bite off any foreign plant part coming into contact with their host plant. Both ant-free myrmecophytes and non-myrmecophytic Macaranga species had a significantly higher incidence of vine growth than specimens with active ant colonies. This may be a factor of considerable importance allowing Macaranga plants to grow at sites of strongest competition. KW - Ant/plant interaction KW - Myrmecophytes KW - Protection KW - Macaranga KW - Crematogaster borneensis Y1 - 1989 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-42857 ER - TY - JOUR A1 - Fiala, Brigitte A1 - Maschwitz, Ulrich T1 - Studies on the south east asian ant-plant association Crematogaster borneensis / Macaranga: adaptations of the ant partner. N2 - C. borneensis (Myrmicinae) lives in dose association with several myrmecophytic species of the South East Asian pioneer tree genus Macaranga (Euphorbiaceae). The ants are adapted to the plants so dosely that they do not survive away from it. The only food they utilize is provided as food bodies by the plant and honeydew from specific scale insects kept inside the hollow internodes. The anatomy of the digestive tract is also adapted to life on the host plant: the crop is very sm all and can store only minute food quantities. C. borneensis exdusively colonizes certain Macaranga species. Queens as weIl as workers are able to recognize their host plant species, probably by chemical cues. Colony founding queens swarm throughout the year, mostly during darkness. There is strong competition among queens for host plants. Queens do not carry scale insects on their nuptial flight. Worker ants are active day and night. Most of them patrol and collect food bodies on the younger parts of the host plant. An important characteristic is their deaning behaviour, which results in removal of aIl foreign objects. Even though they are rather smalI, workers respond very aggressively to certain kinds of disturbance of the host plant. The ants attack most phytophagous insects and are especially effective in killing and removing smalI, softbodied herbivores (e.g. caterpillars). They do not possess a functional sting, but apply defensive secretion and-once biting an intruder-will not let go. Their effective alarm system results in a mass attack, which provides adequate defence for the colony and the host plant. A comparison with another Crematogaster species further illustrated the special adaptations of C. borneensis to its host plant. N2 - Untersuchungen über die südostasiatische Ameisen·Pflanzen-Vergesellschaftung Cremattogaster borneensis Maoaranga : Anpassungen des Ameisenpartners 213 C. borneensis (Myrmicinae) lebt in enger Gemeinschaft mit myrmekophytischen Arten der südostasiatischen Pionierbaumgattung Macaranga (Euphorbiaceae) . Die Ameise ist so eng an die Pflanze adaptiert, daß sie getrennt von ihr nicht lebensfähig ist. Die Nahrung bezieht C. borneensis in Form von Nährkörperchen ausschließlich von der Pflanze. Im Sproßachseninnern gehaltene spezifische Schildläuse bieten eine weitere Nahrungsquelle. Die Adaptationen erstrecken sich bis auf die Anatomie des Verdauungstraktes : Der Kropf ist sehr klein und kann nur geringe Nahrungsmengen speichern. C. borneensis besiedelt spezifisch nur Macaranga-Pflanzen. Sowohl Königinnen als auch Arbeiterinnen sind in der Lage, die Wirtspflanze zu erkennen, wobei offenbar chemische Reize eine Rolle spielen. Die koloniegründenden Königinnen schwärmen das gesamte Jahr über, das Schwärmen erfolgt überwiegend während der Dunkelheit. Um die besiedlungsfähigen Macaranga-Pflanzen herrscht ein starker Konkurrenzdruck. Die beteiligten Schildlausarten sind spezifisch für die Assoziation. Sie werden nicht von der Königin beim Hochzeitsflug mitgenommen. Die Arbeiterinnen sind tag- und nachtaktiv. Die meisten Tiere halten sich im jüngsten Drittel der Pflanze auf, wo sie patrouillieren und Nährkörperchen sammeln. Mittels eines spezifischen Säuberungsverhaltens entfernen die Arbeiterinnen alle Fremdobjekte von der Pflanze. Trotz ihrer geringen Größe attackieren die Ameisen eine Vielzahl phytophager Insekten und sind dabei besonders effektiv in der Abwehr kleiner, wenig sklerotisierter Tiere wie z.B. Raupen. Sie verfügen zwar nicht ' über einen funktionsfähigen Stachel, setzen aber Wehrsekrete ein und beißen sich hartnäckig fest . Mit Hilfe eines effektiven Alarmierungssystems, das einen Massenangriff ermöglicht, gewährleisten sie eine Verteidigung ihrer Kolonien und damit gleichzeitig ihrer Wirtspflanze. Eine Vergleich mit einer anderen Crematogaster-Art demonstriert die besonderen Adaptationen von C. borneensis an ihre Wirtspflanze. Y1 - 1990 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-32689 ER - TY - JOUR A1 - Fiala, Brigitte A1 - Maschwitz, Ulrich T1 - Food bodies and their significance for obligate ant-association in the tree genus Macaranga (Euphorbiaceae) N2 - The production of extrafloral nectar and food bodies plays an important role in many tropical ant-plant mutualisms. In Malaysia, a close association exists between ants and some species of the pioneer tree genus Macaranga (Euphorbiaccac). Macaranga is a very diverse genus which exhibits all stages ofintcraction with ants, from facultative to obligatory associations. The ants nest inside the hollow inlcrnodes and reed mainly on food budies provided by the plants. Food body production had previously been reported only in myrrnecophytic Macaranga species, where it is usually coneentrated on protected parts or the plants such as recurved stipules. We found that non-myrmecophytic Macaranga species also produce food bodies on leaves and stems, where they are collected by a variety or ants. Levels of food body production differ between facultatively and obligatorily ant-associated species but also among the various non-myrmecophytes. This may he rdated to the degree of interaction with ants. Food body production starts at a younger age in the myrmccophytic species than in the transitional or non-myrmcccophytic Macaranga. Although food bodies of the non-inhabited Macaranga species are collected by a variety of ants, there is nu evidence of association with specific ant species. Our observations suggest that food bodies enhance the evolution of ant-plant interactions. Production of food bodies alone, however, does not appear to be the most important factor for the development of obligate myrmccopllytism in Macaranga. KW - Ant-plant interactions KW - evolution KW - food bodies KW - Macaranga KW - Malaysia KW - myrmrcophytism Y1 - 1992 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-32921 ER - TY - JOUR A1 - Fiala, Brigitte A1 - Maschwitz, Ulrich T1 - Domatia as most important adaptations in the evolution of myrmecophytes in the paleotropical tree genus Macaranga (Euphorbiacae) N2 - The paleotropical tree genus Macaranga (Euphorbiaceae) comprises all stages of interaction with ants, from facultative associations to obligate myrmecophytes. In SE.-Asia food availability does not seem to be the limiting factor for the development of a close relationship since all species provide food for ants in form of extrafloral nectar and/or food bodies. Only myrmecophytic Macaranga species offer nesting space for ants (domatia) inside intern odes which become hollow due to degeneration of the pith. Non-myrmecophytic species have a solid stem with a compact and wet pith and many resin ducts. The stem interior of some transitional species remains solid, but the soft pith can be excavated. The role of different ant-attracting attributes for the development of obligate ant-plant interactions is discussed. In the genus Macaranga, the provision of nesting space seems to be the most important factor for the evolution of obligate myrmecophytism. KW - Angiosperms ; Ant-plant interactions ; domatia ; Flora of Malaysia Y1 - 1992 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-32935 ER - TY - JOUR A1 - Fiala, Brigitte A1 - Maschwitz, Ulrich T1 - Extrafloral nectaries in the genus Macaranga (Euphorbiaceae) in Malaysia: comparative studies of their possible significance as predispositions for myrmecophytism. N2 - So me species of the paleotropical tree genus Macaranga (Euphorbiaceae) live in elose association with ants. Thc genus comprises the full range of species from those not regularly inhabited by ants to obligate myrmecophytes. In Malaysia (peninsular and Borneo) 23 ofthe 52 species areknown to be ant-associated (44%). The simplest structural adaptation of plants to attract ants are extrafloral nectaries. We studied the distribution of extraflural nectaries in the genus Macaranga to assess the significance of this character as a possible predisposition for the evolution of obligate myrmecophytism. All species have marginal glands on the leaves. However, only the glands of nonmyrmecophytic species function as nectaries, whereas liquids secreted by these glands in myrmecophytic species did not contain sugar. Some non-myrmecophytic Macaranga and transitional Macaranga species in addition have extrafloral nectaries on the leaf blade near the petiole insertion. All obligatorily myrmecophytic Macaranga species, however, lack additional glands on the lamina. The non-myrmecophytic species are visited by a variety of different ant species, whereas myrmecophytic Macaranga are associated only with one specific ant-partner. Since these ants keep scale insects in the hollow sterns, reduction of nectary production in ant-inhabited Macaranga seems to be biologically significant. We interpret this as a means of (a) saving the assimilates and (b) stabilization of maintenance of the association's specificity. Competition with other ant species for food rewards is avoided and thereby danger ofweakening the protective function ofthe obligate antpartner for the plant is reduced. A comparison with other euphorb species living in the same habitats as Macaranga showed that in genera in which extrafloral nectaries are widespread, no myrmecophytes have evolved. Possession of extrafloral nectaries does not appear to be essential for the development of symbiotic ant-plant interactions. Other predispositions such as nesting space might have played a more important role. KW - Macaranga KW - extrafloral nectaries KW - ant-plant interactions KW - evolution of myrmecophytism KW - Malaysia Y1 - 1991 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-42863 ER - TY - JOUR A1 - Fiala, Brigitte A1 - Grunsky, Harald A1 - Maschwitz, Ulrich A1 - Linsenmair, Karl Eduard T1 - Diversity of ant-plant interactions: Protective efficacy in Macaranga species with different degrees of ant-association. N2 - The pioneer tree Macaranga in SE Asia has developed manyfold associations with ants. The genus comprises all stages of interaction with ants, from facultative relationships to obligate myrmecophytes. Only myrmecophytic Macaranga offer nesting space for ants and are associated with a specific ant partner. The nonmyrmecophytic species are visited by a variety of different ant species which are attracted by extrafloral nectaries (EFN) and food bodies. Transitional Macaranga species like M. hosei are colonized later in their development due to their stem structure. Before the colonization by their specific Crematogaster partner the young plants are visited by different ant species attracted by EFN. These nectaries are reduced and food body production starts as soon as colonization becomes possible. We demonstrated earlier that obligate ant partners can protect their Macaranga plants against herbivore damage and vine cover. In this study we focused on nonspecific interactions and studied M. tanarius and M. hosei, representing a non-myrmecophyte and a transitional species respectively. In ant exclusion experiments both M. tanarius and M. hosei suffered significantly higher mean leaf damage than controls, 37% versus 6% in M. hosei, 16% versus 7% in M. tanarius. M. tanarius offers both EFN and food bodies so that tests for different effects of these two food rewards could be conducted. Plants with food bodies removed but with EFN remaining had the lowest mean increase of herbivore damage of all experimental groups. Main herbivores on M. hosei were mites and caterpillars. Many M. tanarius plants were infested by a shootborer. Both Macaranga species were visited by various ant species. Crematogaster spp. being the most abundant. We found no evidence for any specific relationships. The results of this study strongly support the hypothesis that non-specific, facultative associations with ants can be advantageous for Macaranga plants. Food bodies appear to have lower attractive value for opportunistic ants than EFN and may require a specific dietary adaptation. This is also indicated by the fact that food body production in the transitional M. hosei does not start before stem structure allows a colonization by the obligate Crematogaster species. M. hosei thus benefits from facultative association with a variety of ants until it produces its first domatia and can be colonized by its obligate mutualist. KW - Ant-plant interactions ; Herbivory Macaranga ; Mutualism ; Myrmecophytes Y1 - 1994 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-32905 ER - TY - CHAP A1 - Fiala, Brigitte A1 - Federle, W. A1 - Maschwitz, U. A1 - Azarae, Idris T1 - The first myrmecophytic 2-partner-system in the genus Macaranga: The association between Macaranga puncticulata and a Componotus (Colobopsis) in Malaysia N2 - No abstract available KW - Biologie Y1 - 1994 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-55144 ER - TY - JOUR A1 - Fiala, Brigitte T1 - Extrafloral nectaries versus ant-Homoptera mutualisms : a comment on Becerra and Venable N2 - No abstract available KW - Nektarium KW - Ameise Y1 - 1990 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-32948 ER - TY - THES A1 - Fetiva Mora, Maria Camila T1 - Changes in chromatin accessibility by oncogenic YAP and its relevance for regulation of cell cycle gene expression and cell migration T1 - Änderungen der Chromatinzugänglichkeit durch onkogene YAP und seine Relevanz für die Genexpression während des Zellzyklus und für die Zellmigration N2 - Various types of cancer involve aberrant cell cycle regulation. Among the pathways responsible for tumor growth, the YAP oncogene, a key downstream effector of the Hippo pathway, is responsible for oncogenic processes including cell proliferation, and metastasis by controlling the expression of cell cycle genes. In turn, the MMB multiprotein complex (which is formed when B-MYB binds to the MuvB core) is a master regulator of mitotic gene expression, which has also been associated with cancer. Previously, our laboratory identified a novel crosstalk between the MMB-complex and YAP. By binding to enhancers of MMB target genes and promoting B-MYB binding to promoters, YAP and MMB co-regulate a set of mitotic and cytokinetic target genes which promote cell proliferation. This doctoral thesis addresses the mechanisms of YAP and MMB mediated transcription, and it characterizes the role of YAP regulated enhancers in transcription of cell cycle genes. The results reported in this thesis indicate that expression of constitutively active, oncogenic YAP5SA leads to widespread changes in chromatin accessibility in untransformed human MCF10A cells. ATAC-seq identified that newly accessible and active regions include YAP-bound enhancers, while the MMB-bound promoters were found to be already accessible and remain open during YAP induction. By means of CRISPR-interference (CRISPRi) and chromatin immuniprecipitation (ChIP), we identified a role of YAP-bound enhancers in recruitment of CDK7 to MMB-regulated promoters and in RNA Pol II driven transcriptional initiation and elongation of G2/M genes. Moreover, by interfering with the YAP-B-MYB protein interaction, we can show that binding of YAP to B-MYB is also critical for the initiation of transcription at MMB-regulated genes. Unexpectedly, overexpression of YAP5SA also leads to less accessible chromatin regions or chromatin closing. Motif analysis revealed that the newly closed regions contain binding motifs for the p53 family of transcription factors. Interestingly, chromatin closing by YAP is linked to the reduced expression and loss of chromatin-binding of the p53 family member Np63. Furthermore, I demonstrate that downregulation of Np63 following expression of YAP is a key step in driving cellular migration. Together, the findings of this thesis provide insights into the role of YAP in the chromatin changes that contribute to the oncogenic activities of YAP. The overexpression of YAP5SA not only leads to the opening of chromatin at YAP-bound enhancers which together with the MMB complex stimulate the expression of G2/M genes, but also promotes the closing of chromatin at ∆Np63 -bound regions in order to lead to cell migration. N2 - Ein Kennzeichen vieler Tumoren ist die fehlerhafte Aktivierung von zellzyklusregulierenden Signalwegen. Ein für das Tumorwachstum wichtiger Signalwege ist der Hippo-Signalweg und das durch ihn regulierte Onkogen YAP, ein transkriptioneller Koaktivator. Durch die Regulierung von Zellzyklusgenen ist YAP verantwortlich für onkogene Prozesse wie Zellproliferation und Metastasierung. Der MMB-Multiproteinkomplex wiederum – er entsteht, wenn B-MYB an das MuvB-Kernmodul bindet – ist ein wichtiger Regulator der mitotischen Genexpression, welche ebenso mit der Tumorentstehung in Verbindung gebracht wurde. Unser Labor hat zuvor einen neuen Mechanismus der Regulation mitotischer Gene durch den MMB-Komplex und YAP identifiziert: Durch die Bindung an Enhancer der MMB-Zielgene und die Förderung der B-MYB-Bindung an Promotoren reguliert YAP eine Reihe von mitotischen und zytokinetischen Zielgenen, welche die Zellproliferation fördern. Diese Doktorarbeit befasst sich mit den Mechanismen der YAP- und MMB-vermittelten Transkription und charakterisiert die Rolle der YAP regulierten Enhancer während der Transkription von Zellzyklusgenen. Die in dieser Dissertation dargelegten Ergebnisse zeigen, dass die Expression von konstitutiv aktivem, onkogenem YAP5SA zu weitreichenden Veränderungen in der Chromatinzugänglichkeit nicht-transformierter humaner MCF10A Zellen führt. ATAC-seq zeigte, dass ein grosse Anzahl YAP-gebundene Enhancer zugänglich und aktiviert werden. Gleichzeitig konnte festgestellt werden, dass die MMB-gebundenen Promotoren bereits vor der Expression von YAP zugänglich sind und während der YAP-Induktion offen bleiben. Mittels CRISP-Interferenz (CRISPRi) und Chromatin-Immunpräzipitationen (ChIP) konnten wir zeigen, dass YAP-gebundene Enhancer die Rekrutierung von CDK7 an MMB-regulierten Promotoren sowie die Initiation und Elongation der Transkription von G2/M Genen fördert. Durch die experimentelle Blockade der YAP-B-MYB Proteininteraktion konnten wir darüber hinaus belegen, dass auch die Bindung von YAP an B-MYB für die Initiation der Transkription an MMB-regulierten Genen entscheidend ist. Unerwarteterweise führte die Überexpression von YAP5SA auch dazu, dass bestimmte Regionen im Genom weniger zugänglich werden. Motivanalysen ergaben, dass diese neu geschlossenen Regionen Bindungsmotive für die p53-Familie von Transkriptionsfaktoren enthalten. Die Chromatinschließung durch YAP ist an eine reduzierte Expression und an den Verlust der Chromatinbindung des p53-Familienmitglieds Np63 gekoppelt. Schließlich konnte gezeigt werden, dass die Inhibition von Np63 durch YAP ein wichtiger Schritt in der YAP-abhängigen Förderung der Zellmigration ist. Zusammenfassend liefern die Ergebnisse dieser Dissertation Einblicke in die Rolle von YAP bei Chromatinveränderungen welche zu den onkogenen Aktivitäten von YAP beitragen. Die Überexpression von YAP führt dabei einerseits zur Öffnung des Chromatins an YAP-gebundenen Enhancern, die zusammen mit dem MMB-Komplex die Expression von G2/M Genen stimulieren. Andererseits fördert YAP auch das Schließen von Chromatin an Np63-gebundenen Regionen, was wiederum Zellmigration nach sich zieht. KW - YAP KW - B-MYB KW - MMB KW - enhancers KW - transcription KW - chromatin accessibility KW - opening of chromatin KW - closing of chromatin KW - cell migration KW - G2/M genes KW - Chromatin KW - Genexpression KW - Zellzyklus KW - Zellmigration Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-302910 ER - TY - JOUR A1 - Ferreira, Eliana Aparecida A1 - Boff, Samuel A1 - Verza, Sandra S. A1 - Mussury, Rosilda Mara T1 - Bioecological and behavioral interaction between pollinating bees and the pioneer shrub Ludwigia nervosa in degraded area suggests an exotic bee as its major pollinator JF - Biology N2 - The flowers of plants of the genus Ludwigia are an important source of food for several species of bees. In the current study, we conducted an experiment with the aim to describe the reproductive biology and phenology of L. nervosa; to identify the species of visiting bees; analyze the foraging behavior of bees; and to investigate whether the reproductive success of the species is related to the foraging activity of bees. We found that the flowers received visits from several native bee species (n = 7), in addition of the exotic honey bees which came to be the dominant species. During visits the majority of the bees foraged in both resources, pollen and nectar. The significantly higher production of fruits in open pollinated pollination experiment compared to artificial cross pollination, suggests honey bees as effective pollinator of this plant species in the study site. Pollen deposition occurs efficiently, given the absence of pollen limitation. Despite massive visitation of honey bees, Ludwigianervosa is attractive to native