@article{LakovicPoethkeHovestadt2015, author = {Lakovic, Milica and Poethke, Hans-Joachim and Hovestadt, Thomas}, title = {Dispersal timing: Emigration of insects living in patchy environments}, series = {PLoS One}, volume = {10}, journal = {PLoS One}, number = {7}, doi = {10.1371/journal.pone.0128672}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-126466}, pages = {e0128672}, year = {2015}, abstract = {Dispersal is a life-history trait affecting dynamics and persistence of populations; it evolves under various known selective pressures. Theoretical studies on dispersal typically assume 'natal dispersal', where individuals emigrate right after birth. But emigration may also occur during a later moment within a reproductive season ('breeding dispersal'). For example, some female butterflies first deposit eggs in their natal patch before migrating to other site(s) to continue egg-laying there. How breeding compared to natal dispersal influences the evolution of dispersal has not been explored. To close this gap we used an individual-based simulation approach to analyze (i) the evolution of timing of breeding dispersal in annual organisms, (ii) its influence on dispersal (compared to natal dispersal). Furthermore, we tested (iii) its performance in direct evolutionary contest with individuals following a natal dispersal strategy. Our results show that evolution should typically result in lower dispersal under breeding dispersal, especially when costs of dispersal are low and population size is small. By distributing offspring evenly across two patches, breeding dispersal allows reducing direct sibling competition in the next generation whereas natal dispersal can only reduce trans-generational kin competition by producing highly dispersive offspring in each generation. The added benefit of breeding dispersal is most prominent in patches with small population sizes. Finally, the evolutionary contests show that a breeding dispersal strategy would universally out-compete natal dispersal.}, language = {en} } @phdthesis{Muenz2015, author = {M{\"u}nz, Thomas Sebastian}, title = {Aspects of neuronal plasticity in the mushroom body calyx during adult maturation in the honeybee Apis mellifera}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-111611}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Division of labor represents a major advantage of social insect communities that accounts for their enormous ecological success. In colonies of the honeybee, Apis mellifera, division of labor comprises different tasks of fertile queens and drones (males) and, in general, sterile female workers. Division of labor also occurs among workers in form of an age-related polyethism. This helps them to deal with the great variety of tasks within the colony. After adult eclosion, workers spend around three weeks with various duties inside the hive such as tending the brood or cleaning and building cells. After this period workers switch to outdoor tasks and become foragers collecting nectar, pollen and water. With this behavioral transition, workers face tremendous changes in their sensory environment. In particular, visual sensory stimuli become important, but also the olfactory world changes. Foragers have to perform a completely new behavioral repertoire ranging from long distance navigation based on landmark orientation and polarized-skylight information to learning and memory tasks associated with finding profitable food sources. However, behavioral maturation is not a purely age-related internal program associated with a change, for example, in juvenile hormone titers. External factors such as primer pheromones like the brood pheromone or queen mandibular pheromone can modulate the timing of this transition. In this way colonies are able to flexibly adjust their work force distribution between indoor and outdoor tasks depending on the actual needs of the colony. Besides certain physiological changes, mainly affecting glandular tissue, the transition from indoor to outdoor tasks requires significant adaptations in sensory and higher-order integration centers of the brain. The mushroom bodies integrate olfactory, visual, gustatory and mechanosensory information. Furthermore, they play important roles in learning and memory processes. It is therefore not surprising that the mushroom bodies, in particular their main input region, the calyx, undergo volumetric neuronal plasticity. Similar to behavioral maturation, plastic changes of the mushroom bodies are associated with age, but are also to be affected by modulating factors such as task and experience. In my thesis, I analyzed in detail the neuronal processes underlying volumetric plasticity in the mushroom body. Immunohistochemical labeling of synaptic proteins combined with quantitative 3D confocal imaging revealed that the volume increase of the