bees, and therefore it may help to sustain population of both native and exotic pollinators in fragmented humid areas. KW - cross pollination KW - disturbed humid area KW - germination speed KW - honey bees and native bees KW - pollen limitation Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-228757 SN - 2079-7737 VL - 10 IS - 2 ER - TY - THES A1 - Fernández-Mora, Eugenia T1 - Analysis of the maturation of Rhodococcus equi-containing vacuoles in macrophages T1 - Analyse der Reifung von Rhodococcus equi-enthaltenden Phagosomen in Makrophagen N2 - Rhodococcus equi is a Gram-positive intracellular pathogen which can cause severe bronchopneumonia in foals. In recent years, the role of this bacterium as human pathogen has been noted, as R.equi infections in humans have increase in frequency. This increase is associated with the rise in immunosupressed individuals, specially AIDS patients, where infection leads to symptoms and pathology similar to those seen in foals with a high mortality rate. Due to its capability to survive and multiply in murine and equine macrophages, R.equi has been classified as a facultative intracellular bacterium. R.equi is found frequently in macrophages in alveolar infiltrate from infected animals. The pathogenicity of R.equi depends on its ability to exist and multiply inside macrophages and has been associated with the presence of virulence plasmids. It has been observed that, inside foal alveolar macrophages, R.equi-containing vacuoles (RCVs) do not mature into phagolysosomes. However, most of the intracellular events during R.equi infection have not been investigated in detail. The aim of this study was to elucidate the intracellular compartmentation of R.equi and the mechanism by which the bacteria avoid destruction in host macrophages. The importance of the virulence-associated plasmids of R.equi for the establishment of RCVs was also evaluated. Furthermore, the intracellular fate of viable and non-viable R.equi was compared in order to study whether viability of R.equi influeciantes the establishment of RCVs. In this study, the RCV was characterized by using a variety of endocytic markers to follow the path of the bacteria trhough murine macropages. Transmission electron microscopy-base analysis showed that R.equi was found equally frequently in phagosomes with loosely or thightly apposed membranes, and RCV often contains numerous membranous vesicles. Laser scanning microscopy of infected macrophages showed that the majority of phagosomes containing R.equi acquired transiently the early endosomal markers Rab5, Ptlns3P, and EEA-1, suggesting initially undisturbed phagosome maturation. Although the RCV acquired some late endosomal markers, such as Rab7, LAMP-1, and Lamp-2, they did not acquired vATPase, did not interact with pre-labeled lysosomes, and failed to acidify. These data clearly suggest that the RCV is a compartment which has left vacuoles that resemble multivesicular body compartments (MVB), which are transport intermediates between early and late endosomes and display internal vesicles very similar to the ones observed within RCVs. Analyisis of several R.equi strains containing either VapA- or VapB-expressing plasmids or neither demonstrated that the possession of the virulence-associated plasmids does not affect phagosome trafficking over a two hour period of infection. The finding that non-viable R.equi was still able to inhibit phagosome maturation (although not to the same extent as viable R.equi did) suggests that heat-insensitive factors, such as cell periphery lipids, may play a major role in inhibition of phagosome maturation, although heat-sensitive factors may also be involved. N2 - Rhodococcus equi ist ein Gram-positives, fakultativ intrazelulläres Bakterium, das unter anderem die Ursache von Bronchopneumonien bei Fohlen ist. Menschen und andere Säugetiere können ebenfalls von Infektionen mit R. equi betroffen sein. In den letzten Jahren ist die Häufigkeit klinischer Infektionen mit R. equi bei Menschen gestiegen. Die wachsende Anzahl an mmunosupprimierten Patienten (hauptsächlich AIDS-Patienten) liegt dieser Zunahme an Infektionen zugrunde. Die Symptomatologie und Pathologie der Infektion mit R. equi ist bei AIDS-Patienten und Fohlen ähnlich. Die Sterblichkeitsrate ist in beiden Fällen hoch. Die Fähigkeit der Rhodokokken, innerhalb von Makrophagen zu überleben und sich zu vermehren, ist mit dem Vorhandensein von Virulenzplasmiden (virulence-associated plasmids) verbunden. Innerhalb des Makrophagen befinden sich die Rhodokokken in einem Phagosom, das nicht mit Lysosomen fusioniert. Die genaue Kompartimentierung der Rhodococcus equi-enthaltenden Phagosomen in Makrophagen war bisher unbekannt und wurde deshalb in der vorliegenden Promotionsarbeit untersucht. Mit Hilfe mehrerer endozytischer Marker wurde das R. equi-enthaltende Kompartiment charakterisiert. Mögliche Unterschiede zwischen der Kompartimentierung von R. equi(+)- und R. equi(-)-enthaltenden Phagosomen ist ebenfalls Thema dieser Promotionsarbeit. Weiterhin wurde die Etablierung des phagosomalen Kompartiments für jeweils lebende und tote Rhodokokken verglichen. Transmissionselektronenmikroskopische Analysen haben gezeigt, dass die Phagosomenmembran Rhodococcus equi-enthaltender Phagosomen sowohl locker als auch eng anliegend sein kann (50%). Darüber hinaus wurden häufig zahlreiche, membranöse Vesikel in R. equi-enthaltenden Phagosomen gefunden. Diese Phagosomen zeigen somit Ähnlichkeiten zu Multivesicular Bodies. Multivesicular Bodies sind intermediäre Kompartimente zwischen frühen und späten Endosomen und zeigen ebenfalls eine Vielzahl von internen Vesikeln. Untersuchungen am konfokalen Lasermikroskop ergaben, dass die Mehrheit der R. equi-enthaltenden Phagosomen die früh endosomalen Marker Rab5, PtIns3P und EEA-1 transient akquirieren. Dieser Befund deutet auf eine ungestörte phagosomale Reifung im frühen Stadium hin. Trotz der beobachteten Akquisition der spät endosomalen Marker Rab7, LAMP-1 und LAMP-2 konnte keine Akquisition der vATPase, keine Interaktion mit vormarkierten Lysosomen und keine Ansäuerung von R.equi-enthaltenden Phagosomen nachgewiesen werden. Diese Ergebnisse weisen darauf hin, dass R. equi-enthaltende Phagosomen das früh endosomale Stadium abschließen, aber einen typisch spät endosomale Zustand nicht erreichen. Die Analyse unterschiedlicher R. equi-Stämme, die entweder vapA- oder vapB-exprimierende Virulenzplasmide enthalten, hat gezeigt, dass die Anwesenheit von Virulenzplasmiden die phagosomale Reifung über eine Infektionsperiode von zwei Stunden nicht beeinflusst. Getötete Rhodokokken waren in der Lage, die phagosomale Reifung zu inhibieren, aber in geringerem Ausmaß als lebende Rhodokokken. Das weist darauf hin, dass hitze-insensitive Faktoren (wie zum Beispiel Lipide der Zellwand) zur Inhibierung der phagosomalen Reifung entscheidend sind, obwohl dazu auch hitze-sensitive Faktoren (wie Proteine) relevant sein können. KW - Rhodococcus equi KW - Makrophage KW - Vakuole KW - Endosome KW - Phagosome KW - Rhodococcus KW - Mycobacterium KW - Reifung KW - endosome KW - phagosome KW - Rhodococcus KW - Mycobacterium KW - maturation Y1 - 2005 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-14049 ER - TY - JOUR A1 - Ferero, Andrea A1 - Rivero, Olga A1 - Wäldchen, Sina A1 - Ku, Hsing-Ping A1 - Kiser, Dominik P. A1 - Gärtner, Yvonne A1 - Pennington, Laura S. A1 - Waider, Jonas A1 - Gaspar, Patricia A1 - Jansch, Charline A1 - Edenhofer, Frank A1 - Resink, Thérèse J. A1 - Blum, Robert A1 - Sauer, Markus A1 - Lesch, Klaus-Peter T1 - Cadherin-13 Deficiency Increases Dorsal Raphe 5-HT Neuron Density and Prefrontal Cortex Innervation in the Mouse Brain JF - Frontiers in Cellular Neuroscience N2 - Background: During early prenatal stages of brain development, serotonin (5-HT)-specific neurons migrate through somal translocation to form the raphe nuclei and subsequently begin to project to their target regions. The rostral cluster of cells, comprising the median and dorsal raphe (DR), innervates anterior regions of the brain, including the prefrontal cortex. Differential analysis of the mouse 5-HT system transcriptome identified enrichment of cell adhesion molecules in 5-HT neurons of the DR. One of these molecules, cadherin-13 (Cdh13) has been shown to play a role in cell migration, axon pathfinding, and synaptogenesis. This study aimed to investigate the contribution of Cdh13 to the development of the murine brain 5-HT system. Methods: For detection of Cdh13 and components of the 5-HT system at different embryonic developmental stages of the mouse brain, we employed immunofluorescence protocols and imaging techniques, including epifluorescence, confocal and structured illumination microscopy. The consequence of CDH13 loss-of-function mutations on brain 5-HT system development was explored in a mouse model of Cdh13 deficiency. Results: Our data show that in murine embryonic brain Cdh13 is strongly expressed on 5-HT specific neurons of the DR and in radial glial cells (RGCs), which are critically involved in regulation of neuronal migration. We observed that 5-HT neurons are intertwined with these RGCs, suggesting that these neurons undergo RGC-guided migration. Cdh13 is present at points of intersection between these two cell types. Compared to wildtype controls, Cdh13-deficient mice display increased cell densities in the DR at embryonic stages E13.5, E17.5, and adulthood, and higher serotonergic innervation of the prefrontal cortex at E17.5. Conclusion: Our findings provide evidence for a role of CDH13 in the development of the serotonergic system in early embryonic stages. Specifically, we indicate that Cdh13 deficiency affects the cell density of the developing DR and the posterior innervation of the prefrontal cortex (PFC), and therefore might be involved in the migration, axonal outgrowth and terminal target finding of DR 5-HT neurons. Dysregulation of CDH13 expression may thus contribute to alterations in this system of neurotransmission, impacting cognitive function, which is frequently impaired in neurodevelopmental disorders including attention-deficit/hyperactivity and autism spectrum disorders. KW - serotonin KW - cadherin-13 (CDH13) KW - T-cadherin KW - neurodevelopment KW - psychiatric disorders KW - radial glia KW - dorsal raphe KW - prefrontal cortex Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-170313 VL - 11 IS - 307 ER - TY - JOUR A1 - Ferber, Elena A1 - Gerhards, Julian A1 - Sauer, Miriam A1 - Krischke, Markus A1 - Dittrich, Marcus T. A1 - Müller, Tobias A1 - Berger, Susanne A1 - Fekete, Agnes A1 - Mueller, Martin J. T1 - Chemical Priming by Isothiocyanates Protects Against Intoxication by Products of the Mustard Oil Bomb JF - Frontiers in Plant Science N2 - In Brassicaceae, tissue damage triggers the mustard oil bomb i.e., activates the degradation of glucosinolates by myrosinases leading to a rapid accumulation of isothiocyanates at the site of damage. Isothiocyanates are reactive electrophilic species (RES) known to covalently bind to thiols in proteins and glutathione, a process that is not only toxic to herbivores and microbes but can also cause cell death of healthy plant tissues. Previously, it has been shown that subtoxic isothiocyanate concentrations can induce transcriptional reprogramming in intact plant cells. Glutathione depletion by RES leading to breakdown of the redox potential has been proposed as a central and common RES signal transduction mechanism. Using transcriptome analyses, we show that after exposure of Arabidopsis seedlings (grown in liquid culture) to subtoxic concentrations of sulforaphane hundreds of genes were regulated without depletion of the cellular glutathione pool. Heat shock genes were among the most highly up-regulated genes and this response was found to be dependent on the canonical heat shock factors A1 (HSFA1). HSFA1-deficient plants were more sensitive to isothiocyanates than wild type plants. Moreover, pretreatment of Arabidopsis seedlings with subtoxic concentrations of isothiocyanates increased resistance against exposure to toxic levels of isothiocyanates and, hence, may reduce the autotoxicity of the mustard oil bomb by inducing cell protection mechanisms. KW - autotoxicity KW - heat shock response KW - isothiocyanates KW - mustard oil bomb KW - reactive electrophilic species KW - redox homeostasis KW - sulforaphane Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-207104 SN - 1664-462X VL - 11 ER - TY - THES A1 - Feldmann, Kristina T1 - Signal transduction of transforming growth factor-Beta in cytotoxic T cells T1 - Signaltransduktion von Transforming-Growth-Factor-beta in Zytotoxischen T-Zellen N2 - Transforming-Growth-Factor-beta1 (TGF-b1) ist ein multifunktionelles Zytokin, welches insbesondere Zellwachstum und Zelldifferenzierung koordiniert. TGF-b ist vor allem dafür bekannt, Zellen des Immunsystems zu beeinflussen. TGF-b steuert zum Beispiel die Differenzierung von T-Zellen und und deren Effektorfunktionen. Die Signaltransduktion von TGF-b wird vermittelt durch die Phosphorylierung von Rezeptor-assoziierten Smad-Proteinen (R-Smads). R-Smads werden vom Typ I Rezeptor aktiviert, der seinerseits vom hochaffinen Typ II Rezeptor phosphoryliert wird, sobald der Ligand bindet. Die phosphorylierten RSmads assoziieren darauf mit Co-Smads. Heterooligomere von R-Smads und Co-Smads wandern dann in den Zellkern, wo sie im Zusammenspiel mit Transkriptionsfaktoren wie CBP/p300 oder AP-1 die Transkription TGF-b-spezifischer Zielgene koordinieren. Neue Erkenntnisse lassen vermuten, daß die pleiotropen Effekte von TGF-b durch das Interagieren mit anderen Signalkaskaden entstehen, zum Beispiel mit dem MAP-Kinase-Weg oder der STAT-Kaskade. Wir beschreiben hier den Effekt von TGF-b auf die Effektorfunktionen unterschiedlich stimulierter primärer Maus-Milzzellen und aufgereinigten zytotoxischen CD8+ Maus-TZellen. Langzeitbehandlung mit TGF-b resultierte in der Unfähigkeit der Zellen, Smad2 ligandeninduziert zu phosphorylieren. Entweder wurde überhaupt keine Phosphorylierung beobachtet, oder eine anhaltende Phosphorylierung von Smad2 unabhängig vom Vorhandensein des Liganden. Des weiteren stellten wir einen Zusammenhang zwischen anhaltender Smad2-Phosphorylierung und der Resistenz gegenüber TGF-b induzierter Wachstumshemmung fest. Im Gegensatz dazu zeigen Zellen, die sensitiv sind gegenüber TGF-b vermittelter Wachstumshemmung, keine Smad2-Phosphorylierung mehr. Bezüglich ihrer zytotoxische Aktivtät waren allerdings beide Phänotypen nicht mehr lytisch wirksam, unabhängig von der jeweiligen Smad2-Phosphorylierung. In dieser Arbeit zeigen wir auch die Notwendigkeit eines funktionalen MEK-1-Signalweges auf, der unabdingbar ist, damit TZellen keine Wachstumsinhibierung durch TGF-b mehr erfahren. Das Blockieren dieses Signalweges führt darüberhinaus bei diesen Zellen ebenfalls zu einem veränderten Smad2- Phosphorylierungsmuster. Bezüglich des JNK-Signalweges konnten wir feststellen, daß ein funktional aktiver JNK-Signalweg mit der Resistenz gegenüber TGF-b vermittelter Wachstumsinhibierung einhergeht. Allerdings führt die Zugabe von IFNg und/oder aCD28- Antikörper nicht zu einer veränderten Sensitivität gegenüber TGF-b. Im Gegensatz zuprimären Zellen können die beschriebenen Zusammenhänge in Zellkulturen vom humanen und murinen T Zellen nicht beobachtet werden, und sind somit spezifisch für primare TZellen. Wir beschreiben auch die Klonierung eines chimären dominant-negativen Typ II Rezeptors, der an eine Kinase gekoppelt ist, die bei Aktivierung Zelltod auslöst. Damit soll es in Zukunft möglich sein, T-Zellen gegenüber TGF-b Resistenz zu verleihen. Die hier geschilderten Ergebnisse vertiefen die Kenntnisse über molekulare Mechanismen der Wirkung von TGF-b auf T-Zellen und können vielleicht dazu beitragen, negative Effekte von TGF-b, zum Beispiel in der Tumortherapie, gezielt abzuwenden. N2 - Transforming-Growth-Factor-beta1 (TGF-b1) is a multifunctional cytokine that regulates cell growth and differentiation in many types of cells. TGF-b1 is especially known to exert a variety of regulatory functions in the immune system, such as T cell differentiation and T cell function. Signal transduction of TGF-b1 is mediated by phosphorylation of receptorassociated Smad proteins (R-Smads). R-Smads are phosphorylated by the activated type I receptor, which is itself phosphorylated by the high affinity type II receptor upon ligand binding. The phosphorylated R-Smads then associate with Co-Smads. Heterooligomers of R- and Co-Smads translocate into the nucleus where they regulate transcription of target genes in concert with other transcription factors such as CBP/p300 or AP-1. Recent findings suggest that the pleiotropic effects of TGF-b1 are conferred by crosstalks to other signal transduction pathways such as the MAP-kinases or the STAT-pathway. Here we describe the effect of long-term exposure to TGF-b1 on the effector function of differentially stimulated primary murine splenocytes and purified primary murine CD8+ cytotoxic T cells. Long-term exposure to TGF-b1 results in non-responsiveness to TGF-b1- induced Smad2 phosphorylation. This is seen either by no phosphorylation or sustained phosphorylation of Smad2. Furthermore, we observed a strong correlation between sustained Smad2 phosphorylation and resistance to TGF-b1 mediated growth inhibition. In contrast, splenocyte cultures strongly growth inhibited by TGF-b1 showed no Smad2 phosphorylation. Lytic activity of these cultures, however, was found to be suppressed regardless of proliferation properties and Smad2 phosphorylation pattern. We also describe that a functional MEK-1 pathway is a prerequisite for rendering murine splenocytes unresponsive to TGF-b1 mediated growth inhibition, and that inhibition of the MEK-1 cascade alters the Smad2 phosphorylation pattern. In addition, we show that resistance to TGF-b1 mediated growth inhibition correlates with the activation of the JNK pathway. However, the resistant phenotype was found unable to be reverted upon administration of exogeneous IFNg and/or aCD28 antibody. In human or mouse T cell lines, however, the described correlation between the type of stimulation and TGF-b growth resistance or growth sensitivity is not present. Thus, this correlation is specific for primary T cells. We also cloned a chimeric dominantnegative TGF-b receptor which is coupled to a suicide gene, in order to render T cells resistant to TGF-b mediated effects.These findings shed light on how TGF-b1 mediates its immunosuppressive role, and may help to gain knowledge of averting these TGF-b1 effects in the course of tumor therapy. KW - T-Lymphozyt KW - Transforming Growth Factor beta 1 KW - Signaltransduktion KW - T-Zellen KW - TGF-beta KW - Signaltransduktion KW - Smad KW - T-cells KW - TGF-beta KW - Signal transduction KW - Smad Y1 - 2002 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-4912 ER - TY - JOUR A1 - Feldbauer, Katrin A1 - Schlegel, Jan A1 - Weissbecker, Juliane A1 - Sauer, Frank A1 - Wood, Phillip G. A1 - Bamberg, Ernst A1 - Terpitz, Ulrich T1 - Optochemokine Tandem for Light-Control of Intracellular Ca\(^{2+}\) JF - PLoS ONE N2 - An optochemokine tandem was developed to control the release of calcium from endosomes into the cytosol by light and to analyze the internalization kinetics of G-protein coupled receptors (GPCRs) by electrophysiology. A previously constructed rhodopsin tandem was re-engineered to combine the light-gated Ca\(^{2+}\)-permeable cation channel Channelrhodopsin-2(L132C), CatCh, with the chemokine receptor CXCR4 in a functional tandem protein tCXCR4/CatCh. The GPCR was used as a shuttle protein to displace CatCh from the plasma membrane into intracellular areas. As shown by patch-clamp measurements and confocal laser scanning microscopy, heterologously expressed tCXCR4/CatCh was internalized via the endocytic SDF1/CXCR4 signaling pathway. The kinetics of internalization could be followed electrophysiologically via the amplitude of the CatCh signal. The light-induced release of Ca\(^{2+}\) by tandem endosomes into the cytosol via CatCh was visualized using the Ca\(^{2+}\)-sensitive dyes rhod2 and rhod2-AM showing an increase of intracellular Ca\(^{2+}\) in response to light. KW - capacitance KW - endosomes KW - cell membranes KW - membrane proteins KW - intracellular membranes KW - vesicles KW - confocal laser microscopy KW - cytosol Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-178921 VL - 11 IS - 10 ER - TY - JOUR A1 - Fazeli, Gholamreza A1 - Beer, Katharina B. A1 - Geisenhof, Michaela A1 - Tröger, Sarah A1 - König, Julia A1 - Müller-Reichert, Thomas A1 - Wehman, Ann M. T1 - Loss of the Major Phosphatidylserine or Phosphatidylethanolamine Flippases Differentially Affect Phagocytosis JF - Frontiers in Cell and Developmental Biology N2 - The lipids phosphatidylserine (PtdSer) and phosphatidylethanolamine (PtdEth) are normally asymmetrically localized to the cytosolic face of membrane bilayers, but can both be externalized during diverse biological processes, including cell division, cell fusion, and cell death. Externalized lipids in the plasma membrane are recognized by lipid-binding proteins to regulate the clearance of cell corpses and other cell debris. However, it is unclear whether PtdSer and PtdEth contribute in similar or distinct ways to these processes. We discovered that disruption of the lipid flippases that maintain PtdSer or PtdEth asymmetry in the plasma membrane have opposite effects on phagocytosis in Caenorhabditis elegans embryos. Constitutive PtdSer externalization caused by disruption of the major PtdSer flippase TAT-1 led to increased phagocytosis of cell debris, sometimes leading to two cells engulfing the same debris. In contrast, PtdEth externalization caused by depletion of the major PtdEth flippase TAT-5 or its activator PAD-1 disrupted phagocytosis. These data suggest that PtdSer and PtdEth externalization have opposite effects on phagocytosis. Furthermore, externalizing PtdEth is associated with increased extracellular vesicle release, and we present evidence that the extent of extracellular vesicle accumulation correlates with the extent of phagocytic defects. Thus, a general loss of lipid asymmetry can have opposing impacts through different lipid subtypes simultaneously exerting disparate effects. KW - phagocytosis KW - lipid asymmetry KW - flippase KW - phosphatidylserine KW - phosphatidylethanolamine KW - extracellular vesicle Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-208771 SN - 2296-634X VL - 8 ER - TY - JOUR A1 - Fathy, Moustafa A1 - Saad Eldin, Sahar M. A1 - Naseem, Muhammad A1 - Dandekar, Thomas A1 - Othman, Eman M. T1 - Cytokinins: wide-spread signaling hormones from plants to humans with high medical potential JF - Nutrients N2 - Nature is a rich source of biologically active novel compounds. Sixty years ago, the plant hormones cytokinins were first discovered. These play a major role in cell division and cell differentiation. They affect organogenesis in plant tissue cultures and contribute to many other physiological and developmental processes in plants. Consequently, the effect of cytokinins on mammalian cells has caught the attention of researchers. Many reports on the contribution and potential of cytokinins in the therapy of different human diseases and pathophysiological conditions have been published and are reviewed here. We compare cytokinin effects and pathways in plants and mammalian systems and highlight the most important biological activities. We present the strong profile of the biological actions of cytokinins and their possible therapeutic applications. KW - cytokinins KW - phytohormones KW - biological activities KW - plant system KW - mammalian system Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-271017 SN - 2072-6643 VL - 14 IS - 7 ER - TY - JOUR A1 - Fathy, Moustafa A1 - Okabe, Motonori A1 - Othman, Eman M. A1 - Saad Eldien, Heba M. A1 - Yoshida, Toshiko T1 - Preconditioning of adipose-derived mesenchymal stem-like cells with eugenol potentiates their migration and proliferation in vitro and therapeutic abilities in rat hepatic fibrosis JF - Molecules N2 - Mesenchymal stem cells (MSCs) have considerable therapeutic abilities in various disorders, including hepatic fibrosis. They may be affected with different culture conditions. This study investigated, on molecular basics, the effect of pretreatment with eugenol on the characteristics of adipose tissue-derived MSCs (ASCs) in vitro and the implication of eugenol preconditioning on the in vivo therapeutic abilities of ASCs against CCl\(_4\)-induced hepatic fibrosis in rats. The effect of eugenol on ASCs was assessed using viability, scratch migration and sphere formation assays. Expressions of genes and proteins were estimated by immunofluorescence or qRT-PCR. For the in vivo investigations, rats were divided into four groups: the normal control group, fibrotic (CCl\(_4\)) group, CCl\(_4\)+ASCs group and CCl\(_4\) + eugenol-preconditioned ASCs (CCl\(_4\)+E-ASCs) group. Eugenol affected the viability of ASCs in a concentration- and time-dependent manner. Eugenol improved their self-renewal, proliferation and migration abilities and significantly increased their expression of c-Met, reduced expression 1 (Rex1), octamer-binding transcription factor 4 (Oct4) and nanog genes. Furthermore, E-ASCs showed more of a homing ability than ASCs and improved the serum levels of ALT, AST, albumin, total bilirubin and hyaluronic acid more efficient than ASCs in treating CCl\(_4\)-induced hepatic fibrosis, which was confirmed with histopathology. More interestingly, compared to the CCl\(_4\)+ASCs group, CCl\(_4\)+E-ASCs group showed a lower expression of inducible nitric oxide synthase (iNOS), monocyte chemoattractant protein-1 (MCP-1), cluster of differentiation 163 (CD163) and tumor necrosis factor-α (TNF-α) genes and higher expression of matrix metalloproteinase (MMP)-9 and MMP-13 genes. This study, for the first time, revealed that eugenol significantly improved the self-renewal, migration and proliferation characteristics of ASCs, in vitro. In addition, we demonstrated that eugenol-preconditioning significantly enhanced the therapeutic abilities of the injected ASCs against CCl\(_4\)-induced hepatic fibrosis. KW - adipose tissue-derived MSCs KW - eugenol KW - migration KW - self-renewal KW - hepatic fibrosis KW - CCl\(_4\) Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-203662 SN - 1420-3049 VL - 25 IS - 9 ER - TY - JOUR A1 - Fathy, Moustafa A1 - Fawzy, Michael Atef A1 - Hintzsche, Henning A1 - Nikaido, Toshio A1 - Dandekar, Thomas A1 - Othman, Eman M. T1 - Eugenol exerts apoptotic effect and modulates the sensitivity of HeLa cells to cisplatin and radiation JF - Molecules N2 - Eugenol is a phytochemical present in different plant products, e.g., clove oil. Traditionally, it is used against a number of different disorders and it was suggested to have anticancer activity. In this study, the activity of eugenol was evaluated in a human cervical cancer (HeLa) cell line and cell proliferation was examined after treatment with various concentrations of eugenol and different treatment durations. Cytotoxicity was tested using lactate dehydrogenase (LDH) enzyme leakage. In order to assess eugenol’s potential to act synergistically with chemotherapy and radiotherapy, cell survival was calculated after eugenol treatment in combination with cisplatin and X-rays. To elucidate its mechanism of action, caspase-3 activity was analyzed and the expression of various genes and proteins was checked by RT-PCR and western blot analyses. Eugenol clearly decreased the proliferation rate and increased LDH release in a concentration- and time-dependent manner. It showed synergistic effects with cisplatin and X-rays. Eugenol increased caspase-3 activity and the expression of Bax, cytochrome c (Cyt-c), caspase-3, and caspase-9 and decreased the expression of B-cell lymphoma (Bcl)-2, cyclooxygenase-2 (Cox-2), and interleukin-1 beta (IL-1β) indicating that eugenol mainly induced cell death by apoptosis. In conclusion, eugenol showed antiproliferative and cytotoxic effects via apoptosis and also synergism with cisplatin and ionizing radiation in the human cervical cancer cell line. KW - eugenol KW - HeLa cells KW - cisplatin KW - radiation KW - apoptosis Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-193227 SN - 1420-3049 VL - 24 IS - 21 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 - THES A1 - Fasemore, Akinyemi Mandela T1 - Genomic and internet based analysis of \(Coxiella\) \(burnetii\) T1 - Genomische und Internet-basierte Analyse von \(Coxiella\) \(burnetii\) N2 - Coxiella burnetii, a Gram negative obligate intracellular bacterium, is the causative agent of Q fever. It has a world wide distribution and has been documented to be capable of causing infections in several domestic animals, livestock species, and human beings. Outbreaks of Q fever are still being observed in livestock across animal farms in Europe, and primary transmission to humans still oc- curs especially in animal handlers. Public health authorities in some countries like Germany are required by law to report human acute cases denoting the significance of the challenge posed by C. burnetii to public health. In this thesis, I have developed a platform alongside methods to address the challenges of genomic analyses of C. burnetii for typing purposes. Identification of C. burnetii isolates is an important task in the laboratory as well as in the clinics and genotyping is a reliable method to identify and characterize known and novel isolates. Therefore, I designed and implemented several methods to facilitate the genotyping analyses of C. burnetii genomes in silico via a web platform. As genotyping is a data intensive process, I also included additional features such as visualization methods and databases for interpretation and storage of obtained results. I also developed a method to profile the resistome of C. burnetii isolates using a machine learning approach. Data about antibiotic resistance in C. burnetii are scarce majorly due to its lifestyle and the difficulty of cultivation in laboratory media. Alternative methods that rely on homology identification of resistance genes are also inefficient in C. burnetii, hence, I opted for a novel approach that has been shown to be promising in other bacteria species. The applied method relied on an artificial neural network as well as amino acid composition of position specific scoring matrix profile for feature extraction. The resulting model achieved an accuracy of ≈ 0.96 on test data and the overall performance was significantly higher in comparison to existing models. Finally, I analyzed two new C. burnetii isolates obtained from an outbreak in Germany, I compared the genome to the RSA 493 reference isolate and found extensive deletions across the genome landscape. This work has provided a new digital infrastructure to analyze and character- ize C. burnetii genomes that was not in existence before and it has also made a significant contribution to the existing information about antibiotic resistance genes in C. burnetii. N2 - Coxiella burnetii, ein Gram-negatives, obligat intrazelluläres Bakterium, ist der Erreger des Q-Fiebers. Er hat eine weltweite Verbreitung und ist nachweis- lich in der Lage, Infektionen bei verschiedenen Haustieren, Nutztieren und Menschen zu verursachen. Ausbrüche von Q-Fieber werden immer noch in Tierbeständen in Europa beobachtet, und die Primärübertragung auf den Men- schen erfolgt nach wie vor allem durch Kontakt mit entsprechenden Tieren und ihren Ausscheidungen. Das öffentliche Gesundheitssystem in einigen Ländern wie Deutschland hat eine Meldepflicht für akute Fälle beim Menschen festge- legt, was die Bedeutung des Erregers bzw. seiner ausgelösten Erkrankung für die öffentliche Gesundheit verdeutlicht. In dieser Doktorarbeit habe ich eine Plattform neben weiteren Methoden entwickelt, um die Herausforderungen der Genomanalyse von C. burnetii für Genotypisierungsverfahren zu adressieren. Die Identifizierung von C. burnetii-Isolaten erfüllt eine wichtige Funktion im La- bor sowie in den Krankenhäusern, und die Genotypisierung ist eine verlässliche Methode, um bekannte und neue Isolate zu identifizieren und zu charakte- risieren. Daher habe ich mehrere Methoden konzipiert und implementiert, um die Analyse zur Genotypisierung von C. burnetii-Genomen in silico über eine Web-Plattform zu erleichtern. Da die Genotypisierung ein datenintensiver Prozess ist, habe ich ebenfalls zusätzliche Features wie Visualisierungsme- thoden und Datenbanken zur Interpretation und Speicherung der erhaltenen Ergebnisse mitaufgenommen. Ferner habe ich eine Methode zur Erstellung des Resistomprofils von C. burnetii-Isolaten unter Verwendung eines Ansat- zes des maschinellen Lernens entwickelt. Daten über Resistenzfaktoren bei C. burnetii sind rar, was hauptsächlich auf die obligat intrazelluläre Lebensweise der Coxiellen und die Schwierigkeiten bei der Kultivierung in Labormedien zurückzuführen ist. Alternative Methoden, die auf der Identifizierung der Ho- mologie von Resistenzgenen basieren, sind bei C. burnetii ebenfalls ineffizient. Aus diesem Grund entschied ich mich für einen neuen Ansatz, der sich bereits bei anderen Bakterienspezies als vielversprechend erwiesen hat. Die verwen- dete Methode basiert auf einem artifiziellen neuronalen Netzwerk sowie auf der Aminosäurezusammensetzung des positionsspezifischen Matrixprofils zur Extraktion von Features. Das daraus resultierende Modell erzielte eine Genauig- keit von ≈ 0,96 bei den Testdaten und die Gesamtleistung war signifikant höher im Vergleich zu den bereits vorhandenen Methoden. Schließlich analysierte ich zwei neue C. burnetii-Isolate, die von einem Q-Fieberausbruch in Deutschland stammten. Ich verglich das Genom mit dem RSA 493 Referenz Isolat und fand extensive Deletionen über das Genom sequenz. Mit dieser Arbeit wird eine neue digitale Infrastruktur zu Analyse von C. burnetii- Genomen bereitgestellt, die es vorher noch nicht gab. Zudem liefert diese Arbeit einen wichtigen Beitrag zu den bereits vorhandenen Informationen über Antibiotikaresistenzgene bei in C. burnetii. KW - Bioinformatics KW - Coxiella burnetii KW - Genotyping KW - Web services KW - Genomics Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-296639 ER - TY - JOUR A1 - Falibene, Augustine A1 - Roces, Flavio A1 - Rössler, Wolfgang A1 - Groh, Claudia T1 - Daily Thermal Fluctuations Experienced by Pupae via Rhythmic Nursing Behavior Increase Numbers of Mushroom Body Microglomeruli in the Adult Ant Brain JF - Frontiers in Behavioral Neuroscience N2 - Social insects control brood development by using different thermoregulatory strategies. Camponotus mus ants expose their brood to daily temperature fluctuations by translocating them inside the nest following a circadian rhythm of thermal preferences. At the middle of the photophase brood is moved to locations at 30.8°C; 8 h later, during the night, the brood is transferred back to locations at 27.5°C. We investigated whether daily thermal fluctuations experienced by developing pupae affect the neuroarchitecture in the adult brain, in particular in sensory input regions of the mushroom bodies (MB calyces). The complexity of synaptic microcircuits was estimated by quantifying MB-calyx volumes together with densities of presynaptic boutons of microglomeruli (MG) in the olfactory lip and visual collar regions. We compared young adult workers that were reared either under controlled daily thermal fluctuations of different amplitudes, or at different constant temperatures. Thermal regimes significantly affected the large (non-dense) olfactory lip region of the adult MB calyx, while changes in the dense lip and the visual collar were less evident. Thermal fluctuations mimicking the amplitudes of natural temperature fluctuations via circadian rhythmic translocation of pupae by nurses (amplitude 3.3°C) lead to higher numbers of MG in the MB calyces compared to those in pupae reared at smaller or larger thermal amplitudes (0.0, 1.5, 9.6°C), or at constant temperatures (25.4, 35.0°C). We conclude that rhythmic control of brood temperature by nursing ants optimizes brain development by increasing MG densities and numbers in specific brain areas. Resulting differences in synaptic microcircuits are expected to affect sensory processing and learning abilities in adult ants, and may also promote interindividual behavioral variability within colonies. KW - microglomeruli KW - temperature KW - broodtranslocation KW - camponotus ants KW - olfaction KW - vision KW - synapticplasticity KW - mushroom body Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-146711 VL - 10 IS - 73 ER - TY - JOUR A1 - Falibene, Augustina A1 - Roces, Flavio A1 - Rössler, Wolfgang T1 - Long-term avoidance memory formation is associated with a transient increase in mushroom body synaptic complexes in leaf-cutting ants JF - Frontiers in Behavioural Neuroscience N2 - Long-term behavioral changes related to learning and experience have been shown to be associated with structural remodeling in the brain. Leaf-cutting ants learn to avoid previously preferred plants after they have proved harmful for their symbiotic fungus, a process that involves long-term olfactory memory. We studied the dynamics of brain microarchitectural changes after long-term olfactory memory formation following avoidance learning in Acromyrmex ambiguus. After performing experiments to control for possible neuronal changes related to age and body size, we quantified synaptic complexes (microglomeruli, MG) in olfactory regions of the mushroom bodies (MB) at different times after learning. Long-term avoidance memory formation was associated with a transient change in MG densities. Two days after learning, MG density was higher than before learning. At days 4 and 15 after learning when ants still showed plant avoidance MG densities had decreased to the initial state. The structural reorganization of MG triggered by long-term avoidance memory formation clearly differed from changes promoted by pure exposure to and collection of novel plants with distinct odors. Sensory exposure by the simultaneous collection of several, instead of one, non-harmful plant species resulted in a decrease in MG densities in the olfactory lip. We hypothesize that while sensory exposure leads to MG pruning in the MB olfactory lip, the formation of long-term avoidance memory involves an initial growth of new MG followed by subsequent pruning. KW - Acromyrmex ambiguus KW - leaf-cutting ants KW - avoidance learning KW - olfaction KW - honeybee KW - microglomeruli KW - mushroom body KW - synaptic plasticity Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-148763 VL - 9 IS - 84 ER - TY - JOUR A1 - Falibene, Agustina A1 - Roces, Flavio A1 - Rössler, Wolfgang T1 - Long-term avoidance memory formation is associated with a transient increase in mushroom body synaptic complexes in leaf-cutting ants JF - Frontiers in Behavioral Neuroscience N2 - Long-term behavioral changes related to learning and experience have been shown to be associated with structural remodeling in the brain. Leaf-cutting ants learn to avoid previously preferred plants after they have proved harmful for their symbiotic fungus, a process that involves long-term olfactory memory. We studied the dynamics of brain microarchitectural changes after long-term olfactory memory formation following avoidance learning in Acromyrmex ambiguus. After performing experiments to control for possible neuronal changes related to age and body size, we quantified synaptic complexes (microglomeruli, MG) in olfactory regions of the mushroom bodies (MBs) at different times after learning. Long-term avoidance memory formation was associated with a transient change in MG densities. Two days after learning, MG density was higher than before learning. At days 4 and 15 after learning—when ants still showed plant avoidance—MG densities had decreased to the initial state. The structural reorganization of MG triggered by long-term avoidance memory formation clearly differed from changes promoted by pure exposure to and collection of novel plants with distinct odors. Sensory exposure by the simultaneous collection of several, instead of one, non-harmful plant species resulted in a decrease in MG densities in the olfactory lip. We hypothesize that while sensory exposure leads to MG pruning in the MB olfactory lip, the formation of long-term avoidance memory involves an initial growth of new MG followed by subsequent pruning. KW - microglomeruli KW - olfaction KW - avoidance learning KW - leaf-cutting ants KW - acromyrmex ambiguus KW - synaptic plasticity KW - mushroom body Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-125522 VL - 9 IS - 84 ER - TY - THES A1 - Fadl El Mola, Faisal Mohamed T1 - Bioinformatic and molecular approaches for the analysis of the retinal pigment epithelium (RPE) transcriptome N2 - There is substantial interest in the identification of genes underlying susceptibility to complex human diseases because of the potential utility of such genes in disease prediction and therapy. The complex age-related macular degeneration (AMD) is a prevalent cause of legal blindness in industrialized countries and predominantly affects the elderly population over 75 years of age. Although vision loss in AMD results from photoreceptor cell death in the central retina, the initial pathogenesis likely involves processes in the retinal pigment epithelium (RPE) (Liang and Godley, 2003). The goal of the current study was to identify and characterize genes specifically or abundantly expressed in the RPE in order to determine more comprehensively the transcriptome of the RPE. In addition, our aim was to assess the role of these genes in AMD pathogenesis. Towards this end, a bovine cDNA library enriched for RPE transcripts was constructed in-house using a PCR-based suppression subtractive hybridization (SSH) technique (Diatchenko et al., 1996, 1999), which normalizes for sequence abundance and achieves high enrichment for differentially expressed genes. CAP3 (Huang and Madan, 1999) was used to assemble the high quality sequences of all the 2379 ESTs into clusters or singletons. 1.2% of the 2379 RPE-ESTs contains vector sequences and was excluded from further analysis. 5% of the RPE-ESTs showed homology to multipe chromosomes and were not included in further assembly process. The rest of the ESTs (2245) were assembled into 175 contigs and 509 singletons, which revealed approximately 684 unique genes in the dataset. Out of the 684, 343 bovine RPE transcripts did not align to their human orthologues. A large fraction of clones were shown to include a considerable 3´untranslated regions of the gene that are not conserved between bovine and human. It is the coding regions that can be conserved between bovine and human and not the 3’ UTR (Sharma et al., 2002). Therefore, more sequencing from the cDNA library with reclustering of those 343 ESTs together with continuous blasting might reveal their human orthologoues. To handle the large volume of data that the RPE cDNA library project has generated a highly efficient and user-friendly RDBMS was designed. Using RDBMS data storage can be managed efficiently and flexibly. The RDBMS allows displaying the results in query-based form and report format with additional annotations, links and search functions. Out of the 341 known and predicted genes identified in this study, 2 were further analyzed. The RPE or/and retina specificity of these two clones were further confirmed by RT-PCR analysis in adult human tissues. Construction of a single nucleotide polymphism (SNP) map was initiated as a first step in future case/control association studies. SNP genotyping was carried out for one of these two clones (RPE01-D2, now known as RDH12). 