mushroom body calyx is largely caused by the growth of the Kenyon cell dendritic network. This outgrowth is accompanied by changes in the synaptic architecture of the mushroom body calyx, which is organized in a distinct pattern of synaptic complexes, so called microglomeruli. During the first week of natural adult maturation microglomeruli remain constant in total number. With subsequent behavioral transition from indoor duties to foraging, microglomeruli are pruned while the Kenyon cell dendritic network is still growing. As a result of these processes, the mushroom body calyx neuropil volume enlarges while the total number of microgloumeruli becomes reduced in foragers compared to indoor workers. In the visual subcompartments (calyx collar) this process is induced by visual sensory stimuli as the beginning of pruning correlates with the time window when workers start their first orientation flights. The high level of analysis of cellular and subcellular process underlying structural plasticity of the mushroom body calyx during natural maturation will serve as a framework for future investigations of behavioral plasticity in the honeybee. The transition to foraging is not purely age-dependent, but gets modulated, for example, by the presence of foragers. Ethyl oleate, a primer pheromone that is present only in foragers, was shown to delay the onset of foraging in nurse bees. Using artificial application of additional ethyl oleate in triple cohort colonies, I tested whether it directly affects adult neuronal plasticity in the visual input region of the mushroom body calyx. As the pheromonal treatment failed to induce a clear behavioral phenotype (delayed onset of foraging) it was not possible to show a direct link between the exposure to additional ethyl oleate and neuronal plasticity in mushroom body calyx. However, the general results on synaptic maturation confirmed my data of natural maturation processes in the mushroom body calyx. Given the result that dendritic plasticity is a major contributor to neuronal plasticity in the mushroom body calyx associated with division of labor, the question arose which proteins could be involved in mediating these effects. Calcium/calmodulin-dependent protein kinase II (CaMKII) especially in mammals, but also in insects (Drosophila, Cockroach), was shown to be involved in facilitating learning and memory processes like long-term synaptic potentiation. In addition to presynaptic effects, the protein was also revealed to directly interact with cytoskeleton elements in the postsynapse. It therefore is a likely candidate to mediate structural synaptic plasticity. As part of my thesis, the presence and distribution of CaMKII was analyzed, and the results showed that the protein is highly concentrated in a distinct subpopulation of the mushroom body intrinsic neurons, the noncompact Kenyon cells. The dendritic network of this population arborizes in two calyx subregions: one receiving mainly olfactory input - the lip - and the collar receiving visual input. This distribution pattern did not change with age or task. The high concentration of CaMKII in dendritic spines and its overlap with f-actin indicates that CaMKII could be a key player inducing structural neuronal plasticity associated with learning and memory formation and/or behavioral transitions related to division of labor. Interestingly CaMKII immunoreactivity was absent in the basal ring, another subregion of the mushroom body calyx formed almost exclusively by the inner compact Kenyon cells and known to receive combined visual and olfactory input. This indicates differences of this mushroom body subregion regarding the molecular mechanisms controlling plastic changes in corresponding Kenyon cells. How is timing of behavioral and neuronal plasticity regulated? The primer pheromone ethyl oleate was found in high concentrations on foragers and was shown to influence behavioral maturation by delaying the onset of foraging when artificially applied in elevated concentrations. But how is ethyl oleate transferred and how does it shift the work force distribution between indoor and outdoor tasks? Previous work showed that ethyl oleate concentrations are highest in the honeycrop of foragers and suggested that it is transferred and communicated inside the colony via trophallaxis. The results of this thesis however clearly show, that ethyl oleate was not present inside the honey crop or the regurgitate, but rather in the surrounding tissue of the honey crop. As additionally the second highest concentration of ethyl oleate was measured on the surface of the cuticle of forgers, trophallaxis was ruled out as a mode of transmission. Neurophysiological measurements at the level of the antennae (electroantennogram recordings) and the first olfactory neuropil (calcium imaging of activity in the antennal