12 SNPs were identified from direct sequencing of the 23.4-kb region, of which 5 are of high frequency. In a next step, comparison of allele frequencies between AMD patients and healthy controls is required. Completion of the expression analysis for other predicted genes identified during this study is in progress using real time RT-PCR and will provide additional candidate genes for further analyses. This study is expected to contribute to our understanding of the genetic basis of RPE function and to clarify the role of the RPE-expressed genes in the predisposition to AMD. It may also help reveal the mechanisms and pathways that are involved in the development of AMD or other retinal dystrophies. N2 - Es besteht ein grosses medizinisches Interesse an der Identifizierung von Genen, welche an der Entstehung komplexer, häufiger Krankheiten des Menschen beteiligt sind. Eine solche Krankheit ist die alters-korrelierte Makuladegeneration (AMD). Die AMD ist eine der häufigsten Ursachen für den Verlust der Sehfähigkeit im Alter von über 75 Jahren. Obwohl die Erblindung bei der AMD letztlich durch das Absterben von Photorezeptor-Zellen in der zentralen Retina bedingt wird, gibt es genügend Hinweise dafür, dass die Pathogenese der AMD ihren Ausgang vom retinalen Pigmentepithel (RPE) nimmt (Liang and Godley, 2003). Ziel dieser Arbeit war die Identifizierung und Charakterisierung von RPE-spezifischen Genen als Beitrag zur umfassenden Charakterisierung des RPE-Transkriptoms. Darüberhinaus war es Ziel der Arbeit, die mögliche Rolle der RPE-spezifischen Gene bei der Entstehung der AMD zu explorieren. Ausgangspunkt der Arbeit war eine RPE-spezifische, bovine cDNA Bibliothek, welche in der Arbeitsgruppe auf der Grundlage der SSH-Technik (Diatchenko et al, 1996, 1999) hergestellt worden war. Die SSH-Technik gestattet die Anreicherung von differentiell exprimierten Genen bei gleichzeitiger Normalisierung redundanter Sequenzen. Mit Hilfe des Software-Programms CAP3 (Huang and Madan, 1999) wurden insgesamt 2379 ESTs gruppiert und geordnet. 1,2% der 2379 RPE-ESTs enthielten Vektor Sequenzen und wurden daher von der weiteren Analyse ausgeschlossen. 5% der RPE-ESTs wiesen Homologien zu multiplen Chromosomen auf und wurden daher ebenfalls von der weiteren Analyse ausgeschlossen. Die übrigen 2245 ESTs wurden in 175 Contigs und 509 Singletons gruppiert, woraus sich Hinweise auf insgesamt 684 putative Einzelgene ergaben. 343 dieser 684 Klone zeigten jedoch keine Homologien zu humanen orthologen Sequenzen. Ursache für die fehlende Homologie muss in der grossen Zahl der Klone gesehen werden, bei welchen nur die 3´untranslatierten verglichen wurden. Im Gegensatz zu den kodierenden Sequenzabschnitten kommt es in den nicht-kodierenden Regionen in der Regel zu einer relativ raschen evolutionären Divergenz und damit zum Verlust der Homologie (Sharma et al, 2002). Durch zusätzliche Sequenzierung und Sequenzvergleiche der kodierenden Bereiche dieser 343 Klone lassen sich möglicherweise weitere RPE-spezifische Gene finden. Um die grosse Anzahl der im Rahmen des RPE-Projektes generierten Daten bearbeiten zu können wurde eine sehr effiziente und Benutzer-freundliche Datenbank auf Grundlage des RDBMS-Moduls etabliert. Dieses System gestattet die interaktive Bearbeitung der gespeicherten Daten im Query-Format. Darüberhinaus können die Daten in beliebiger Weise annotiert und verbunden werden. Nach Abzug der 343 nicht-homologen cDNA Klone von den 684 putativen Einzelsequenzen verblieben 341 Kandidaten-Sequenzen. 2 dieser Sequenzen wurden als putative neue RPE-spezifische Gene einer weiteren Analyse zugeführt. Dabei wurde zunächst die RPE- bzw. Retina-Spezifität dieser Kandidaten-Sequenzen mit Hilfe der RT-PCR Analyse bestätigt. Als Basis für zukünftige Fall-Kontroll- und Assoziationsstudien wurde eine SNP-Genotypisierung eines dieser zwei Klone (ursprüngliche Bezeichnung: RPE01-D2; derzeitige Bezeichnung: RDH12) durchgeführt. Die direkte Sequenzanalyse umfasste 23.4 kb und ergab insgesamt 12 SNPs, von denen sich 5 als hoch-informativ erwiesen. Auf dieser Grundlage können zukünftig Allel-Frequenzen zwischen Kontrollpersonen und AMD-Patienten ermittelt und verglichen werden. Zukünftig werden darüberhinaus real-time PCR Methoden zur Expressionsanalyse der verbliebenen Kandidaten-Klone eingesetzt. Zusammenfassend liefert die vorliegende Arbeit einen Beitrag zum Verständnis der genetischen Grundlagen der RPE-Funktionen und trägt zur Aufklärung der Rolle von RPE-spezifischen Genen bei der Disposition zur AMD bei. Zusätzlich ergaben sich Hinweise auf Kandidatengene, welche möglicherweise in der Pathogenese der AMD eine Rolle spielen. KW - Senile Makuladegeneration KW - Netzhaut KW - Pigmentepithel KW - Molekulargenetik KW - RPE KW - Bioinformatics KW - Age-related macular degeneration KW - Molecular approaches Y1 - 2003 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-6877 ER - TY - THES A1 - Fackler, Marc T1 - Biochemical characterization of GAS2L3, a target gene of the DREAM complex T1 - Biochemische Charakterisierung von GAS2L3, ein Zielgen des DREAM Komplex N2 - GAS2L3 was identified recently as a target gene of the DREAM complex (Reichert et al., 2010; Wolter et al., 2012). It was shown that GAS2L3 is expressed in a cell cycle specific manner and that depletion of the protein leads to defects in cytokinesis and genomic instability (Wolter et al., 2012). Major aim of this thesis was, to further characterize the biochemical properties and physiological function of GAS2L3. By in vitro co-sedimentation and bundling assays, GAS2L3 was identified as a cytoskeleton associated protein which bundles, binds and crosslinks F-actin and MTs. GST pulldown assays and co-immunoprecipitation experiments revealed that GAS2L3 interacts in vitro and in vivo with the chromosomal passenger complex (CPC), a very important regulator of mitosis and cytokinesis, and that the interaction is mediated by the GAR domain of GAS2L3 and the C-terminal part of Borealin and the N-terminal part of Survivin. Kinase assays showed that GAS2L3 is not a substrate of the CPC but is strongly phosphorylated by CDK1 in vitro. Depletion of GAS2L3 by shRNA influenced protein stability and activity of the CPC. However pharmacological studies showed that the decreased CPC activity is not responsible for the observed cytokinesis defects upon GAS2L3 depletion. Immunofluorescence experiments revealed that GAS2L3 is localized to the constriction zone by the CPC in a GAR dependent manner and that the GAR domain is important for proper protein function. New interacting proteins of GAS2L3 were identified by stable isotope labelling by amino acids in cell culture (SILAC) in combination with tandem affinity purification and subsequent mass spectrometrical analysis. Co-immunoprecipitation experiments further confirmed the obtained mass spectrometrical data. To address the physiological function of GAS2L3 in vivo, a conditional and a non-conditional knockout mouse strain was established. The non-conditional mouse strain showed a highly increased mortality rate before weaning age probably due to heart failure. The physiological function of GAS2L3 in vivo as well as the exact reason for the observed heart phenotype is not known at the moment. N2 - GAS2L3 wurde vor kurzem als Zielgen des DREAM Komplex identifiziert (Reichert et al., 2010; Wolter et al., 2012). Es konnte gezeigt werden, dass die Expression von GAS2L3 Zellzyklus abhängig reguliert wird und dass Depletion des Proteins zu Fehlern in der Zytokinese und genomischer Instabilität führt (Wolter et al., 2012). Hauptziel dieser Doktorarbeit war es, GAS2L3 hinsichtlich seiner biochemischen Eigenschaften und physiologischer Funktion näher zu charakterisieren. Unter Verwendung verschiedener in vitro Experimente konnte gezeigt werden, dass GAS2L3 sowohl F-Aktin als auch Mikrotubuli binden, bündeln und quervernetzen kann. In vitro und in vivo Protein-Protein Interaktionsexperimente zeigten, dass GAS2L3 mit dem „chromosomal passenger complex“ (CPC), einem wichtigen Mitose- und Zytokineseregulator, interagiert und dass diese Interaktion durch die GAR Domäne von GAS2L3 und den C-Terminus von Borealin beziehungsweise den N-terminus von Survivin vermittelt wird. Phosphorylierungsexperimente zeigten deutlich, dass GAS2L3 kein Substrat des CPC ist, jedoch von CDK1 phosphoryliert wird. Zellbiologische Experimente belegten, dass Depletion von GAS2L3 mittels shRNA die Proteinstabilität und Aktivität des CPC beeinflusst. Experimente mit einem chemischen Aurora B Inhibitor dokumentierten, dass die verringerte CPC Aktivität nicht die Ursache der beobachteten Zytokinesefehler nach GAS2L3 Depletion ist. Immunfluoreszenzexperimente machten deutlich, dass GAS2L3 mit Hilfe des CPC an der Abschnürungszone lokalisiert wird und dass die Lokalisation abhängig von der GAR Domäne erfolgt. Mit Hilfe von SILAC in Kombination mit Tandem-Affinitätsaufreinigung und anschließender massenspektrometrischer Auswertung wurden neue Proteininteraktoren von GAS2L3 identifiziert. Protein-Protein Interaktionsexperimente bestätigten die massenspektrometrisch ermittelten Daten. Um die physiologische Funktion von GAS2L3 in vivo näher analysieren zu können, wurden verschiedene Knockout Mauslinien etabliert. Die nicht-konditionelle Mauslinie zeigte erhöhte Sterblichkeit vor dem Absetzalter wahrscheinlich verursacht durch Herzversagen. Die genaue physiologische Funktion von GAS2L3 und der Grund für den beobachteten Herzphänotyp sind momentan noch unbekannt. KW - Zellzyklus KW - Zellteilung KW - Cytoskeleton Chromosomal Passenger Complex Interaction GAR Domain KW - Regulation KW - Molekulargenetik KW - GAS2L3 KW - Chromosomal Passenger Complex Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-103394 ER - TY - JOUR A1 - Ewald, Jan A1 - Bartl, Martin A1 - Dandekar, Thomas A1 - Kaleta, Christoph T1 - Optimality principles reveal a complex interplay of intermediate toxicity and kinetic efficiency in the regulation of prokaryotic metabolism JF - PLOS Computational Biology N2 - A precise and rapid adjustment of fluxes through metabolic pathways is crucial for organisms to prevail in changing environmental conditions. Based on this reasoning, many guiding principles that govern the evolution of metabolic networks and their regulation have been uncovered. To this end, methods from dynamic optimization are ideally suited since they allow to uncover optimality principles behind the regulation of metabolic networks. We used dynamic optimization to investigate the influence of toxic intermediates in connection with the efficiency of enzymes on the regulation of a linear metabolic pathway. Our results predict that transcriptional regulation favors the control of highly efficient enzymes with less toxic upstream intermediates to reduce accumulation of toxic downstream intermediates. We show that the derived optimality principles hold by the analysis of the interplay between intermediate toxicity and pathway regulation in the metabolic pathways of over 5000 sequenced prokaryotes. Moreover, using the lipopolysaccharide biosynthesis in Escherichia coli as an example, we show how knowledge about the relation of regulation, kinetic efficiency and intermediate toxicity can be used to identify drug targets, which control endogenous toxic metabolites and prevent microbial growth. Beyond prokaryotes, we discuss the potential of our findings for the development of antifungal drugs. KW - Enzyme regulation KW - Toxicity KW - Metabolic pathways KW - Enzymes KW - Transcriptional control KW - Enzyme kinetics KW - Enzyme metabolism KW - Predictive toxicology Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-180870 VL - 13 IS - 2 ER - TY - THES A1 - Esterlechner, Jasmina T1 - Role of the DREAM complex in mouse embryonic stem cells and identification of ZO-2 as a new LIN9 interacting protein T1 - Die Rolle des DREAM-Komplexes in embryonalen Stammzellen der Maus und Identifikation von ZO-2 als neues LIN9- interagierendes Protein N2 - The DREAM complex plays an important role in regulation of gene expression during the cell cycle. It was previously shown that the DREAM subunits LIN9 and B-MYB are required for early embryonic development and for the maintenance of the inner cell mass in vitro. In this work the effect of LIN9 or B-MYB depletion on embryonic stem cells (ESC) was examined. It demonstrates that LIN9 and B-MYB knock down changes the cell cycle distribution of ESCs and results in an accumulation of cells in G2 and M and in an increase of polyploid cells. By using genome-wide expression studies it was revealed that the depletion of LIN9 leads to downregulation of mitotic genes and to upregulation of differentiation-specific genes. ChIP-on chip experiments determined that mitotic genes are direct targets of LIN9 while lineage specific markers are regulated indirectly. Importantly, depletion of LIN9 does not alter the expression of the pluripotency markers Sox2 and Oct4 and LIN9 depleted ESCs retain alkaline phosphatase activity. I conclude that LIN9 is essential for proliferation and genome stability of ESCs by activating genes with important functions in mitosis and cytokinesis. The exact molecular mechanisms behind this gene activation are still unclear as no DREAM subunit features a catalytically active domain. It is assumed that DREAM interacts with other proteins or co-factors for transcriptional activation. This study discovered potential binding proteins by combining in vivo isotope labeling of proteins with mass spectrometry (MS) and further analysed the identified interaction of the tight junction protein ZO-2 with DREAM which is cell cycle dependent and strongest in S-phase. ZO-2 depletion results in reduced cell proliferation and decreased G1 gene expression. As no G2/M genes, typical DREAM targets, are affected upon ZO-2 knock down, it is unlikely that ZO-2 binding is needed for a functional DREAM complex. However, this work demonstrates that with (MS)-based quantitative proteomics, DREAM interacting proteins can be identified which might help to elucidate the mechanisms underlying DREAM mediated gene activation. N2 - Der DREAM Komplex spielt eine bedeutende Rolle in der Genregulation im Verlauf des Zellzyklus. Es wurde gezeigt, dass die DREAM Untereinheiten LIN9 und B-MYB für die frühe Embryogenese und den in vitro Erhalt der inneren Zellmasse erforderlich sind. In der vorligenden Arbeit wurde die Auswirkung von LIN9 und B-MYB Depletierung auf embryonale Stammzellen untersucht. Es zeigt sich, dass Depletion von LIN9 und B-MYB die Zellzyklus-Verteilung von embryonalen Stammzellen beeinflusst, zur Akkumulation der Zellen in G2 und M Phase und zu erhöhter Polyploidie führt. Genomweite Expressionsstudien ergaben, dass die Verringerung von LIN9 in der Runterregulierung von mitotischen und in der Hochregulierung von differenzierungsspezifischen Genen resultiert. ChIP-on-chip Experimente ermittelten, dass LIN9 Mitosegene als direkte Ziele hat, wohingegen entwicklungslinienspezifische Marker indirekt reguliert werden. Wesentlich ist, dass LIN9 Depletion nicht die Expression der Pluripotenzgene Oct4 oder Sox2 beeinflusst und embryonale Stammzellen ihre Alkaline Phosphatase Aktivität behalten. Daraus lässt schließen, dass LIN9 essentiell für die Proliferation und genomische Stabilität von embryonalen Stammzellen ist, in dem es Gene aktiviert, die wichtige Funktionen in Mitose und Zytokinese ausüben. Der exakte Mechanismus hinter der Genaktivierung ist noch nicht geklärt, da keine DREAM Untereinheit eine katalytisch aktive Domäne aufweist. Vermutlich ist die Interaktion mit weiteren Proteinen oder Co-Faktoren für die Genaktivierung vonnöten. Diese Studie entdeckte mit in vivo Isotop-Markierung von Proteinen und Massenspektrometrie (MS) potentielle Bindungspartner und untersuchte die identifizierte Bindung mit dem Tight Junction Protein ZO-2 genauer. Diese Bindung ist zellzyklus-abhängig und ist am stärksten während der S-Phase. ZO-2 Depletion führt zu reduzierter Zellproliferation und verringerter G1-Genexpression. Da keine G2/M Gene, typische DREAM Ziele, von einer ZO-2 Depletion beeinflusst werden, ist es unwahrscheinlich, dass die ZO-2 Bindung für einen funktionellen DREAM Komplex benötigt wird. Jedoch demonstriert diese Studie, dass mit (MS)-basierender, quantitativer Proteomik DREAM interagierende Proteine identifiziert werden können. Dies ist hilfreich um die Mechanismen hinter der DREAM vermittelten Genaktivierung aufzuklären. KW - Zellzyklus KW - cellcycle KW - Stammzelle KW - Maus KW - stem cells KW - DREAM KW - Genregulation Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-90440 ER - TY - THES A1 - Esch, Mandy T1 - Novel Nucleic Acid Sensors for the Rapid Detection of Cryptosporidium Parvum T1 - Neue Nukleinsäure-Sensoren für die Detektion von Cryptosporidium parvum N2 - Recent advances in the development of immunoassays and nucleic acid assays have improved the performance and increased the sensitivity of sensors that are based on biochemical recognition. The new approaches taken by researchers include detecting pathogens by detecting their nucleic acids, using new nontoxic reporter entities for generating signals, and downscaling and miniaturizing sensors to micromigration and microfluidic formats. This dissertation connects some of these successful approaches, thereby leading to the development of novel nucleic acid sensors for rapid and easy detection of pathogens. The author's goal was to develop diagnostic tools that enable investigators to detect pathogens rapidly and on site. While the sensors can be used to detect any pathogen, the author first customized them for detecting particularly Cryptosporidium parvum, a pathogen whose detection is important, yet presents many challenges. Chapter 2 of this thesis presents a novel test-strip for the detection of C. parvum. The test-strip is designed to detect nucleic acids rather than proteins or other epitopes. While test strips are commonly used for sensors based on immunological recognition, this format is very new in applications in which nucleic acids are detected. Further, to indicate the presence or absence of a specific target on the test strip, dye-entrapped, oligonucleotide-tagged liposomes are employed. Using liposomes as reporter particles has advantages over using other reporter labels, because the cavity that the phospholipidic membranes of the liposomes form can be filled with up to 106 dye molecules. By using heterobifunctional linkers liposomes can be tagged with oligonucleotides, thereby enabling their use in nucleic acid hybridization assays. The developed test-strip provides an internal control. The limit of detection is 2.7 fmol/mL with a sample volume of 30 mL. In chapter 3 the detection of nucleic acids by means of oligonucleotide-tagged liposomes is scaled down to a microfluidic assay format. Because the application of biosensors to microfluidic formats is very new in the field of analytical chemistry, the first part of this chapter is devoted to developing the design and the method to fabricate the microchip devices. The performance of the microchips is then optimized by investigating the interactions of nucleic acids and liposomes with the material the chips consist of and by passivating the surface of the chips with blocking reagents. The developed microfluidic chip enabled us to reduce the sample volume needed for one assay to 12.5 mL. The limit of detection of this assay was determined to be 0.4 fmol/mL. Chapters 4 and 5 expand on the development of the microfluidic assay. A prototype microfluidic array that is able to detect multiple analytes in a single sample simultaneously is developed. Using such an array will enable investigators to detect pathogens that occur in the same environment, for example, C. parvum and Giardia duodenalis by conducting a single test. The array's ability to perform multiple sample analysis is shown by detecting different concentrations of target nucleic acids. Further, the author developed a microfluidic chip in which interdigitated microelectrode arrays (IDAs) that consist of closely spaced microelectrodes are integrated. The IDAs facilitate electrochemical detection of cryptosporidial RNA. Electrochemical detection schemes offer benefits of technical simplicity, speed, and sensitivity. In this project liposomes are filled with electrochemically active molecules and are then utilized to generate electrochemical signals. Chapter 6 explores the feasibility of liposomes for enhancing signals derived from nucleic acid hybridization in surface plasmon resonance (SPR) spectroscopy. SPR spectroscopy offers advantages because nucleic acid hybridization can be monitored in real time and under homogeneous conditions because no washing steps are required. SPR spectroscopy is very sensitive and it can be expected that, in the future, SPR will be integrated into microfluidic