lobe) revealed that the primer pheromone ethyl oleate is received and processed as an olfactory stimulus. Appetitive olfactory conditioning using the proboscis extension response as a behavioral paradigm showed that ethyl oleate can be associated with a sugar reward. This indicates that workers are able to perceive, learn and memorize the presence of this pheromone. As ethyl oleate had to be presented by a heated stimulation device at close range, it can be concluded that this primer pheromone acts via close range/contact chemoreception through the olfactory system. This is also supported by previous behavioral observations. Taken together, the findings presented in this thesis revealed structural changes in the synaptic architecture of the mushroom body calyx associated with division of labor. For the primer pheromone ethyl oleate, which modulates the transition from nursing to foraging, the results clearly showed that it is received via the olfactory system and presumably acts via this pathway. However, manipulation experiments did not indicate a direct effect of ethyl oleate on synaptic plasticity. At the molecular level, CaMKII is a prime candidate to mediate structural synaptic plasticity in the mushroom body calyx. Future combined structural and functional experiments are needed to finally link the activity of primer pheromones like ethyl oleate to the molecular pathways mediating behavioral and synaptic plasticity associated with division of labor in Apis mellifera. The here identified underlying processes will serve as excellent models for a general understanding of fundamental mechanisms promoting behavioral plasticity.}, subject = {Biene}, language = {en} } @phdthesis{Stoll2015, author = {Stoll, Georg}, title = {Identification of the mRNA-associated TOP3β- TDRD3-FMRP (TTF) -complex and its implication for neurological disorders}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-111440}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {The propagation of the genetic information into proteins is mediated by messenger- RNA (mRNA) intermediates. In eukaryotes mRNAs are synthesized by RNA- Polymerase II and subjected to translation after various processing steps. Earlier it was suspected that the regulation of gene expression occurs primarily on the level of transcription. In the meantime it became evident that the contribution of post- transcriptional events is at least equally important. Apart from non-coding RNAs and metabolites, this process is in particular controlled by RNA-binding proteins, which assemble on mRNAs in various combinations to establish the so-called "mRNP- code". In this thesis a so far unknown component of the mRNP-code was identified and characterized. It constitutes a hetero-trimeric complex composed of the Tudor domain-containing protein 3 (TDRD3), the fragile X mental retardation protein (FMRP) and the Topoisomerase III beta (TOP3β) and was termed TTF (TOP3β-TDRD3-FMRP) -complex according to its composition. The presented results also demonstrate that all components of the TTF-complex shuttle between the nucleus and the cytoplasm, but are predominantly located in the latter compartment under steady state conditions. Apart from that, an association of the TTF-complex with fully processed mRNAs, not yet engaged in productive translation, was detected. Hence, the TTF-complex is a component of „early" mRNPs. The defined recruitment of the TTF-complex to these mRNPs is not based on binding to distinct mRNA sequence-elements in cis, but rather on an interaction with the so-called exon junction complex (EJC), which is loaded onto the mRNA during the process of pre-mRNA splicing. In this context TDRD3 functions as an adapter, linking EJC, FMRP and TOP3β on the mRNP. Moreover, preliminary results suggest that epigenetic marks within gene promoter regions predetermine the transfer of the TTF-complex onto its target mRNAs. Besides, the observation that TOP3β is able to catalytically convert RNA-substrates disclosed potential activities of the TTF-complex in mRNA metabolism. In combination with the already known functions of FMRP, this finding primarily suggests that the TTF-complex controls the translation of bound mRNAs. In addition to its role in mRNA metabolism, the TTF-complex is interesting from a human genetics perspective as well. It was demonstrated in collaboration with researchers from Finland and the US that apart from FMRP, which was previously linked to neurocognitive diseases, also TOP3β is associated with neurodevelopmental disorders. Understanding the function of the TTF-complex in mRNA metabolism might hence provide important insight into the etiology of these diseases.