nucleic acid sensors. N2 - Jüngste Fortschritte in der Entwicklung von Immuno- und Nucleinsäure- Assays haben die Arbeitsleistung und die Spezifität von Sensoren, die auf biochemischer Erkennung basieren (Biosensoren), verbessert. Neu entwickelte Methoden umfassen die Detektion von Pathogenen durch die Detektion ihrer RNA oder DNA, das Benutzen von neuen nicht-toxischen Reporter Molekülen, um Signale in Sensoren zu erzeugen, und die Verkleinerung und Miniaturisierung von Sensoren zu Mikromigrations- und Mikrofluid Formaten. Die in dieser Dissertation entwickelten Sensoren, die der Detektion von Pathogenen dienen, verbinden einige der neu entwickelten Methoden. Das Ziel der Autorin war es, Sensoren zu entwickeln, die es ermöglichen, Pathogene an Ort und Stelle zu detektieren. Die entwickelten Sensoren können zur Detektion von einer Reihe von Pathogenen benutzt werden. In dieser Dissertation sind sie für die spezifische Detektion von Cryptosporidium parvum entwickelte worden. Kapitel 2 der Dissertation präsentiert einen neuen Teststreifen für die Detektion von C. parvum. Der Teststreifen detektiert die RNA von C. parvum, die als Reaktion auf einen Hitzeschock produziert wird. Das Teststreifen-Format ist üblich für Sensoren, die auf immunologischer Erkennung basieren. Es ist jedoch neu für Anwendungen in denen RNA oder DNA detektiert werden sollen. Die An- oder Abwesenheit eines bestimmten Ziel Moleküls wird durch Liposomen, die Oligonukleotide auf der Aussenseite ihrer Membranen enthalten und mit Farbstoff gefüllt sind, angedeutet. Die Experimente zeigten, dass die mit dem entwickelten Test-Streifen kleinste detektierbare Konzentration von RNA in einem 30 mL Probenvolumen 2.7 fmol/mL ist. In Kapitel 3 ist die Signalerzeugung durch Liposomen in ein Mikrofliess-System integriert. Da die Entwicklung von Mikrofliess-Systemen ein sehr neues Forschungsgebiet ist, befasst sich ein Teil dieses Kapitels mit dem Design und der Herstellung des Microchips. Die Untersuchung von Interaktionen von Nukleinsäuren und Liposomen mit dem Material aus dem der Chip hergestellt ist und die Passivierung dieses Materials ist dabei ein Schwerpunkt. Das Probenvolumen, dass zur Detektion mit dem entwickelten Mikrofliess-Sensor nötig ist, konnte auf 12.5 mL reduziert werden. Die kleinste detektierbare Konzentration von Nucleinsäuren ist 5 fmol/mL. In Kapitel 4 und 5 erweitert die Autorin die Entwicklung des Mikrofliess-Sensors aus Kapitel 3. Das Detektionsformat ist auf ein Array, das für die gleichzeitige Detektion von mehreren Pathogenen benutzt werden kann, angewandt. Eine Methode zum Herstellen eines Arrays-Prototypen ist entwickelt. Ferner, stellte die Autorin verzahnte Mikroelektroden her und benutzte diese um die elektrochemische Detektion der RNA von C. parvum zu ermöglichen. In Kapitel 6 ist die Anwendbarkeit von Liposomen zur Erhöhung von Signalen von Nukleinsäure-Hybridisierungen in Surface Plasmon Resonance Spectroscopy (SPR) untersucht. KW - Cryptosporidium KW - RNS KW - Biosensor KW - Nucleinsäure-Sensoren KW - RNA KW - Cryptosporidium parvum KW - Mikrofliess-System KW - Liposomen KW - Teststreifen KW - Nuleic Acids Sensors KW - RNA KW - Cryptosporidium parvum KW - Microfluidic Chip KW - Liposomes KW - Test-Strip Y1 - 2001 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-323 ER - TY - THES A1 - Ernst, Raffael T1 - Anuran communities on the cutting edge : Analysing patterns and processes in anthropogenically altered tropical forests - Studies from the Guiana Shield and West Africa T1 - Anurengemeinschaften auf Messers Schneide: Muster und Prozesse in anthropogen veränderten tropischen Wäldern - Studien vom Guiana Schild und Westafrika N2 - Summary Timber harvesting is currently the most common commercial utilisation activity in tropical forests. Assessing the effects of logging on different aspects of biodiversity and general ecosystem properties is hence of prime importance if the few remaining areas of intact tropical forest are to be protected effectively and efficiently. Tropical amphibian communities are an appropriate model system for studies on the impacts of human-induced environmental changes on the dynamics of complex biological systems. This thesis elaborates on patterns of diversity changes in tropical forest amphibian communities facing habitat alterations associated with selective logging in two globally important eco-regions (Côte d’Ivoire, Upper Guinea, West Africa and Guyana, the Guiana Shield, northern South America). The thesis is organised along two main themes. After a general introduction, a section on general methodology and an introduction to the model systems studied, the first theme moves from general patterns to underlying processes. A second theme running through both chapters carries from undisturbed systems to disturbed systems. A final section integrates findings and addresses implications for conservation management of anthropogenically altered tropical forests. Several case studies at the species- population and community level are being presented and data on the direct and indirect impacts of anthropogenic habitat alteration on respective organizational levels are provided. A key statement that is stressed on throughout the studies is the fact that common measures of diversity, such as species richness and species-diversity only inadequately reflect processes of diversity change following anthropogenic disturbance. They also fail to describe actual impacts on the dynamics of complex biological systems. It is argued that commonly used measures produce an incoherent and insufficient picture of diversity patterns and the underlying processes that shape these patterns. Thus, an understanding of higher levels of diversity, such as β-diversity and functional diversity (and hence compositional patterns) appears to be the key to effectively mitigating the impacts of human-induced disturbance on amphibian communities. It is shown that the predictability of amphibian community composition depends on the respective level of anthropogenic disturbance imposed on a particular habitat. Hence, human activities that lead to changes in the structure of a forest, such as logging, not only alter simple system descriptors, such as the number of species in a given community, but rather alter the dynamics of the entire system. In this context, functional diversity is shown to be an important aspect underlying the actual mechanism that leads to the observed change of predictability patterns. Functional differences between species, rather than number of species per se appear to be the decisive factor in sustaining desirable ecosystem states and thus in maintaining important ecosystem services. Because biological diversity appears to play a substantial role in ecosystem resilience required to safeguard essential ecosystem functions in the face of environmental change, the thesis calls for a critical revision of common diversity assessments approaches. The studies advocate the reconsideration of the uncritical use of widespread measures and descriptors of biodiversity on grounds of inconsistent patterns found throughout numerous studies, including those presented herein. N2 - Zusammenfassung Forst- und Holzwirtschaft gehört derzeit zu einer der wichtigsten kommerziellen Nutzungsformen tropischer Wälder. Der Analyse und Untersuchung von direkten und indirekten Auswirkungen von Holzeinschlag auf verschiedene Aspekte biologischer Vielfalt und genereller Ökosystemeigenschaften muß daher eine zentrale Bedeutung eingeräumt werden. Dies trifft im besonderen Maße zu, wenn die verbleibenden noch intakten Regenwaldflächen effizient und auch langfristig effektiv geschützt werden sollen. Tropische Amphibiengemeinschaften haben sich bei der Untersuchung von Auswirkungen anthropogen induzierter Habitatveränderungen auf die Dynamik komplexer biologischer Systeme als geeignetes Modellsystem erwiesen. Die hier vorliegende Arbeit befasst sich mit den Mustern der Diversität und deren Änderung in tropischen Waldamphibiengemeinschaften unter dem Einfluss anthropogener Habitatveränderungen (selektiver Holzeinschlag) in zwei geographisch distinkten Ökoregionen von globaler Bedeutung (Côte d’Ivoire, Oberguinea, West Afrika und Guyana, Guiana Schild, nördliches Südamerika). Die thematische Gliederung der Arbeit folgt zwei unterschiedlichen Organisationssträngen. Der erste Strang leitet, nach einer allgemeinen Einführung und einem Abschnitt zur Methodik und Einführung in die untersuchten Modellsysteme, über, von den generellen Mustern zu den zugrunde liegenden Prozessen. Ein zweiter führt von ungestörten Systemen zu Systemen unter Störungseinfluss. Ein abschließender Abschnitt befasst sich mit den Implikationen für Naturschutzmanagement von anthropogen veränderten tropischen Wäldern. In einer Reihe von Fallstudien auf Art-, Populations- und Gemeinschaftsniveau werden die direkten und indirekten Einflüsse anthropogener Habitatänderungen auf die jeweilige Organisationsebene erörtert. Grundtenor aller vorgestellten Untersuchungen ist die Tatsache, dass herkömmliche Diversitätsmaße, wie etwa Artenreichtum und Artendiversität die in Zusammenhang mit anthropogenen Störungen auftretenden Veränderungen von Diversitätsmustern nur unzureichend erklären. Diese Maße erscheinen ebenfalls ungeeignet für die Beschreibung des Einflusses auf die Dynamik komplexer biologischer Systeme. Herkömmlich verwendete Diversitätsindizes generieren ein inkohärentes und unzureichendes Bild tatsächlicher Diversitätsmuster und der zugrunde liegenden Prozesse, die diese Muster formen. Das Verständnis höherer Ebenen der Diversität, wie etwa β-Diversität oder funktionale Diversität (und somit Muster der Artzusammensetzung) erscheint essentiell für die Minimierung des Einflusses von anthropogen induzierten Störungen auf Amphibiengemeinschaften und könnte somit zu einer effektiven Schadensbegrenzung beitragen. In den vorgestellten Untersuchungen konnte gezeigt werden, dass die Vorhersagbarkeit der Zusammensetzung einer gegebenen Amphibiengemeinschaft unmittelbar vom Störungsgrad des jeweiligen Systems abhängt. Menschliche Aktivitäten, die zu strukturellen Änderungen von Waldssystemen führen, wie etwa kommerzieller Holzeinschlag, führen nicht nur zu Änderungen einfacher Systemdeskriptoren, wie der Anzahl der Arten innerhalb einer Gemeinschaft, vielmehr beeinflussen sie die Dynamik des Gesamtsystems. In diesem Zusammenhang erwiesen sich funktionale Diversitätskomponenten als äußerst wichtige determinierende Faktoren für die beobachteten Vorhersagbarkeitsmuster und deren Veränderung. Funktionale Unterschiede und nicht Artenzahl per se scheinen demnach für den Erhalt zu bevorzugender Ökossystemzustände ausschlaggebend zu sein. Der Erhalt dieser funktionalen Merkmalsdiversität trägt unmittelbar zum Erhalt wichtiger ökosystemarer Leistungen bei. Da anzunehmen ist, dass biologischer Diversität eine maßgebliche Rolle in Bezug auf die Belastbarkeit und Elastizität von Ökosystemen zukommt (essentielle Eigenschaften, die das langfristige Funktionieren von Ökosystemen unter Störungseinfluss gewährleisten), unterstreichen die Ergebnisse der hier vorliegenden Arbeit die Notwendigkeit einer kritischen Revision traditioneller Ansätze der Diversitätserfassung. KW - Tropischer Regenwald KW - Westafrika KW - Lurche KW - Ökologie KW - anthropogene Störungen KW - Amphibiengemeinschaften KW - Vorhersagbarkeitsmuster KW - Naturschutz KW - Afro- Neotropen KW - anthropogenic disturbance KW - amphibian communities KW - predictabilitiy patterns KW - conservation KW - Afro- Neotropics Y1 - 2006 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-18373 ER - TY - JOUR A1 - Erbelding-Denk, Claudia A1 - Schroder, Johannes H. A1 - Schartl, Manfred A1 - Nanda, Indrajit A1 - Schmid, Michael A1 - Epplen, Jörg T. T1 - Male polymorphism in Limia perugiae (Pisces: Poeciliidae) N2 - The male-polymorphic poeciliid fish, Limia perugiae, a small teleostean endemic to the southeast of the Caribbean island Hispafiola, consists of three male size morphs with uniform females. Large males differentiate at a size va:rying between 25 and 38 mm; intermediate males, between 21 and 25 mm. Under competition, !arge males exhibit an elaborate courtship display, whereas small males show only a sneak-chase behavior. Intermediate males adapt their tactics to the respective competitors. However, all malemorphs can switch from courtship display to sneak-chase behavior. In large mating groups with four males of different size and five or six virgin females, large dominant a-males as weil as small subordinate \(\delta\)-males did not produce any offspring. Unexpectedly, all progeny were sired exclusively by the intemediate subordinate ß- and \(\gamma\)-males. Breeding experiments with the three male morphs can best be explained by a model of Y -linked genes for small and !arge size which are both suspended by the activity of an autosomal recessive repressor responsible for the development of intermediate males. The dominant allele of the recessive repressor, in either its homoorits heterozygous state, activates the Y-chromosomal genes for !arge or small size, respectively. Accordingly, intermediate males may produce male offspring of all size classes, depending on the presence of either the Y-linked gene or the autosomal repressor. KW - Physiologische Chemie KW - Poeciliid fish KW - male size polymorphism KW - reproductive success Y1 - 1994 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-61573 ER - TY - CHAP A1 - Epplen, J. T. A1 - Ammer, H. A1 - Epplen, C. A1 - Kammerbauer, C. A1 - Mitreiter, R. A1 - Roewer, L. A1 - Schwaiger, W. A1 - Steimle, V. A1 - Zischler, H. A1 - Albert, E. A1 - Andreas, A. A1 - Beyermann, B. A1 - Meyer, W. A1 - Buitkamp, J. A1 - Nanda, I. A1 - Nürnberg, P. A1 - Pena, S. D. J. A1 - Pöche, H. A1 - Sprecher, W. A1 - Schartl, Manfred A1 - Weising, K. A1 - Yassouridis, A. T1 - Oligonucleotide fingerprinting using simple repeat motifs: a convenient, ubiquitously applicable method to detect hypervariability for multiple purposes N2 - A panel of simple repetitive oligonucleotide probes has been designed and tested for multilocus DNA fingerprinting in some 200 fungal, plant and animal species as well as man. To date at least one of the probes has been found to be informative in each species. The human genome, however, has been the major target of many fingerprintins studies. Using the probe (CAC)5 or (GTG)5, individualization of all humans is possible except for monozygotic twins. Paternity analyses are now perfonned on a routine basis by the use of multilocus fingerprints, inctuding also cases of deficiency, i.e. where one of the parents is not available for analysis. In forensie science stain analysis is feasible in all tissue remains containing nuc)eated cells. Depending on the degree of DNA degradation a variety of oligonucleotides are informative, and they have been proven useful in actual case work. Advantages in comparison to other methods including enzymatic DNA amplification techniques (PCR) are evident. Fingerprint patterns of tumors may be changed due to the gain or loss of chromosomes and/or intrachromosomal deletion and amplification events. Locus-specific probes were isolated from the human (CAC)5/( GTG)5 fingerprint with a varying degree of informativeness (monomorphic versus truly hypervariable markers). The feasibility of three different approaches. for the isolation of hypervariable mono-locus probes was evaluated. Finally, one particular mixed simple (gt)n(ga)m repeat locus in the second intron of the HLA-DRB genes has been scrutinized to allow comparison of the extent of exon-encoded (protein-) polymorphisms versus intronie bypervariability of simple repeats: adjacent to a single gene sequence (e.g. HLA-DRB1*0401) many different length alleles were found. Group-specific structures of basic repeats were identified within the evolutionarily related DRB alleles. As a further application it is suggested here that due to the ubiquitous interspersion of their targets, short probes for simple repeat sequences are especially useful tools for ordering genomic cosmid, yeast artificial chromosome and phage banks. KW - DNS KW - Fingerprint-Verfahren Y1 - 1991 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-86371 ER - TY - JOUR A1 - Engstler, Markus A1 - Beneke, Tom T1 - Gene editing and scalable functional genomic screening in Leishmania species using the CRISPR/Cas9 cytosine base editor toolbox LeishBASEedit JF - eLife N2 - CRISPR/Cas9 gene editing has revolutionised loss-of-function experiments in Leishmania, the causative agent of leishmaniasis. As Leishmania lack a functional non-homologous DNA end joining pathway however, obtaining null mutants typically requires additional donor DNA, selection of drug resistance-associated edits or time-consuming isolation of clones. Genome-wide loss-of-function screens across different conditions and across multiple Leishmania species are therefore unfeasible at present. Here, we report a CRISPR/Cas9 cytosine base editor (CBE) toolbox that overcomes these limitations. We employed CBEs in Leishmania to introduce STOP codons by converting cytosine into thymine and created http://www.leishbaseedit.net/ for CBE primer design in kinetoplastids. Through reporter assays and by targeting single- and multi-copy genes in L. mexicana, L. major, L. donovani, and L. infantum, we demonstrate how this tool can efficiently generate functional null mutants by expressing just one single-guide RNA, reaching up to 100% editing rate in non-clonal populations. We then generated a Leishmania-optimised CBE and successfully targeted an essential gene in a plasmid library delivered loss-of-function screen in L. mexicana. Since our method does not require DNA double-strand breaks, homologous recombination, donor DNA, or isolation of clones, we believe that this enables for the first time functional genetic screens in Leishmania via delivery of plasmid libraries. KW - CRISPR/Cas9 KW - Leishmania KW - cytosine base editor (CBE) toolbox KW - gene editing KW - scalable functional genomic screening KW - LeishBASEedit Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-350002 VL - 12 ER - TY - JOUR A1 - Englmeier, Jana A1 - von Hoermann, Christian A1 - Rieker, Daniel A1 - Benbow, Marc Eric A1 - Benjamin, Caryl A1 - Fricke, Ute A1 - Ganuza, Cristina A1 - Haensel, Maria A1 - Lackner, Tomáš A1 - Mitesser, Oliver A1 - Redlich, Sarah A1 - Riebl, Rebekka A1 - Rojas-Botero, Sandra A1 - Rummler, Thomas A1 - Salamon, Jörg-Alfred A1 - Sommer, David A1 - Steffan-Dewenter, Ingolf A1 - Tobisch, Cynthia A1 - Uhler, Johannes A1 - Uphus, Lars A1 - Zhang, Jie A1 - Müller, Jörg T1 - Dung-visiting beetle diversity is mainly affected by land use, while community specialization is driven by climate JF - Ecology and Evolution N2 - Dung beetles are important actors in the self-regulation of ecosystems by driving nutrient cycling, bioturbation, and pest suppression. Urbanization and the sprawl of agricultural areas, however, destroy natural habitats and may threaten dung beetle diversity. In addition, climate change may cause shifts in geographical distribution and community composition. We used a space-for-time approach to test the effects of land use and climate on α-diversity, local community specialization (H\(_2\)′) on dung resources, and γ-diversity of dung-visiting beetles. For this, we used pitfall traps baited with four different dung types at 115 study sites, distributed over a spatial extent of 300 km × 300 km and 1000 m in elevation. Study sites were established in four local land-use types: forests, grasslands, arable sites, and settlements, embedded in near-natural, agricultural, or urban landscapes. Our results show that abundance and species density of dung-visiting beetles were negatively affected by agricultural land use at both spatial scales, whereas γ-diversity at the local scale was negatively affected by settlements and on a landscape scale equally by agricultural and urban land use. Increasing precipitation diminished dung-visiting beetle abundance, and higher temperatures reduced community specialization on dung types and γ-diversity. These results indicate that intensive land use and high temperatures may cause a loss in dung-visiting beetle diversity and alter community networks. A decrease in dung-visiting beetle diversity may disturb decomposition processes at both local and landscape scales and alter ecosystem functioning, which may lead to drastic ecological and economic damage. KW - coleoptera KW - coprophagous beetles KW - decomposition KW - global change KW - hill numbers KW - network analysis Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-312846 SN - 2045-7758 VL - 12 IS - 10 ER - TY - JOUR A1 - Englmeier, Jana A1 - Mitesser, Oliver A1 - Benbow, M. Eric A1 - Hothorn, Torsten A1 - von Hoermann, Christian A1 - Benjamin, Caryl A1 - Fricke, Ute A1 - Ganuza, Cristina A1 - Haensel, Maria A1 - Redlich, Sarah A1 - Riebl, Rebekka A1 - Rojas Botero, Sandra A1 - Rummler, Thomas A1 - Steffan-Dewenter, Ingolf A1 - Stengel, Elisa A1 - Tobisch, Cynthia A1 - Uhler, Johannes A1 - Uphus, Lars A1 - Zhang, Jie A1 - Müller, Jörg T1 - Diverse effects of climate, land use, and insects on dung and carrion decomposition JF - Ecosystems N2 - Land-use intensification and climate change threaten ecosystem functions. A fundamental, yet often overlooked, function is decomposition of necromass. The direct and indirect anthropogenic effects on decomposition, however, are poorly understood. We measured decomposition of two contrasting types of necromass, rat carrion and bison dung, on 179 