}, subject = {Messenger-RNS}, language = {en} } @phdthesis{Schmitt2015, author = {Schmitt, Alexandra}, title = {Role of Peroxiredoxin 6 in human melanoma}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-111465}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Peroxiredoxin 6 (PRDX6) is a bifunctional enzyme comprising a peroxidase and a Ca2+-independent phospholipase (iPLA2) activity. This renders the enzyme capable of detoxifying reactive oxygen species (ROS) and of catalyzing the liberation of arachidonic acid (AA) from cellular membranes. Released AA can be further metabolized to bioactive lipids including eicosanoids, which are involved in inflammation, cell growth, differentiation, invasion and proliferation. Human melanoma cells are often characterized by imbalances in both ROS and lipid levels, which can be generated by oncogenic signaling, altered metabolism or UV irradiation. In previous studies, a comparative proteome analysis of the Xiphophorus fish melanoma model revealed a strong upregulation of Prdx6 in benign and malignant lesions compared to healthy skin. As the Xiphophorus melanoma model displays in many respects molecular characteristics that are similar to human melanoma, I investigated the functional role of PRDX6 in human melanoma cells. The first part of the study deals with the regulation of PRDX6 in melanocytes and human melanoma cells. I could demonstrate that the protein level of PRDX6 was strongly enhanced by the induction of the EGFR orthologue Xmrk from the Xiphophorus fish as well as the human EGFR. The upregulation of PRDX6 was further shown to be mediated in a PI3K-dependent and ROS-independent manner. The main part of the thesis comprises the investigation of the functional role of PRDX6 in human melanoma cells as well as the analysis of the underlying mechanism. I could show that knockdown of PRDX6 enhanced the oxidative stress response and led to decreased proliferation of melanoma cells. This cell growth effect was mainly mediated by the iPLA2 activity of PRDX6. Under conditions of strongly enhanced oxidative stress, the peroxidase activity became also important for cellular proliferation. Furthermore, the anti-proliferative effect in cells with lowered PRDX6 levels was the result of reduced cellular AA content and the decrease in the activation of SRC family proteins. Similarly, supplementation with AA led to regeneration of SRC family kinase activity and to an improvement in the reduced proliferation after knockdown of PRDX6. Since AA can be further processed into the prostaglandin PGE2, which has a pro-tumorigenic function in some cancer types, I further examined whether this eicosanoid is involved in the proliferative function of PRDX6. In contrast to AA, PGE2 was not consistently required for melanoma proliferation. In summary, I could demonstrate that PRDX6 plays a major role in AA-dependent lipid signaling in melanoma cells and thereby regulates proliferation. Interestingly, the proliferation relevant iPLA2 activity can be pharmacologically targeted, and melanoma cell growth was clearly blocked by the inhibitor BEL. Thus, I could identify the phospholipase activity of PRDX6 as a new therapeutically interesting target for melanoma treatment.}, subject = {Melanom}, language = {en} } @phdthesis{Fliesser2015, author = {Fließer, Mirjam}, title = {Hypoxia and hypoxia-inducible factor 1α modulate the immune response of human dendritic cells against Aspergillus fumigatus}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-121392}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {The mold Aspergillus fumigatus causes life-threatening infections in immunocompromised patients. Over the past decade new findings in research have improved our understanding of A. fumigatus-host interactions. One of them was the detection of localized areas of tissue hypoxia in the lungs of mice infected with A. fumigatus. The transcription factor hypoxia-inducible factor 1α (HIF 1α) is known as the central regulator of cellular responses to hypoxia. Under normoxia, this constitutively expressed protein is degraded by oxygen-dependent mechanisms in most mammalian cell types. Interaction with pathogens can induce HIF 1α stabilization under normoxic conditions in innate immune cells. Bacterial infection models revealed that hypoxic microenvironments and signaling via HIF 1α modulate functions of host immune cells. Moreover, it was recently described that in murine phagocytes, HIF 1α expression is essential to overcome an A. fumigatus infection. However, the influence of hypoxia and the role of HIF 1α signaling for anti-A. fumigatus immunity is still poorly understood, especially regarding dendritic cells (DCs), which are important regulators of anti-fungal immunity. In this study, the functional relevance of hypoxia and HIF 1α signaling in the response of human DCs against A. fumigatus has been investigated. Hypoxia attenuated the pro-inflammatory response of DCs against A. fumigatus during the initial infection as shown by genome-wide microarray expression analyses and cytokine quantification. The up-regulation of maturation-associated molecules on DCs stimulated with A. fumigatus under hypoxia was reduced; however, these DCs possessed an enhanced capacity to stimulate T cells. This study thereby revealed divergent influence of hypoxia on anti-A. fumigatus DC functions that included both, inhibiting and enhancing effects. HIF-1α was stabilized in DCs following stimulation with A. fumigatus under normoxic and hypoxic conditions. This stabilization was partially dependent on Dectin-1, the major receptor for A. fumigatus on human DCs. Using siRNA-based HIF 1α silencing combined with gene expression microarrays, a modulatory effect of HIF-1α on the anti-fungal immune response of human DCs was identified. Specifically, the transcriptomes of HIF-1α silenced DCs indicated that HIF-1α enhanced DC metabolism and cytokine release in response to A. fumigatus under normoxic and hypoxic conditions. This was confirmed by further down-stream analyses that included quantification of glycolytic activity and cytokine profiling of DCs. By that, this study demonstrated functional relevance of HIF 1α expression in DCs responding to A. fumigatus. The data give novel insight into the cellular functions of HIF 1α in human DCs that include regulation of the anti-fungal immune response under normoxia and hypoxia. The comprehensive transcriptome datasets in combination with the down-stream protein analyses from this study will promote further investigations to further characterize the complex interplay between hypoxia, activation of Dectin-1 and HIF-1α signaling in host responses against A. fumigatus.}, subject = {Immunologie}, language = {en} } @phdthesis{Frank2015, author = {Frank, Nicolas Clemens}, title = {Lokale axonale Wirkungen der CNTF-STAT3 Signalkaskade in Motoneuronen der pmn Maus - einem Mausmodel f{\"u}r die Amyotrophe Lateralsklerose}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-121065}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {1. Zusammenfassung W{\"a}hrend der Embryogenese und nach Verletzungen von Nerven regulieren neurotrophe Faktoren Signalwege f{\"u}r Apoptose, Differenzierung, Wachstum und Regeneration von Neuronen. In vivo Experimente an neugeborenen Nagern haben gezeigt, dass der Verlust von Motoneuronen nach peripherer Nervenl{\"a}sion durch die Behandlung mit GDNF, BDNF, und CNTF reduziert werden kann In der pmn-Mausmutante, einem Modell f{\"u}r die Amyotrophe Lateralsklerose, f{\"u}hrt die Gabe von CNTF, nicht aber von GDNF zu einem verz{\"o}gerten Krankheitsbeginn und einem verlangsamten Fortschreiten der Motoneuronendegeneration. Ausl{\"o}ser der Motoneuronendegeneration in der pmn-Maus ist eine Mutation im Tubulin spezifischen Chaperon E (Tbce) Gen, das f{\"u}r eines von f{\"u}nf Tubulin spezifischen Chaperonen (TBCA-TBCE) kodiert und an der Bildung von -Tubulinheterodimeren beteiligt ist. Diese Arbeit sollte dazu beitragen, die CNTF-induzierten Signalwege zu entschl{\"u}sseln, die sich lindernd auf den progredienten Verlauf der Motoneuronendegeneration in der pmn-Maus auswirken. Prim{\"a}re pmn mutierte Motoneurone zeigen ein reduziertes Axonwachstum und eine erh{\"o}hte Anzahl axonaler Schwellungen mit einer anomalen H{\"a}ufung von Mitochondrien - ein fr{\"u}hes Erkennungsmerkmal bei ALS-Patienten. Die Applikation von CNTF nicht aber von BDNF oder GDNF, kann in vitro die beobachteten Wachstumsdefekte und das bidirektionale axonale Transportdefizit in pmn mutierten Motoneurone verhindern. Aus {\"a}lteren Untersuchungen war bekannt, dass CNTF {\"u}ber den dreiteiligen transmembranen Rezeptorkomplex, bestehend aus CNTFR, LIFR und gp130, Januskinasen aktiviert, die STAT3 an Tyrosin 705 phosphorylieren (pSTAT3Y705). Ich konnte beobachten, dass axonales fluoreszenzmarkiertes pSTAT3Y705 nach CNTF-Gabe nicht retrograd in den Nukleus transportiert wird. Stattdessen f{\"u}hrt die CNTF-induzierte Phosphorylierung von STAT3 an Tyrosin 705 zu einer transkriptionsunabh{\"a}ngigen lokalen Reaktion im Axon. Diese pSTAT3Y705 abh{\"a}ngige Reaktion ist notwendig und ausreichend, um das reduzierte Axonwachstum pmn mutierter Motoneurone zu beheben. Wie die Kombination einer CNTF Behandlung mit dem shRNA vermittelten knock-down von Stathmin in pmn mutierten Motoneuronen zeigt, zielt die CNTF-STAT3 Signalkaskade auf die Stabilisierung axonaler Mikrotubuli ab und wirkt sich positiv auf die anterograde und retrograde Mobilit{\"a}t von axonalen Mitochondrien aus. Interessanter Weise konnte ich außerdem feststellen, dass eine akute Gabe von CNTF das mitochondriale Membranpotential in Axonen prim{\"a}rer pmn mutierter und wildtypischer Motoneurone erh{\"o}ht und einen Anstieg von ATP ausl{\"o}st. Meine Beobachtungen legen nahe, dass CNTF unerwarteter Weise auch eine transiente Phosphorylierung an STAT3 Serin 727 (pSTAT3S727) ausl{\"o}st, die zur anschließenden Translokation von pSTAT3S727 in Mitochondrien f{\"u}hrt. Diese Ergebnisse zeigen, dass STAT3 mehrere lokale Ziele im Axon besitzt, n{\"a}mlich axonale Mikrotubuli und Mitochondrien.