study sites in Central Europe across an elevational climate gradient of 168–1122 m a.s.l. and within both local and regional land uses. Local land-use types included forest, grassland, arable fields, and settlements and were embedded in three regional land-use types (near-natural, agricultural, and urban). The effects of insects on decomposition were quantified by experimental exclusion, while controlling for removal by vertebrates. We used generalized additive mixed models to evaluate dung weight loss and carrion decay rate along elevation and across regional and local land-use types. We observed a unimodal relationship of dung decomposition with elevation, where greatest weight loss occurred between 600 and 700 m, but no effects of local temperature, land use, or insects. In contrast to dung, carrion decomposition was continuously faster with both increasing elevation and local temperature. Carrion reached the final decomposition stage six days earlier when insect access was allowed, and this did not depend on land-use effect. Our experiment identified different major drivers of decomposition on each necromass form. The results show that dung and carrion decomposition are rather robust to local and regional land use, but future climate change and decline of insects could alter decomposition processes and the self-regulation of ecosystems. KW - decay KW - ecosystem function KW - global change KW - land-use intensification KW - necrobiome KW - urbanization Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-325064 SN - 1432-9840 VL - 26 IS - 2 ER - TY - THES A1 - Englmeier, Jana T1 - Consequences of climate change and land-use intensification for decomposer communities and decomposition processes T1 - Folgen von Klimawandel und intensiver Landnutzung für Zersetzergemeinschaften und Abbauprozesse N2 - The increase in intensively used areas and climate change are direct and indirect consequences of anthropogenic actions, caused by a growing population and increasing greenhouse gas emissions. The number of research studies, investigating the effects of land use and climate change on ecosystems, including flora, fauna, and ecosystem services, is steadily growing. This thesis contributes to this research area by investigating land-use and climate effects on decomposer communities (arthropods and microbes) and the ecosystem service ‘decomposition of dead material’. Chapter II deals with consequences of intensified land use and climate change for the ecosystem service ‘decomposition of dead organic material’ (necromass). Considering the severe decline in insects, we experimentally excluded insects from half of the study objects. The decomposition of both dung and carrion was robust to land-use changes. Dung decomposition, moreover, was unaffected by temperature and the presence/ absence of insects. Along the altitudinal gradient, however, highest dung decomposition was observed at medium elevation between 600 and 700 m above sea level (although insignificant). As a consequence, we assume that at this elevation there is an ideal precipitation:temperature ratio for decomposing organisms, such as earthworms or collembolans. Carrion decomposition was accelerated by increasing elevation and by the presence of insects, indicating that increasing variability in climate and an ongoing decline in insects could modify decomposition processes and consequently natural nutrient cycles. Moreover, we show that different types of dead organic material respond differently to environmental factors and should be treated separately in future studies. In Chapter III, we investigated land-use and climate effects on dung-visiting beetles and their resource specialization. Here, all beetles that are preferentially found on dung, carrion or other rotten material were included. Both α- and γ-diversity were strongly reduced in agricultural and urban areas. High precipitation reduced dung-visiting beetle abundance, whereas γ-diversity was lowest in the warmest regions. Resource specialization decreased with increasing temperatures. The results give evidence that land use as well as climate can alter dung-visiting beetle diversity and resource specialization and may hence influence the natural balance of beetle communities and their contribution to the ecosystem service ‘decomposition of dead material’. The following chapter, Chapter IV, contributes to the findings in Chapter II. Here, carrion decomposition is not only explained by land-use intensity and climate but also by diversity and community composition of two taxonomic groups found on carrion, beetles and bacteria. The results revealed a strong correlation between bacteria diversity and community composition with temperature. Carrion decomposition was to a great extent directed by bacterial community composition and precipitation. The role of beetles was neglectable in carrion decomposition. With this study, I show that microbes, despite their microscopic size, direct carrion decomposition and may not be neglected in future decomposition studies. In Chapter V a third necromass type is investigated, namely deadwood. The aim was to assess climate and land-use effects on deadwood-inhabiting fungi and bacteria. Main driver for microbial richness (measured as number of OTUs) was climate, including temperature and precipitation. Warmer climates promoted the diversity of bacteria, whereas fungi richness was unaffected by temperature. In turn, fungi richness was lower in urban landscapes compared to near-natural landscapes and bacteria richness was higher on meadows than on forest sites. Fungi were extremely specialized on their host tree, independent of land use and climate. Bacteria specialization, however, was strongly directed by land use and climate. These results underpin previous studies showing that fungi are highly specialized in contrast to bacteria and add new insights into the robustness of fungi specialization to climate and land use. I summarize that climate as well as intensive land use influence biodiversity. Temperature and precipitation, however, had positive and negative effects on decomposer diversity, while anthropogenic land use had mostly negative effects on the diversity of decomposers. N2 - Die Zunahme intensiv genutzter Landschaften und der Klimawandel sind direkte und indirekte Folgen menschlichen Handelns, verursacht durch eine wachsende Weltbevölkerung und zunehmende Mengen an Treibhausgasen. Die Zahl der wissenschaftlichen Studien, die sich mit den Veränderungen der Umwelt und den Konsequenzen für Ökosysteme, einschließlich Flora, Fauna und Ökosystemleistungen auseinandersetzen, steigt stetig. Mit dieser Thesis möchte ich meinen Beitrag zu diesem wichtigen und aktuellen Forschungsgebiet leisten. Dazu untersuche ich die Auswirkungen von Landnutzung und Klima auf die Ökosystemleistung „Zersetzung toten organischen Materials“ (Nekromasse) und die Auswirkungen auf die daran beteiligten Arthropoden- und Mikrobengemeinschaften. Kapitel II dieser Thesis setzt sich mit den Konsequenzen von intensiver Landnutzung und Klimawandel für die Ökosystemleistung „Zersetzung toten Materials“ auseinander. Unter Anbetracht des globalen Insektenrückgangs, wurde dieser Aspekt anhand eines Insektenausschluss-Experimentes zusätzlich simuliert. Es stellt sich heraus, dass sowohl der Abbau von Dung als auch von Aas sehr robust gegenüber landschaftlicher Nutzung war. Zudem blieb der Abbau von Dung unberührt von Temperaturänderungen und dem Ausschluss von Insekten. Entlang eines Höhengradienten wurde hingegen ein Trend zu einem unimodalen Muster mit maximaler Zersetzung bei ca. 600-700 m ü.M. beobachtet. Dieser Trend lässt vermuten, dass in dieser Höhe das Verhältnis von Niederschlag und Temperatur ideal für Dung zersetzende Gemeinschaften ist. Aas hingegen wurde in zunehmender Höhe und unter der Beteiligung von Insekten schneller zersetzt, was verdeutlich, dass Klimaänderungen und ein ansteigender Insektenrückgang starke Auswirkungen auf die Zersetzung von Aas und somit auf Nährstoffkreisläufe haben können. Hierbei wurde zudem ersichtlich, dass verschiedene Typen von Nekromasse unterschiedlich auf Umweltparameter reagieren und daher in künftigen Studien und Auswertungen separat betrachtet werden sollten. Kapitel III behandelt die Auswirkungen von Landnutzung und Klima auf die Biodiversität und Spezialisierung von Käfergemeinschaften an Dung. Hierbei wurden sämtliche Käfer berücksichtigt, welche vor allem an Dung, Aas oder sonstigem faulenden Material gefunden werden können. Sowohl α- als auch γ-Diversität von diesen Käfern wurde durch Agrarlandschaften und urbane Gebiete stark reduziert. Hohe Niederschlagsmengen wirkten sich negativ auf die Abundanz von Dungkäfern aus, wohingegen die γ-Diversität in warmen Regionen am niedrigsten war. Der Grad der Spezialisierung von Käfergemeinschaften auf verschiedene Dungressourcen nahm mit abnehmenden Temperaturen zu. Aus den Ergebnissen geht hervor, dass sowohl intensive Landnutzung als auch Klimaveränderungen Auswirkungen auf die Diversität und den Spezialisierungsgrad von Käfergemeinschaften an Dung haben können und somit das ökologische Gleichgewicht der Dungkäfergemeinschaften und ihren Ökosystemfunktionen beeinflussen können. Das darauffolgende Kapitel IV stellt eine Ergänzung zu Kapitel II dar. Hier wird die Zersetzung von Aas nicht nur anhand von Landnutzung und Klima erklärt, sondern auch anhand der α-Diversität und der Artenzusammensetzung von Käfern und Bakterien an Aas diskutiert. Es zeigte sich, dass Abundanz und Artenzusammensetzung der Bakteriengemeinschaft an Aas vor allem von der Temperatur abhingen. Außerdem wurde die Zersetzungsgeschwindigkeit maßgeblich von der Bakteriengemeinschaft und der Niederschlagsmenge bestimmt. Mit dieser Studie konnte ich zeigen, dass Bakterien trotz ihrer mikroskopischen Größe maßgeblich an der Zersetzung von Aas beteiligt sind und diese in Zersetzungsversuchen nicht vernachlässigt werden sollten. Das letzte Kapitel, Kapitel V, befasst sich mit den Konsequenzen von intensiver Landnutzung und Klimawandel auf mikrobielle Gemeinschaften in Totholz. Untersucht wurden hier sowohl Bakterien- als auch Pilzgemeinschaften. Haupttreiber der Artenvielfalt für beide Gruppen (gemessen als Anzahl an OTUs) war das Klima (Niederschlag und Temperatur). Ein wärmeres Klima kam der Vielfalt von Bakterien zugute, wohingegen die Pilzvielfalt nicht tangiert wurde. Außerdem reagierten Pilze negativ auf urbane Landnutzung, Bakterienvielfalt in Totholz war auf Wiesen jedoch höher als im Wald. Vor allem Pilze zeigten eine sehr starke Bindung zu ihrem Wirtsbaum, welche auch von äußeren Einflüssen wie Landnutzung und Klima nicht beeinflusst werden konnte. Die Spezialisierung von Bakterien hingegen wurde stark von Landnutzung und Klima beeinflusst. Diese Ergebnisse untermauern frühere Studien, die besagen, dass Pilze hoch spezialisiert sind und geben neue Erkenntnisse zur Robustheit der Spezialisierung gegenüber Landnutzungsintensität und Klima. Zusammenfassend kann ich sagen, dass sowohl Klima als auch Landnutzung Auswirkungen auf die Biodiversität haben. Während Temperatur und Niederschlag jedoch positive so wie negative Effekte hatten, wirkte sich anthropogene Landnutzung überwiegend negativ auf die Diversität von Zersetzergemeinschaften aus. KW - Mikroorganismus KW - decomposition KW - Klimaänderung KW - Zersetzungsprozess KW - microbes KW - dead organic material KW - Mikroben Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-313994 ER - TY - THES A1 - Englberger, Eva T1 - Gene regulation in hearts of Hey-mutant mouse embryos and monitoring of sub-cellular Hey1 distribution T1 - Genregulation in Herzen Hey-mutierter Mausembryonen und Darstellung der sub-zellulären Verteilung von Hey1 N2 - Hey-mutant mouse hearts at embryonic day E14.5 were shown to react to the knock out of Hey2 with several up-regualted genes. This up-regulation is due to the lack of Hey2 and cannot be explained by the structural changes in heart morphology as shown using control animals. Part of the gene regulation was further validated using in situ hybridization. Hey1 was located to the nucleus in immunofluorescence experiments. However, experiments on protein level showed also amount of Hey1 within the cytoplasm. The nuclear localization of Hey1 was unchanged during all cell cycle phases as well as when CaMKII was co-expressed or other cellular pathways were inhibited or stimulated. Hey1 does not seem to interact with the nuclear transport proteins importin-alpha and -beta, therefore it still needs to be elucidated how Hey1 is transported into the nucleus. N2 - Am Embryonaltag 14,5 zeigten Herzproben von Hey2-KO-Mäusen eine deutliche Hochregulation mehrerer Gene, die auf das Fehlen von Hey2 zurückzuführen ist, da Kontroll-Tiere gezeigt haben, dass die morphologischen Veränderungen in der Herzstruktur keinen Einfluss auf die Genregulation haben. Vereinzelt wurden die regulierten Gene noch mittels in situ Hybridisierung weiter verdeutlicht. In Immunfloureszenzexperimenten wurde Hey1 im Zellkern lokalisiert. Auf Proteinebene zeigte sich allerdings auch ein Vorhandensein von Hey1 im Cytoplasma der Zellen. Die Kernlokalisaiton von Hey1 veränderte sich während des gesamten Zellzykluses nicht und wurde auch nicht durch die Co-Expression von CaMKII beeinflusst oder die Inhibition oder Stimulation anderer Signalwege in der Zelle. Hey1 scheint nicht mit den Kerntransportproteinen Importin-alpha und -beta zu interagieren, so dass weiterhin nach einem Kernimport-System für Hey1 gesucht werden muss. KW - Maus KW - Herz KW - Embryonalentwicklung KW - Genregulation KW - Herzentwicklung KW - Kerntransport KW - Hey KW - heart development KW - nuclear transport Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-73395 ER - TY - THES A1 - Engelmann, Julia Cathérine T1 - DNA microarrays: applications and novel approaches for analysis and interpretation T1 - DNA Mikroarrays: Anwendungen und neue Ansätze für die Analyse und Interpretation N2 - In der vorliegenden Dissertation wird die Entwicklung eines phylogenetischen DNA Microarrays, die Analyse von mehreren Microarray-Genexpressionsdatensätzen und neue Ansätze für die Datenanalyse und Interpretation der Ergebnisse vorgestellt. Die Entwicklung und Analyse der Daten eines phylogenetischen DNA Microarrays wird in der ersten Publikation dargestellt. Ich konnte zeigen, dass die Spezies-Detektion mit phylogenetischen Microarrays durch die Datenanalyse mit einem linearen Regressionsansatz signifikant verbessert werden kann. Standard-Methoden haben bislang nur Signalintensitäten betrachtet und eine Spezies als an- oder abwesend bezeichnet, wenn die Signalintensität ihres Messpunktes oberhalb eines willkürlich gesetzten Schwellenwertes lag. Dieses Verfahren ist allerdings aufgrund von Kreuz-Hybridisierungen nicht auf sehr nah verwandte Spezies mit hoher Sequenzidentität anwendbar. Durch die Modellierung des Hybridisierungs und Kreuz-Hybridisierungsverhaltens mit einem linearen Regressionsmodell konnte ich zeigen, dass Spezies mit einer Sequenzähnlichkeit von 97% im Markergen immer noch unterschieden werden können. Ein weiterer Vorteil der Modellierung ist, dass auch Mischungen verschiedener Spezies zuverlässig vorhergesagt werden können. Theoretisch sind auch quantitative Vorhersagen mit diesem Modell möglich. Um die großen Datenmengen, die in öffentlichen Microarray-Datenbanken abgelegt sind besser nutzen zu können, bieten sich Meta-Analysen an. In der zweiten Publikation wird eine explorative Meta-Analyse auf Arabidopsis thaliana-Datensätzen vorgestellt. Mit der Analyse verschiedener Datensätze, die den Einfluss von Pflanzenhormonen, Pathogenen oder verschiedenen Mutationen auf die Genexpression untersucht haben, konnten die Datensätze anhand ihrer Genexpressionsprofile in drei große Gruppen eingeordnet werden: Experimente mit Indol-3-Essigsäure (IAA), mit Pathogenen und andere Experimente. Gene, die charakteristisch für die Gruppe der IAA-Datensätze beziehungsweise für die Gruppe der Pathogen-Datensätze sind, wurden näher betrachtet. Diese Gene hatten Funktionen, die bereits mit Pathogenbefall bzw. dem Einfluss von IAA in Verbindung gebracht wurden. Außerdem wurden Hypothesen über die Funktionen von bislang nicht annotierten Genen aufgestellt. In dieser Arbeit werden auch Primäranalysen von einzelnen Arabidopsis thaliana Genexpressions-Datensätzen vorgestellt. In der dritten Publikation wird ein Experiment beschrieben, das durchgeführt wurde um herauszufinden ob Mikrowellen-Strahlung einen Einfluss auf die Genexpression einer Zellkultur hat. Dazu wurden explorative Analysemethoden angewendet. Es wurden geringe aber signifikante Veränderungen in einer sehr kleinen Anzahl von Genen beobachtet, die experimentell bestätigt werden konnten. Die Funktionen der regulierten Gene und eine Meta-Analyse mit öffentlich zugänglichen Datensätzen einer Datenbank deuten darauf hin, dass die pflanzliche Zellkultur die Strahlung als eine Art Energiequelle ähnlich dem Licht wahrnimmt. Des weiteren wird in der vierten Publikation die funktionelle Analyse eines Arabidopsis thaliana Genexpressionsdatensatzes beschrieben. Die Analyse der Genexpressions eines pflanzlichen Tumores zeigte, dass er seinen Stoffwechsel von aerob und auxotroph auf anaerob und heterotroph umstellt. Gene der Photosynthese werden im Tumorgewebe reprimiert, Gene des Aminosäure- und Fettstoffwechsels, der Zellwand und Transportkanäle werden so reguliert, dass Wachstum und Entwicklung des Tumors gefördert werden. In der fünften Publikation in dieser Arbeit wird GEPAT (Genome Expression Pathway Analysis Tool) beschrieben. Es besteht aus einer Internet- Anwendung und einer Datenbank, die das einfache Hochladen von Datensätzen in die Datenbank und viele Möglichkeiten der Datenanalyse und die Integration anderer Datentypen erlaubt. In den folgenden zwei Publikationen (Publikation 6 und Publikation 7) wird GEPAT auf humane Microarray-Datensätze angewendet um Genexpressionsdaten mit weiteren Datentypen zu verknüpfen. Genexpressionsdaten und Daten aus vergleichender Genom-Hybridisierung (CGH) von primären Tumoren von 71 Mantel-Zell-Lymphom (MCL) Patienten ermöglichte die Ermittlung eines Prädiktors, der die Vorhersage der Überlebensdauer von Patienten gegenüber herkömmlichen Methoden verbessert. Die Analyse der CGH Daten zeigte, dass auch diese für die Vorhersage der Überlebensdauer geeignet sind. Für den Datensatz von Patienten mit großzellig diffusem B-Zell-Lymphom DLBCL konnte aus den Genexpressionsdaten ebenfalls ein neuer Prädiktor vorgeschlagen werden. Mit den zwischen lang und kurz überlebenden Patienten differentiell exprimierten Genen der MCL Patienten und mit den Genen, die zwischen den beiden Untergruppen von DLBCL reguliert sind, wurden Interaktionsnetzwerke gebildet. Diese zeigen, dass bei beiden Krebstypen Gene des Zellzyklus und der Proliferation zwischen Patienten mit kurzer und langer Überlebensdauer unterschiedlich reguliert sind. N2 - In this thesis, the development of a phylogenetic DNA microarray, the analysis of several gene expression microarray datasets and new approaches for improved data analysis and interpretation are described. In the first publication, the development and analysis of a phylogenetic microarray is presented. I could show that species detection with phylogenetic DNA microarrays can be significantly improved when the microarray data is analyzed with a linear regression modeling approach. Standard methods have so far relied on pure signal intensities of the array spots and a simple cutoff criterion was applied to call a species present or absent. This procedure is not applicable to very closely related species with high sequence similarity because cross-hybridization of non-target DNA renders species detection impossible based on signal intensities alone. By modeling hybridization and cross-hybridization with linear regression, as I have presented in this thesis, even species with a sequence similarity of 97% in the marker gene can be detected and distinguished from related species. Another advantage of the modeling approach over existing methods is that the model also performs well on mixtures of different species. In principle, also quantitative predictions can be made. To make better use of the large amounts of microarray data stored in public databases, meta-analysis approaches need to be developed. In the second publication, an explorative meta-analysis exemplified on Arabidopsis thaliana gene expression datasets is presented. Integrating datasets studying effects such as the influence of plant hormones, pathogens and different mutations on gene expression levels, clusters of similarly treated datasets could be found. From the clusters of pathogen-treated and indole-3-acetic acid (IAA) treated datasets, representative genes were selected which pointed to functions which had been associated with pathogen attack or IAA effects previously. Additionally, hypotheses about the functions of so far uncharacterized genes could be set up. Thus, this kind of meta-analysis could be used to propose gene functions and their regulation under different conditions. In this work, also primary data analysis of Arabidopsis thaliana datasets is presented. In the third publication, an experiment which was conducted to find out if microwave irradiation has an effect on the gene expression of a plant cell culture is described. During the first steps, the data analysis was carried out blinded and exploratory analysis methods were applied to find out if the irradiation had an effect on gene expression of plant cells. Small but statistically significant