}, subject = {Motoneuron}, language = {de} } @phdthesis{Hafen2015, author = {Hafen, Bettina}, title = {Physical contact between mesenchymal stem cells and endothelial precursors induces distinct signatures with relevance to tissue regeneration and engineering}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-119417}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {The goal of the project VascuBone is to develop a tool box for bone regeneration, which on one hand fulfills basic requirements (e.g. biocompatibility, properties of the surface, strength of the biomaterials) and on the other hand is freely combinable with what is needed in the respective patient's situation. The tool box will include a variation of biocompatible biomaterials and cell types, FDA-approved growth factors, material modification technologies, simulation and analytical tools like molecular imaging-based in vivo diagnostics, which can be combined for the specific medical need. This tool box will be used to develop translational approaches for regenerative therapies of different types of bone defects. This project receives funding from the European Union's Seventh Framework Program (VascuBone 2010). The present study is embedded into this EU project. The intention of this study is to assess the changes of the global gene expression patterns of endothelial progenitor cells (EPCs) and mesenchymal stem cells (MSCs) after direct cell-cell contact as well as the influence of conditioned medium gained from MSCs on EPCs and vice versa. EPCs play an important role in postnatal vasculogenesis. An intact blood vessel system is crucial for all tissues, including bone. Latest findings in the field of bone fracture healing and repair by the use of tissue engineering constructs seeded with MSCs raised the idea of combining MSCs and EPCs to enhance vascularization and therefore support survival of the newly built bone tissue. RNA samples from both experimental set ups were hybridized on Affymetrix GeneChips® HG-U133 Plus 2.0 and analyzed by microarray technology. Bioinformatic analysis was applied to the microarray data and verified by RT-PCR. This study gives detailed information on how EPCs and MSCs communicate with each other and therefore gives insights into the signaling pathways of the musculoskeletal system. These insights will be the base for further functional studies on protein level for the purpose of tissue regeneration. A better understanding of the cell communication of MSCs and EPCs and subsequently the targeting of relevant factors opens a variety of new opportunities, especially in the field of tissue engineering. The second part of the present work was to develop an ELISA (enzyme-linked immunosorbent assay) for a target protein from the lists of differentially expressed genes revealed by the microarray analysis. This project was in cooperation with Immundiagnostik AG, Bensheim, Germany. The development of the ELISA aimed to have an in vitro diagnostic tool to monitor e.g. the quality of cell seeded tissue engineering constructs. The target protein chosen from the lists was klotho. Klotho seemed to be a very promising candidate since it is described in the literature as anti-aging protein. Furthermore, studies with klotho knock-out mice showed that these animals suffered from several age-related diseases e.g. osteoporosis and atherosclerosis. As a co-receptor for FGF23, klotho plays an important role in bone metabolism. The present study will be the first one to show that klotho is up-regulated in EPCs after direct cell-cell contact with MSCs. The development of an assay with a high sensitivity on one hand and the capacity to differentiate between secreted and shedded klotho on the other hand will allow further functional studies of this protein and offers a new opportunity in medical diagnostics especially in the field of metabolic bone disease.}, subject = {Vorl{\"a}uferzelle}, language = {en} } @article{GalluzziBravoSanPedroVitaleetal.2015, author = {Galluzzi, L. and Bravo-San Pedro, J. M. and Vitale, I. and Aaronson, S. A. and Abrams, J. M. and Adam, D. and Alnemri, E. S. and Altucci, L. and Andrews, D. and Annicchiarico-Petruzelli, M. and Baehrecke, E. H. and Bazan, N. G. and Bertrand, M. J. and Bianchi, K. and Blagosklonny, M. V. and Blomgren, K. and Borner, C. and Bredesen, D. E. and Brenner, C. and Campanella, M. and Candi, E. and Cecconi, F. and Chan, F. K. and Chandel, N. S. and Cheng, E. H. and Chipuk, J. E. and Cidlowski, J. A. and Ciechanover, A. and Dawson, T. M. and Dawson, V. L. and De Laurenzi, V. and De Maria, R. and Debatin, K. M. and Di Daniele, N. and Dixit, V. M. and Dynlacht, B. D. and El-Deiry, W. S. and Fimia, G. M. and Flavell, R. A. and Fulda, S. and Garrido, C. and Gougeon, M. L. and Green, D. R. and Gronemeyer, H. and Hajnoczky, G. and Hardwick, J. M. and Hengartner, M. O. and Ichijo, H. and Joseph, B. and Jost, P. J. and Kaufmann, T. and Kepp, O. and Klionsky, D. J. and Knight, R. A. and Kumar, S. and Lemasters, J. J. and Levine, B. and Linkermann, A. and Lipton, S. A. and Lockshin, R. A. and L{\´o}pez-Ot{\´i}n, C. and Lugli, E. and Madeo, F. and Malorni, W. and Marine, J. C. and Martin, S. J. and Martinou, J. C. and Medema, J. P. and Meier, P. and Melino, S. and Mizushima, N. and Moll, U. and Mu{\~n}oz-Pinedo, C. and Nu{\~n}ez, G. and Oberst, A. and Panaretakis, T. and Penninger, J. M. and Peter, M. E. and Piacentini, M. and Pinton, P. and Prehn, J. H. and Puthalakath, H. and Rabinovich, G. A. and Ravichandran, K. S. and Rizzuto, R. and Rodrigues, C. M. and Rubinsztein, D. C. and Rudel, T. and Shi, Y. and Simon, H. U. and Stockwell, B. R. and Szabadkai, G. and Tait, S. W. and Tang, H. L. and Tavernarakis, N. and Tsujimoto, Y. and Vanden Berghe, T. and Vandenabeele, P. and Villunger, A. and Wagner, E. F. and Walczak, H. and White, E. and Wood, W. G. and Yuan, J. and Zakeri, Z. and Zhivotovsky, B. and Melino, G. and Kroemer, G.}, title = {Essential versus accessory aspects of cell death: recommendations of the NCCD 2015}, series = {Cell Death and Differentiation}, volume = {22}, journal = {Cell Death and Differentiation}, doi = {10.1038/cdd.2014.137}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-121207}, pages = {58-73}, year = {2015}, abstract = {Cells exposed to extreme physicochemical or mechanical stimuli die in an uncontrollable manner, as a result of their immediate structural breakdown. Such an unavoidable variant of cellular demise is generally referred to as 'accidental cell death' (ACD). In most settings, however, cell death is initiated by a genetically encoded apparatus, correlating with the fact that its course can be altered by pharmacologic or genetic interventions. 'Regulated cell death' (RCD) can occur as part of physiologic programs or can be activated once adaptive responses to perturbations of the extracellular or intracellular microenvironment fail. The biochemical phenomena that accompany RCD may be harnessed to classify it into a few subtypes, which often (but not always) exhibit stereotyped morphologic features. Nonetheless, efficiently inhibiting the processes that are commonly thought to cause RCD, such as the activation of executioner caspases in the course of apoptosis, does not exert true cytoprotective effects in the mammalian system, but simply alters the kinetics of cellular demise as it shifts its morphologic and biochemical correlates. Conversely, bona fide cytoprotection can be achieved by inhibiting the transduction of lethal signals in the early phases of the process, when adaptive responses are still operational. Thus, the mechanisms that truly execute RCD may be less understood, less inhibitable and perhaps more homogeneous than previously thought. Here, the Nomenclature Committee on Cell Death formulates a set of recommendations to help scientists and researchers to discriminate between essential and accessory aspects of cell death.}, language = {en} } @phdthesis{Endt2015, author = {Endt, Daniela}, title = {Fanconi An{\"a}mie : Entwicklung von h{\"a}matopoetischen Mosaiken sowie funktionelle Studien von FANCO (RAD51C) und FANCN (PALB2)}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-127836}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Zur Wahrung der Genomstabilit{\"a}t entwickelten sich verschiedene Reparaturmechanismen, deren Defekte zu diversen Erkrankungen f{\"u}hren. Der 1927 erstmals beschriebenen Fanconi An{\"a}mie (FA) (Fanconi 1927) liegt eine fehlerhafte Reparatur der DNA-Doppelstrang-Quervernetzung zugrunde. Als Ursache wurden Defekte innerhalb des FA/BRCA-Weges lokalisiert, welche zur Chromosomeninstabilit{\"a}t f{\"u}hren. Das Krankheitsbild der autosomal rezessiven oder X-chromosomalen Erkrankung wird meist von kongenitalen Fehlbildungen, progressivem Knochenmarkversagen sowie bereits im jugendlichen Alter erh{\"o}hten Tumor-raten und An{\"a}mien gepr{\"a}gt. Bisher wurden Defekte in 19 verschiedenen Genen als urs{\"a}chlich f{\"u}r diese Erkrankung diskutiert. Anhand des betroffenen Gens k{\"o}nnen nur begrenzt R{\"u}ckschl{\"u}sse auf die Auspr{\"a}-gung des Ph{\"a}notyps geschlossen werden, vielmehr scheinen die Art der Mutation und deren Position im Gen mit der Schwere der Erkrankung zu korrelieren. Im Laufe der Zeit wurden immer mehr Patienten mit mild ausgepr{\"a}gtem Erkrankungsbild beobachtet. Eine m{\"o}gliche Erkl{\"a}rung hierf{\"u}r liefern milde Mutationen, eine weitere das Vorhandensein von Mosaiken blutbildender Zellen. Zu letzterem f{\"u}hrt die Reversion einer