changes in a few genes were found and could be experimentally confirmed. From the functions of the regulated genes and a meta-analysis with publicly available microarray data, it could be suspected that the plant cell culture somehow perceived the irradiation as energy, similar to perceiving light rays. The fourth publication describes the functional analysis of another Arabidopsis thaliana gene expression dataset. The gene expression data of the plant tumor dataset pointed to a switch from a mainly aerobic, auxotrophic to an anaerobic and heterotrophic metabolism in the plant tumor. Genes involved in photosynthesis were found to be repressed in tumors; genes of amino acid and lipid metabolism, cell wall and solute transporters were regulated in a way that sustains tumor growth and development. Furthermore, in the fifth publication, GEPAT (Genome Expression Pathway Analysis Tool), a tool for the analysis and integration of microarray data with other data types, is described. It consists of a web application and database which allows comfortable data upload and data analysis. In later chapters of this thesis (publication 6 and publication 7), GEPAT is used to analyze human microarray datasets and to integrate results from gene expression analysis with other datatypes. Gene expression and comparative genomic hybridization data from 71 Mantle Cell Lymphoma (MCL) patients was analyzed and allowed proposing a seven gene predictor which facilitates survival predictions for patients compared to existing predictors. In this study, it was shown that CGH data can be used for survival predictions. For the dataset of Diffuse Large B-cell lymphoma (DLBCL) patients, an improved survival predictor could be found based on the gene expression data. From the genes differentially expressed between long and short surviving MCL patients as well as for regulated genes of DLBCL patients, interaction networks could be set up. They point to differences in regulation for cell cycle and proliferation genes between patients with good and bad prognosis. KW - Microarray KW - Differentielle Genexpression KW - Genexpression KW - Statistische Analyse KW - Cluster-Analyse KW - Datenanalyse KW - Explorative Datenanalyse KW - Non-Hodgkin-Lymphom KW - B-Zell-Lymphom KW - Metabolom KW - Tumorklassifikation KW - Tumor KW - Krebs KW - Schmalwa KW - phylogenetische Arrays KW - Interaktionsnetzwerke KW - lineare Regression KW - DNA microarray KW - gene expression KW - statistical analysis KW - clustering KW - classification KW - interaction networks Y1 - 2008 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-29747 ER - TY - THES A1 - Engelhardt [geb. Christiansen], Frauke T1 - Synaptic Connectivity in the Mushroom Body Calyx of Drosophila melanogaster T1 - Synaptische Konnektivität im Pilzkörper Kalyx in Drosophila melanogaster N2 - Learning and memory is considered to require synaptic plasticity at presynaptic specializations of neurons. Kenyon cells are the intrinsic neurons of the primary olfactory learning center in the brain of arthropods – the mushroom body neuropils. An olfactory mushroom body memory trace is supposed to be located at the presynapses of Kenyon cells. In the calyx, a sub-compartment of the mushroom bodies, Kenyon cell dendrites receive olfactory input provided via projection neurons. Their output synapses, however, were thought to reside exclusively along their axonal projections outside the calyx, in the mushroom body lobes. By means of high-resolution imaging and with novel transgenic tools, we showed that the calyx of the fruit fly Drosophila melanogaster also comprised Kenyon cell presynapses. At these presynapses, synaptic vesicles were present, which were capable of neurotransmitter release upon stimulation. In addition, the newly identified Kenyon cell presynapses shared similarities with most other presynapses: their active zones, the sites of vesicle fusion, contained the proteins Bruchpilot and Syd-1. These proteins are part of the cytomatrix at the active zone, a scaffold controlling synaptic vesicle endo- and exocytosis. Kenyon cell presynapses were present in γ- and α/β-type KCs but not in α/β-type Kenyon cells. The newly identified Kenyon cell derived presynapses in the calyx are candidate sites for an olfactory associative memory trace. We hypothesize that, as in mammals, recurrent neuronal activity might operate for memory retrieval in the fly olfactory system. Moreover, we present evidence for structural synaptic plasticity in the mushroom body calyx. This is the first demonstration of synaptic plasticity in the central nervous system of Drosophila melanogaster. The volume of the mushroom body calyx can change according to changes in the environment. Also size and numbers of microglomeruli - sub-structures of the calyx, at which projection neurons contact Kenyon cells – can change. We investigated the synapses within the microglomeruli in detail by using new transgenic tools for visualizing presynaptic active zones and postsynaptic densities. Here, we could show, by disruption of the projection neuron - Kenyon cell circuit, that synapses of microglomeruli were subject to activity-dependent synaptic plasticity. Projection neurons that could not generate action potentials compensated their functional limitation by increasing the number of active zones per microglomerulus. Moreover, they built more and enlarged microglomeruli. Our data provide clear evidence for an activity-induced, structural synaptic plasticity as well as for the activity-induced reorganization of the olfactory circuitry in the mushroom body calyx. N2 - Synaptische Plastizität an den präsynaptischen Spezialisierungen von Neuronen sind nach allgemeinem Verständnis die Grundlage für Lern- und Gedächtnisprozesse. Kenyon Zellen sind die intrinsischen Zellen des Zentrums für olfaktorisches Lernen im Gehirn von Arthropoden – den Pilzkörper Neuropilen. An den Präsynapsen der Kenyon Zellen wird eine olfaktorische Gedächtnisspur vermutet. Im Kalyx, einer Substruktur der Pilzkörper, erhalten die Kenyon Zell Dendriten ihren olfaktorischen Input durch Projektionsneurone. Ihre Präsynapsen wiederum befinden sich ausschließlich in ihren axonalen Kompartimenten außerhalb des Kalyx, nämlich in den Loben der Pilzkörper. Mit Hilfe von hochauflösenden bildgebenden Techniken und neuen transgenen Methoden, ist es uns in der Fruchtfliege Drosophila melanogaster gelungen, Kenyon Zell Präsynapsen im Kalyx zu identifizieren. Diese Präsynapsen enthalten synaptische Vesikel, die nach Stimulation ihren Inhalt freisetzen können. Sie weisen noch weitere Gemeinsamkeiten mit den meisten anderen Präsynapsen auf: Ihre Aktiven Zonen, die Orte der Transmitterfreisetzung, enthalten die Proteine Bruchpilot und Syd-1. Diese sind Teil der Zytomatrix an der Aktiven Zone, ein Proteingerüst das Endo- und Exozytose der synaptischen Vesikel kontrolliert. Die Präsynapsen im Kalyx wurden in γ- and α/β-Typ Kenyon Zellen aber nicht in α/β-Typ Kenyon Zellen gefunden. Die neu identifizierten Kenyon Zell Präsynapsen beherbergen potentiell eine Gedächtnisspur für olfaktorisch assoziatives Lernen. Möglicherweise wird im olfaktorischen Nervensystem von Fruchtfliegen rücklaufende neuronale Aktivität benötigt, um Gedächtnis abzurufen, so wie es auch für Säuger beschrieben ist. Darüber hinaus zeigen wir synaptische Plastizität im Kalyx. Dies ist die erste Beschreibung überhaupt von synaptischer Plastizität im zentralen Nervensystem von Drosophila melanogaster. Das Volumen des Kalyx kann sich als Antwort auf äußere Einflüsse verändern. Genauso auch Größe und Anzahl der Mikroglomeruli, Substrukturen des Kalyx, in denen Projektionsneurone und Kenyon Zellen aufeinander treffen. Wir untersuchten die Synapsen in Mikroglomeruli detailliert, mithilfe von neuen transgenen Methoden, die es erlauben, präsynaptische Aktive Zonen sowie Postsynaptische Spezialisierungen zu visualisieren. Mittels Beeinträchtigung der Kommunikation zwischen Projektionsneuronen und Kenyon Zellen, konnten wir synaptische Plastizität in Mikroglomeruli zeigen. Projektionsneurone, die nicht in der Lage waren, Aktionspotentiale zu erzeugen, kompensierten ihre funktionelle Einschränkung durch den vermehrten Einbau von Aktiven Zonen in Mikroglomeruli. Außerdem produzierten sie mehr und vergrößerte Mikroglomeruli. Unsere Daten zeigen deutlich eine aktivitätsinduzierte Veränderung des olfaktorischen neuronalen Netzes, sowie strukturelle synaptische Plastizität im Kalyx. KW - Taufliege KW - Pilzkörper KW - Drosophila melanogaster KW - mushroom body KW - calyx KW - Geruch KW - Lernen KW - Gedächtnis KW - Kalyx Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-85058 ER - TY - JOUR A1 - Endres, Marcel A1 - Kneitz, Susanne A1 - Orth, Martin F. A1 - Perera, Ruwan K. A1 - Zernecke, Alma A1 - Butt, Elke T1 - Regulation of matrix metalloproteinases (MMPs) expression and secretion in MDA-MB-231 breast cancer cells by LIM and SH3 protein 1 (LASP1) JF - Oncotarget N2 - The process of tumor invasion requires degradation of extracellular matrix by proteolytic enzymes. Cancer cells form protrusive invadopodia, which produce and release matrix metalloproteinases (MMPs) to degrade the basement membrane thereby enabling metastasis. We investigated the effect of LASP1, a newly identified protein in invadopodia, on expression, secretion and activation of MMPs in invasive breast tumor cell lines. By analyzing microarray data of in-house generated control and LASP1-depleted MDA-MB-231 breast cancer cells, we observed downregulation of MMP1, -3 and -9 upon LASP1 depletion. This was confirmed by Western blot analysis. Conversely, rescue experiments restored in part MMP expression and secretion. The regulatory effect of LASP1 on MMP expression was also observed in BT-20 breast cancer cells as well as in prostate and bladder cancer cell lines. In line with bioinformatic FunRich analysis of our data, which mapped a high regulation of transcription factors by LASP1, public microarray data analysis detected a correlation between high LASP1 expression and enhanced c-Fos levels, a protein that is part of the transcription factor AP-1 and known to regulate MMP expression. Compatibly, in luciferase reporter assays, AP-1 showed a decreased transcriptional activity after LASP1 knockdown. Zymography assays and Western blot analysis revealed an additional promotion of MMP secretion into the extracellular matrix by LASP1, thus, most likely, altering the microenvironment during cancer progression. The newly identified role of LASP1 in regulating matrix degradation by affecting MMP transcription and secretion elucidated the migratory potential of LASP1 overexpressing aggressive tumor cells in earlier studies. KW - LASP1 KW - c-Fos KW - extracellular matrix KW - AP-1 KW - matrix metalloproteinases KW - breast cancer Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-176920 VL - 7 IS - 39 ER - TY - JOUR A1 - Endres, Leo M. A1 - Jungblut, Marvin A1 - Divyapicigil, Mustafa A1 - Sauer, Markus A1 - Stigloher, Christian A1 - Christodoulides, Myron A1 - Kim, Brandon J. A1 - Schubert-Unkmeir, Alexandra T1 - Development of a multicellular in vitro model of the meningeal blood-CSF barrier to study Neisseria meningitidis infection JF - Fluids and Barriers of the CNS N2 - Background Bacterial meningitis is a life-threatening disease that occurs when pathogens such as Neisseria meningitidis cross the meningeal blood cerebrospinal fluid barrier (mBCSFB) and infect the meninges. Due to the human-specific nature of N. meningitidis, previous research investigating this complex host–pathogen interaction has mostly been done in vitro using immortalized brain endothelial cells (BECs) alone, which often do not retain relevant barrier properties in culture. Here, we developed physiologically relevant mBCSFB models using BECs in co-culture with leptomeningeal cells (LMCs) to examine N. meningitidis interaction. Methods We used BEC-like cells derived from induced pluripotent stem cells (iBECs) or hCMEC/D3 cells in co-culture with LMCs derived from tumor biopsies. We employed TEM and structured illumination microscopy to characterize the models as well as bacterial interaction. We measured TEER and sodium fluorescein (NaF) permeability to determine barrier tightness and integrity. We then analyzed bacterial adherence and penetration of the cell barrier and examined changes in host gene expression of tight junctions as well as chemokines and cytokines in response to infection. Results Both cell types remained distinct in co-culture and iBECs showed characteristic expression of BEC markers including tight junction proteins and endothelial markers. iBEC barrier function as determined by TEER and NaF permeability was improved by LMC co-culture and remained stable for seven days. BEC response to N. meningitidis infection was not affected by LMC co-culture. We detected considerable amounts of BEC-adherent meningococci and a relatively small number of intracellular bacteria. Interestingly, we discovered bacteria traversing the BEC-LMC barrier within the first 24 h post-infection, when barrier integrity was still high, suggesting a transcellular route for N. meningitidis into the CNS. Finally, we observed deterioration of barrier properties including loss of TEER and reduced expression of cell-junction components at late time points of infection. Conclusions Here, we report, for the first time, on co-culture of human iPSC derived BECs or hCMEC/D3 with meningioma derived LMCs and find that LMC co-culture improves barrier properties of iBECs. These novel models allow for a better understanding of N. meningitidis interaction at the mBCSFB in a physiologically relevant setting. KW - brain endothelial cells KW - bacterial meningitis KW - meningeal blood-csf barrier KW - induced pluripotent stem cells KW - neisseria meningitidis KW - leptomeningeal cells Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-300208 VL - 19 IS - 1 ER - TY - THES A1 - Endler, Annett T1 - Regulation of reproductive division of labor in the ant Camponotus floridanus : behavioral mechanisms and pheromonal effects T1 - Regulation der reproduktiven Arbeitsteilung bei der Ameise Camponotus floridanus: Verhaltensmechanismen und Einfluss von Pheromonen N2 - A hitherto unresolved problem is how workers are prevented from reproducing in large insect societies. The queen informs about her fertility and health which ensures sufficient indirect fitness benefits for workers. In the ant Camponotus floridanus, I found such a signal located on eggs of highly fertile queens. Groups of workers were regularly provided with different sets of brood. Only in groups with queen eggs workers refrain from reproducing. Thus, the eggs seem to inform the workers about queen presence. The signal on queen eggs is presumably the same that enables workers to distinguish between queen and worker-laid eggs, latter are destroyed by workers. Queen and worker-laid eggs differ in their surface hydrocarbons in a similar way as fertile queens differ from workers in the composition of their cuticular hydrocarbons. When I transferred hydrocarbons from the queen cuticle to worker eggs the eggs were no longer destroyed, indicating that they now carry the signal. These hydrocarbons thus represent a queen signal that regulates worker reproduction in this species. But the signal is not present in all fertile queens. Founding queens with low egg-laying rates differ in the composition of cuticular hydrocarbons from queens with high productivity. Similar differences in the composition of surface hydrocarbons were present on their eggs. The queen signal develops along with an increasing fertility and age of the queen, and this is perceived by the workers. Eggs from founding queens were destroyed like worker eggs. This result shows that founding queens lack the appropriate signal. In these little colony foundations chemical communication of queen status may not be necessary to prevent workers from reproducing, since workers may benefit more from investing in colony growth and increased productivity of large colonies rather than from producing male eggs in incipient colonies. If the queen is missing or the productivity of the queen decreases, workers start laying eggs. There is some evidence from correlative studies that, under queenless conditions, worker police each other because of differences in individual odors as a sign of social status. It can be expressed as either aggressive inhibition of ovarian activity, workers with developed ovaries are attacked by nest-mates, or destruction by worker-laid eggs. I found that in C. floridanus workers, in contrast to known studies, police only by egg eating since they are able to discriminate queen- and worker-laid eggs. Workers with developed ovaries will never attacked by nest-mates. This is further supported by qualitative and quantitative differences in the cuticular hydrocarbon profile of queens and workers, whereas profiles of workers with and without developed ovaries show a high similarity. I conclude that workers discriminate worker eggs on the basis of their hydrocarbon profile, but they are not able to recognize egg-laying nest-mates. Improving our knowledge of the proximate mechanisms of the reproductive division of labor in evolutionary derived species like C. floridanus will help to understand the evolution of extreme reproductive altruism involving sterility as a characteristic feature of advanced eusocial systems. N2 - Es ist eine bisher ungelöste Frage, wie Arbeiterinnen in großen Insektenkolonien von der Reproduktion abgehalten werden. Arbeiterinnen würden einen erheblichen Fitnessvorteil erlangen, falls die Königin über ihre Fertilität und ihren Gesundheitszustand informiert. Bei der Ameise Camponotus floridanus konnte auf den Eiern hochfertiler Königinnen so ein Signal gefunden werden. Gruppen von Arbeiterinnen wurden regelmäßig mit verschiedenen Brutansätzen versorgt. Aber nur in Gruppen, welche Eier der Königin erhielten, wurden die Arbeiterinnen von der Reproduktion abgehalten. Die Eier informieren demnach über die Anwesenheit der Königin. Das Signal der Königineier ermöglicht Arbeiterinnen offensichtlich auch zwischen Eiern von Königin und Arbeiterinnen zu unterscheiden, wobei letztere zerstört werden. Königin- und Arbeiterinneneier unterscheiden sich in ihren Oberflächenkohlenwasserstoffen auf ähnliche Weise wie sich die kutikulären Kohlenwasserstoffprofile von fertilen Königinnen und Arbeiterinnen unterscheiden. Wurden Kohlenwasserstoffe von der Kutikula der Königin auf Eier von Arbeiterinnen übertragen, schützten sie diese vor der Zerstörung. Dies zeigt, dass die Eier das Signal transportieren. Die Kohlenwasserstoffe stellen ein Königinsignal dar, welches die Reproduktion der Arbeiterinnen bei C. floridanus regelt. Allerdings kommt das Signal nicht bei allen fertilen Königinnen vor. Gründungsköniginnen mit einer geringen Eiablagerate unterscheiden sich in der Zusammensetzung der Kohlenwasserstoffe von Königinnen mit einer höheren Produktivität. Ähnliche Unterschiede in der Zusammensetzung der Oberflächenkohlenwasserstoffe finden sich ebenfalls auf den jeweiligen Eiern. Das Königinsignal gewinnt an Stärke mit zunehmender Fertilität und Alter der Königin, was von den Arbeiterinnen erkannt wird. Eier von Gründungsköniginnen werden wie die Eier von Arbeiterinnen zerstört. Das Ergebnis zeigt, dass Gründungsköniginnen das betreffende Signal nicht besitzen. Um Arbeiterinnen von der Reproduktion abzuhalten, scheint es in kleinen Gründungskolonien nicht notwendig über den Zustand der Königin zu informieren. Arbeiterinnen in diesen Kolonien profitieren mehr von der Investition in das Koloniewachstum als von der Produktion von Männchen. Fehlt die Königin oder nimmt ihre Produktivität ab, dann beginnen Arbeiterinnen mit der Eiablage. Es gibt Belege aus anderen Studien, dass unter königinlosen Bedingungen Arbeiterinnen sich gegenseitig von der erfolgreichen Reproduktion abhalten (worker policing). Dabei orientieren sie sich am individuellen Geruch der Tiere je nach sozialem Status. Die Inhibierung der Ovarienaktivität erfolgt über Aggression, indem fertile Arbeiterinnen von ihren Nestgenossinnen attackiert werden, oder über die Zerstörung von Eiern. Arbeiterinnen von C. floridanus policen, im Gegensatz zu den bekannten Studien, nur durch Eifrass, da sie in der Lage sind Eier von Königin und Arbeiterinnen zu unterscheiden. Fertile Arbeiterinnen werden dagegen nie von Nestgenossinnen angegriffen. Dies wird unterstützt durch qualitative und quantitative Unterschiede im kutikulären Kohlenwasserstoffprofil zwischen Königin und Arbeiterinnen, während sich das Profil fertiler und infertiler Arbeiterinnen dagegen nicht unterscheidet. Arbeiterinnen nutzen demnach das Kohlenwasserstoffprofil um Eier zu unterscheiden, sind aber nicht in der Lage fertile Nestgenossinnen zu erkennen. Die Aufklärung der Regulationsmechanismen der reproduktiven Arbeitsteilung bei stark abgeleiteten Arten wie C. floridanus liefert einen Beitrag zum Verständnis, wieso es im Laufe der Evolution zur reproduktiven Degeneration von Arbeiterinnen gekommen ist, einem Charakteristikum hoch entwickelter eusozialer Systeme. KW - Camponotus floridanus KW - Fortpflanzung KW - Pheromon KW - soziale Insekten KW - Ameisen KW - Fertilitätssignal KW - kutikuläre Kohlenwasserstoffe KW - worker policing KW - social insects KW - ants KW - fertility signal KW - cuticular hydrocarbons KW - worker policing Y1 - 2006 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-18872 ER - TY - JOUR A1 - Endesfelder, Ulrike A1 - Malkusch, Sebastian A1 - Flottmann, Benjamin A1 - Mondry, Justine A1 - Liguzinski, Piotr A1 - Verveer, Peter J. A1 - Heilemann, Mike T1 - Chemically Induced Photoswitching of Fluorescent Probes - A General Concept for Super-Resolution Microscopy N2 - We review fluorescent probes that can be photoswitched or photoactivated and are suited for single-molecule localization based super-resolution microscopy. We exploit the underlying photochemical mechanisms that allow photoswitching of many synthetic organic fluorophores in the presence of reducing agents, and study the impact of these on the photoswitching properties of various photoactivatable or photoconvertible fluorescent proteins. We have identified mEos2 as a fluorescent protein that exhibits reversible photoswitching under various imaging buffer conditions and present strategies to characterize reversible photoswitching. Finally, we discuss opportunities to combine fluorescent proteins with organic fluorophores for dual-color photoswitching microscopy. KW - Super-Resolution Microscopy KW - photoswitchable organic fluorophores KW - fluorescent proteins KW - super-resolution KW - PALM KW - dSTORM Y1 - 2011 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-74896 ER - TY - JOUR A1 - Endesfelder, Ulrike A1 - Malkusch, Sebastian A1 - Flottmann, Benjamin A1 - Mondry, Justine A1 - Liguzinski, Piotr A1 - Verveer, Peter J. A1 - Heilemann, Mike T1 - Chemically Induced Photoswitching of Fluorescent Probes - A General Concept for Super-Resolution Microscopy JF - Molecules N2 - We review fluorescent probes that can be photoswitched or photoactivated and are suited for single-molecule localization based super-resolution microscopy. We exploit the underlying photochemical mechanisms that allow photoswitching of many synthetic organic fluorophores in the presence of reducing agents, and study the impact of these on the photoswitching properties of various photoactivatable or photoconvertible fluorescent proteins. We have identified mEos2 as a fluorescent protein that exhibits reversible photoswitching under various imaging buffer conditions and present strategies to characterize reversible photoswitching. Finally, we discuss opportunities to combine fluorescent proteins with organic fluorophores for dual-color photoswitching microscopy. KW - Photoactivated localization microscopy KW - Fusion proteins KW - Molecules KW - Patterns KW - Switch KW - Limit KW - Time KW - photoswitchable organic fluorophores KW - fluorescent proteins KW - super-resolution KW - PALM KW - dSTORM Y1 - 2011 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-134080 VL - 16 IS - 4 ER - TY - THES A1 - Eltz, Thomas T1 - Ecology of stingless bees (Apidae, Meliponini) in lowland dipterocarp forests in Sabah, Malaysia, and an evaluation of logging impact on populations and communities T1 - Ökologie Stachelloser Bienen (Apidae, Meliponini) in Dipterocarpaceen-Wäldern im Tiefland von Sabah, Malaysia, mit einer Evaluierung des Einflusses der kommerziellen Holznutzung auf Populationen und Gemeinschaften N2 - The present thesis reports on four years of field research on stingless bee ecology in Sabah, Malaysia. Hereby, it was the main focus to evaluate the effect of selective logging for timber extraction on communities of bees, and to elucidate causative relationships involved in regulating bee populations. Included were background studies on resource use (3.1, 3.2, 3.3) and nesting biology (3.4) as well as comparative studies on stingless bee diversity and abundance in logged and unlogged lowland rainforest sites (4.1, 4.2). Stingless bees proved to be generalist foragers that used a large range of plant species as pollen sources. Nevertheless, different species of bees had rather distinct pollen diets, a findind that was independent of fluctuations in flowering activity in the habitat. At one particular point in time colonies of one species (Trigona collina)collected mold spores (Rhizopus sp.) as a pollen surrogate. In order to obtain low-effort estimates of meliponine pollen sources a new method was developed: Trapping of bee garbage (with funnel traps) and the quantitative analysis of pollen in garbage samples. Pollen in bee garbage reflected pollen import with a certain time lag and could therefore be used for an assessment of long-term pollen foraging (see below). The majority of stingless bee nests (275 nests of 12 species) were found in cavities in trunks or under the bases of large, living canopy trees. Nest trees mostly belonged to commercial species and were of the correct size and (partly) timber quality to warrant harvesting. It was estimated that roughly one third of stingless bee nests in an given forest area would be killed during a selective logging operation. Besides causing direct mortality, logging may also indirectly affect bee populations by reducing the availability of potential nest sites (trees). However, in a comparison of primary and differentially logged forest sites (10 to 30 years after logging) no effect of the degree of disturbance on meliponine nest density was found. Instead, the variation in nest density (0 to 16.2 nest/ha) was best explained by differences in the available floral resources (assessed by analysis of pollen in bee garbage). Bee populations in forest edge situations were favored: there was a positive correlation between nest density and the proportion of external non-forest pollen (e.g. from crop plants, road edge vegetation, mangroves) in the bees’ diet. The highest nest density was found in a site bordering the mangroves in Sandakan Bay. Here, the mangrove tree Rhizophora apiculata represented a extraordinary large fraction of the pollen volume. Presumably, external pollen sources effectively supplement bee diets at times when little flowering occurs inside the forest, thus increasing overall bee carrying-capacity. The idea of differential pollen limitation was strengthened by direct measurements of pollen import and foraging activity over a period of five months. Both were elevated in colonies in a site with high bee density. It is concluded that the abundance of stingless bees in forests in Sabah is chiefly dependent on the local availability of food resources. Hereby, bee populations strongly benefit from edge effects and increased habitat diversity. Although direct negative effects of selective logging are strongly indicated by a close association of bee nests with commercial trees, no clear effects were detected in regenerating forests ten to 30 years after logging. N2 - Die vorliegende Dissertation umfaßt die Ergebnisse einer vierjährigen Studie zur Ökologie von Stachellosen Bienen in den Regenwäldern von Sabah, Malaysia. Hauptziel war es dabei, mögliche Auswirkungen der selektiven Holznutzung auf Bienengemeinschaften zu erforschen und, falls sich ein Effekt nachweisen läßt, die dafür verantwortlichen Wirkfaktoren zu identifizieren. Die Arbeiten schlossen sowohl Hintergrundstudien zur Nahrungsökologie (3.1, 3.2, 3.3) und Nistbiologie (3.4) ein, als auch vergleichende Erfassungen der Bienenabundanz und -diversität in primären und durch Holznutzung gestörten Tieflandregenwäldern (4.1, 4.2). Stachellose Bienen erwiesen sich als generalistische Blütenbesucher, die über die Zeit eine Vielzahl verschiedener Blütenpflanzen als Pollenquellen nutzen. Die Überlappung der Pollenspektren zwischen verschiedenen Bienenarten war jedoch sowohl bei geringer als bei höherer Blühaktivität relative niedrig. In einer Ausnahmesituation wurden von mehreren Kolonien einer Art (Trigona collina) auch Schimmelpilzsporen (Rhizopus sp.) als Pollenersatz eingetragen. Um die Pollennahrung von Meliponinen mit geringerem Aufwand und noch detaillierter erfassen zu können wurde eine neue Methode entwickelt: das automatisierte Absammeln von ‚Bienenmüll‘ (mittels Trichtefallen) und die quantitative Analyse der enthaltenen Pollenexinen. Die Polleninhalte des Mülls erwiesen sich dabei als verzögertes Abbild des eingetragenen Pollens und konnte daher für eine grobe Bestimmung langfristiger Nahrungsgewohnheiten herangezogen werden (siehe unten). Die große Mehrzahl der gefundenen Meliponinen-Nester (275 von 12 Arten) befanden sich entweder in Hohlräumen des Stämme oder unter der Stammbasis großer, lebender und oft kommerziell nutzbarer Kronenbäume. Grobe Berechnungen ergaben, daß mehr als ein Drittel aller Bienennester einer durchschnittlichen selektiven Fällaktion zum Opfer fallen würden. Neben diesem direkten Schaden könnte die kommerzielle Holznutzung auch indirekt (über eine Verringerung der zur Verfügung stehenden, potentiellen Nistbäume) die Bienenpopulationen negativ beeinflussen. Im Vergleich unterschiedlich stark eingeschlagener Flächen (10 bis 30 Jahre nach der letzen Nutzung) konnte allerdings kein Zusammenhang der Bienennestdichte mit dem Störungsgrad des Waldes gefunden werden. Statt dessen wurde die hohe Variation der Nestdichte (0 bis 16.2 Nester/ha) am besten durch die Unterschiede in den verfügbaren Nahrungsressourcen erklärt (bestimmt durch Müllpollenanalyse). Hier waren vor allem Waldflächen in Randlage begünstigt. Es bestand eine positive Korrelation der Nestdichte und dem Anteil externer, nicht aus dem Wald stammender Pollentypen (z. B. Kulturpflanzen, Straßenrandvegetation, Mangrovenpflanzen) an der Bienennahrung. Die bei weitem höchste Nestdichte wurden in einem an die Mangroven der Sandakan Bay angrenzenden Wald gefunden, wo ein herausragender Teil der Pollennahrung aus Pollen des Mangrovenbaums Rhizophora apiculata bestand. Vermutlich stellen externe Pollenquellen eine wichtige Ergänzung der Bienennahrung zu Zeiten geringer Blühaktivität im Wald dar, die die ‘carrying capacity’ des Waldes für Meliponinen erhöht. Die Theorie der unterschiedlichen Limitierung durch Pollenquellen wurde durch direkte Messungen von Polleneintrag und Fouragieraktivität überprüft: Beides war über fünf Monate hinweg bei Nestern in einer bienenreichen Fläche erhöht. Zusammenfassend läßt sich schließen, daß die Abundanz von Stachellosen Bienen in Sabahanischen Wäldern hauptsächlich von der lokalen Nahrungsverfügbarkeit abhängt und Bienenpopulationen hierbei stark von Randeffekten und erhöhter Habitatdiversität profitieren. Ein Einfluß von anthropogener Störung durch selektive Holznutzung ist aufgrund der Nistbiologie von Meliponinen kurz und mittelfristig zu erwarten, konnte aber in regenerierenden Wäldern zehn bis 30 Jahren nach dem Einschlag nicht eindeutig nachgewiesen werden. KW - Sabah KW - Stachellose Biene KW - Anthropogener Einfluss KW - Demökologie KW - Meliponini KW - stingless bees KW - Pollennahrung KW - Ressourcenteilung KW - begrenzte Ressource KW - Blühphänologie KW - Pollenanalyse KW - Nistgelegenheit KW - Holznutzung KW - Meliponini KW - stingless bees KW - pollen foraging KW - resource partitioning KW - resource limitation KW - flowering phenology KW - pollen analysis KW - nesting resources Y1 - 2001 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-1130 ER - TY - JOUR A1 - Elkon, Ran A1 - Loayza-Puch, Fabricio A1 - Korkmaz, Gozde A1 - Lopes, Rui A1 - van Breugel, Pieter C A1 - Bleijerveld, Onno B A1 - Altelaar, AF Maarten A1 - Wolf, Elmar A1 - Lorenzin, Francesca A1 - Eilers, Martin A1 - Agami, Reuven T1 - Myc coordinates transcription and translation to enhance transformation and suppress invasiveness JF - EMBO reports N2 - c‐Myc is one of the major human proto‐oncogenes and is often associated with tumor aggression and poor clinical outcome. Paradoxically, Myc was also reported as a suppressor of cell motility, invasiveness, and metastasis. Among the direct targets of Myc are many components of the protein synthesis machinery whose induction results in an overall increase in protein synthesis that empowers tumor cell growth. At present, it is largely unknown whether beyond the global enhancement of protein synthesis, Myc activation results in translation modulation of specific genes. Here, we measured Myc‐induced global changes in gene expression at the transcription, translation, and protein levels and uncovered extensive transcript‐specific regulation of protein translation. Particularly, we detected a broad coordination between regulation of transcription and translation upon modulation of Myc activity and showed the connection of these responses to mTOR signaling to enhance oncogenic transformation and to the TGFβ pathway to modulate cell migration and invasiveness. Our results elucidate novel facets of Myc‐induced cellular responses and provide a more comprehensive view of the consequences of its activation in cancer cells. KW - c‐Myc KW - transcriptional responses KW - translational regulation KW - transcription KW - transformation KW - metastasis KW - cancer KW - protein biosynthesis & quality control Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-150373 VL - 16 IS - 12 ER - TY - THES A1 - El-Masri, Harun T1 - A genetic analysis of somitogenesis in the Medaka (Oryzias latipes) T1 - Genetische Analyse der Somitogenese in Medaka (Oryzias latipes) N2 - Somites are repeated epithelial segments that are generated in a rhythmic manner from the presomitic mesoderm (PSM) in the embryonic tailbud. Later, they differentiate into skeletal muscle, cartilage and dermis. Somitogenesis is regulated by a complex interplay of different pathways. Notch/Delta signaling is one of the pathways well characterized in zebrafish through mutants affected in its different components. Previous work in mouse, chicken and zebrafish has shown that also additional components are required during somitogenesis, most importantly through an FGF and Retinoic acid (RA) gradient, as well as Wnt signaling. However, no zebrafish mutants with defects in these pathways showing specific somite malformations are described. This was explained by functional redundancies among related genes that have resulted from a whole genome duplication which occurred in a teleost fish ancestor 350 million years ago. As distinct duplicates exist in different teleost species, a large scale mutagenesis screen in the medaka (Oryzias latipes) has been performed successfully in Kyoto, Japan. I analyzed nine of the isolated medaka mutants that show variable aspects of somitic phenotypes. This includes a complete or partial loss of somite boundaries (e.g. bms and sne), somites with irregular sizes and shapes (e.g. krz and fsl) or partially fused and enlarged somites (e.g. dpk). Although some of these medaka mutants share characteristics with previously described zebrafish somite mutants, most of the mutants represent unique phenotypes, not obtained in the zebrafish screens. In-situ hybridization analyses with marker genes implicated in the segmentation clock (e.g. her7), establishment of anterior-posterior (A-P) polarity (e.g. mesp) and differentiation of somites (e.g. myf5, lfng) revealed that the medaka mutants can be separated into two classes. Class I shows defects in tailbud formation and PSM prepatterning, and lateron somite boundary formation was impaired in these mutants. A unique member of this class with a novel phenotype is the doppelkorn (dpk) mutant that has single fused or enlarged somites. This phenotype has not been reported till now in zebrafish somite mutants. In-situ analyses on dpk showed that stabilization of the cyclically expressed somitogenesis clock genes must be affected in this mutant. This is accompanied by a disrupted regulation of A-P polarity genes like mesp. This suggests that dpk is a mutant deficient in the wave front, which is necessary for the down-regulation of oscillating genes in the anterior PSM. Furthermore, as the initiation of oscillation of all three cyclic her genes was unaffected in dpk embryos, I could exclude that this mutant in affected in the Notch/Delta pathway. Another mutant that belongs to this class is the samidare (sam) mutant. Morphologically, sam mutants are similar to zebrafish after eight (aei). In both cases, the first 7-9 somites are formed properly, but after this somite formation ceases. Different to the situation in aei, sam mutant embryos presented an additional defect in the mid-hindbrain boundary (MHB) region. Similar MHB defects were described in the zebrafish fgf8 mutant acerebellar (ace). In ace zebrafish mutant, somites were only slightly defective, although FGF signaling has been shown to be important for somite formation in chicken, mouse and zebrafish. This was explained by functional redundancy between fgf8 and fgf24 ligands in the tailbud of zebrafish. Thus, it is interesting to suggest that the sam mutant, based on the parallel defects in somites and MHB, is a potential member of the FGF signaling pathway muatnts. It was shown that FGF plays a crucial role during MHB formation in medaka. In addition, I showed that fgf8 acts non-redundantly during tailbud formation and somitogenesis in medaka. Furthermore, I showed that FGF signaling regulates somite size also in medaka and that fgfr1 is the only FGF receptor expressed in the tailbud and somites. In class II medaka somite mutants, PSM prepatterning appears normal, whereas A-P polarity, boundary formation, epithelialization or the later differentiation of somites appears to be affected. Such mutants have not been isolated so far in zebrafish, mice or chicken. Therefore, medaka class II somite mutants seem to be a novel group of mutants that opens new perspectives to analyze A-P polarity regulation, determination and boundary formation in the presence of a normally functioning clock in the PSM. Identifying the encoding genes for all analyzed medaka somite mutants will contribute to the understanding of the molecular interactions of different signaling pathways involved during somitogenesis, and is expected to result in the identification of new components. N2 - Die Somitogenese stellt einen entscheidenden Prozess bei der Entwicklung von Wirbeltierembryonen dar. Somiten sind transiente Strukturen, die sich im Verlauf der Embryonalentwicklung zu Skelettmuskulatur, Dermis und Wirbelkörper differenzieren. Somiten entstehen in einem sich regelmäßig wiederholenden Zyklus aus Stammzellen des präsomitischen Mesoderms (PSM), einer Wachstumszone am caudalen Ende des Embryos. Ein wichtiger Bestandteil der Somitogenese ist ein molekularer Oszillator, das so genannte „Segmentierungs-Uhrwerk“. Die periodische Segmentierung des präsomitischen Mesoderms wird reguliert durch eine Reihe komplexer Interaktionen von unterschiedlichen Signale wegen. Der Notch/Delta Signalweg spielt dabei eine zentrale Bedeutung, da hierbei Komponenten entdeckt wurden, die während der Somitogenese zyklisch im PSM exprimiert werden. Außer dem Notch/Delta Signalweg spielen auch ein FGF und Retinolsäure Gradient, sowie Wnt Signale eine wichtige Rolle bei der Somitogenese. Trotz mehrerer Mutagenese Screens im Zebrafisch wurden bislang keine Mutanten im FGF oder Wnt Signalweg entdeckt, die einen spezifischen Somiten Defekt besitzen. Die wurde durch eine funktionelle Redundanz unterschiedlicher Gene erklärt, die durch eine Duplikation im Genom von Teleostieren vor 350 Millionen Jahren enstanden ist. Da unterschiedliche Duplikate in verschiedenen Fischspezies existieren, wurde in den letzten Jahren ein grosser Mutagenese Screen bei Medaka (Oryzias latipes) in Kyoto, Japan durchgeführt. In meiner Arbeit habe ich neue Somitogenese Mutanten aus dieser Screen isoliert und Phänotypisch charakterisiert. Die neun isolierten Mutanten zeigten unterschiedliche Somiten Phänotypen. Einige Mutanten hatten wenige oder gar keine Somitengrenzen (z.B bms oder sne), andere hatten unregelmäßige Somiten Formen (z.B. krz oder fsl) oder unterschiedlich große Somiten (z.B dpk). Manche dieser Medaka wiesen Änlichkeiten Mutanten zu im Zebrafisch beschriebenen Somiten Mutanten auf. Die Mehrzahl der Mutanten zeigten jedoch Phänotypen, die bis jetzt noch nicht in Zebrafisch Screens gefunden worden. In-Situ Analysen mit Hilfe unterschiedlicher, neu isolierter Somitenmarker, wie z.B. her7 einem Bestandteil des molekularen Oszillators, mesp einem anterior-posterioren Gen oder den Somitendifferenzierungsgenen lfng oder myf5 erlaubten, die Medaka Mutanten in zwei unterschiedliche Gruppen zuzuordnen. Gruppe I zeigt Defekte in der Bildung der Schwanzknospe und der Musterbildung im PSM. Ein besonderes Beispiel dieser Gruppe ist die Mutante doppelkorn (dpk), die einen bislang nicht beschriebenen Somitenphänotyp besitzt. In-situ Analysen von dpk zeigten, dass zyklische Gene im anterioren PSM dieser Mutante nicht stabilisiert werden und auch A-P Polaritätsgene fehlerhaft reguliert werden. Das deutet darauf hin, dass in der dpk Mutante ein Faktor der sogenannten „Wavefront“ betroffen sein könnte, der wichtig ist für die Regulation von oszillierenden Genen im anterioren PSM ist. Ich konnte zeigen, daß der wichtige Notch/Delta Signalweg in dieser Mutante nicht betroffen ist, weil alle unterschiedlichen zyklischen Gene, her1, her5 und her7, eine normale dynamische initiation ihrer Expression zeigten. Gruppe II Mutanten zeigen Defekte bei der Bildung der Somitengrenzen und Epithelialisierung der Somiten trotz normales, Musterbildung im PSM. Solche Mutanten wurden bislang weder in Zebrafisch, noch in Maus oder Hühnchen gefunden. Deshalb sollten nach der molekularen Identifiezierung der mutierten Gene neue Faktoren erhalten werden, die vor allem für die Regulation später Somitogenese-phasen wichtig sind. KW - Japankärpfling KW - Somit KW - Genanalyse KW - Somiten KW - Präsomitisches Mesoderm KW - Medaka KW - FGF Signalweg KW - Notch/Delta Signalweg KW - Somites KW - Presomitic meoderm KW - Medaka KW - FGF pathway KW - Notch/Delta pathway Y1 - 2005 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-14515 ER -