der beiden Mutationen. Diese Art der „nat{\"u}rlichen Gentherapie" wurde bei 10-30\% der FA-Patienten beobachtet. Um die Entwicklung von Reversionen besser zu verstehen, erfolgte im Rahmen dieser Arbeit die Untersuchung verschiedener Zelllinien von 5 Patienten im Alter von 11 (Pat. 5) bis 33 (Pat. 4) Jahren. Die FA-A-Patienten 1 und 2 wurden bereits von Gross et al. 2002 als Mosaikpatienten beschrieben. F{\"u}r die weiteren Patienten f{\"u}hrten unterschiedliche Aspekte, wie normale Blutwerte, MMC-tolerante lympho-blastoide Zelllinien und gDNA-Analysen des Blutes zum Mosaikverdacht. N{\"a}here Analysen best{\"a}tigten f{\"u}r die FA-D2-Patienten (Pat. 4, 5) ebenfalls das Vorliegen einer Reversion in den Blutzellen. Allen Patienten gemein war die Reversion in Form einer R{\"u}ckmutation (Pat. 1: c.971T>G, Pat. 2: c.856 C>T, Pat. 4: c.3467-2A>G, Pat. 5: c.3707G>A), welche meist in einem oder in der N{\"a}he eines Mutationsmotives vorlag. Zur Einsch{\"a}tzung des Mosaikstatus in den Patientenblutzellen wurden, neben der meist mehrj{\"a}hrigen Be-obachtung der Blutwerte (Thrombo-, Mono-, Granulo-, Lymphozyten, H{\"a}moglobin), gDNA-, Chromoso-menbruch- und Zellzyklusanalysen durchgef{\"u}hrt. Chromosomenbruchanalysen von Metaphasen der T-Lymphozyten der Patienten 4 und 5 zeigten nach MMC-Behandlung die mosaik-typische bimodale Vertei-lung der Chromosomenbruchraten. Die nur moderat erh{\"o}hten Bruchraten in Metaphasen des Patienten 1 sprachen f{\"u}r eine starke Reversion. Zur besseren Absch{\"a}tzung des Mosaikstatus wurden Zellzyklusanaly-sen an Mischungsreihen aus FA- und nicht FA- Blut durchgef{\"u}hrt. Die Detektionsgrenze f{\"u}r FA-Mosaike lag bei einem Anteil von 30\% Zellen mit spontanem/MMC-induziertem G2-Phasen-Arrest. In Anlehnung an Mischungskurven wurden f{\"u}r die vier Patienten Reversionen von 0\% (Pat. 4) bis 90-95\% (Pat. 2) ange-nommen. Die gDNA-Analyse MACS-sortierter T-/B-Lympho-, Mono- und Granulozyten sowie von Fib-roblasten und lymphoblastoiden Zelllinien erm{\"o}glichte einen detaillierten Einblick in die Mosaikstatus auf molekularer Ebene. Wir fanden bei allen Patienten einen unterschiedlich stark ausgepr{\"a}gten Mosaikstatus ihrer Blutzellreihen. Tendenziell scheinen die Reversionsgrade mit der Zell-Lebensdauer korrelieren, hier-bei zeigen kurzlebige Zellen (Mono-, Granulo-, B-Lymphozyten) h{\"o}here Reversionsgrade als langlebige T-Lymphozyten. Das Auftreten von gleichen Reversionen in allen Zelllinien l{\"a}sst eine Reversion in einer gemeinsamen Vorl{\"a}uferzelle vermuten. Als Besonderheit fanden wir, unseren Erachtens erstmalig, eine komplette Reversion einer Knochenmark-Fibroblastenzelllinie (Pat. 1). H{\"a}ufig in Kultur stattfindende Re-versionen in lymphoblastoiden Zelllinien beobachteten wir f{\"u}r alle vier Patienten. Die Mosaikentstehung im Patientenblut konnte mit allen Methoden best{\"a}tigt werden. Jede Methode wies Vor- und Nachteile auf. Zur Absch{\"a}tzung der Mosaikstatus empfiehlt sich deshalb eine Kombination der Methoden. Ein weiteres Projekt besch{\"a}ftigte sich mit Interaktionen des FANCO (RAD51C) innerhalb der RAD51 Paraloge (RAD51B, -C, -D, XRCC2, XRCC3) und mit RAD51. Die Analysen erfolgten im Mammalian Two- und Three-Hybrid (M2H/M3H) System. Die Untersuchungen best{\"a}tigten die meisten der bisher detektierten Interaktionen, welche zur Ausbildung des RAD51C-XRCC3 Komplexes und des, aus den Subkomplexen RAD51B-RAD51C (BC) und RAD51D-XRCC2 (DX2) bestehenden, BCDX2-Komplex f{\"u}hren. Die M3H-Analysen weisen auf eine wichtige Rolle des RAD51B-Proteins bei der Auspr{\"a}gung dieses Komplexes hin. Es scheint die Ausbildung der RAD51C-RAD51D-Interaktion erst zu erm{\"o}glichen und zus{\"a}tzlich, anders als bisher beobachtet, auch mit XRCC2 zu interagieren. Diese Interaktion wiederum wird durch die Anwesenheit von RAD51D stark gef{\"o}rdert. Unsere M2H-/M3H-Beobachtungen weisen darauf hin, dass die Ausbildung der Subkomplexe f{\"u}r die Entstehung des BDCX2-Komplexes wichtig ist und dieser vermutlich als Ringstruktur vorliegt. Zus{\"a}tzlich fanden wir Hinweise auf m{\"o}gliche Wechselwir-kungen zwischen den BCDX2- und den XRCC3-Komplexproteinen. Aufgrund der Beteiligung der Protei-ne an der Doppelstrangl{\"a}sionsreparatur wurde die Auswirkung von MMC-induzierten DNA-Sch{\"a}den un-tersucht. Diese f{\"u}hrten innerhalb der Subkomplexe zu gegens{\"a}tzlichen {\"A}nderungen der Interaktionsinten-sit{\"a}t. W{\"a}hrend die Substanz im DX2-Komplex zum Sinken der Interaktionsst{\"a}rke f{\"u}hrte, erh{\"o}hte sich diese im BC-Komplex. Die in der Literatur beschriebene und charakterisierte RAD51C-FANCN-Interation war im M2H-Test nicht darstellbar. M{\"o}glicherweise w{\"u}rde diese jedoch durch die Anwesenheit eines drit-ten Proteins gef{\"o}rdert werden. Zus{\"a}tzlich wurde ein RAD51C-Protein, welches die Patientenmutation R258H enthielt, {\"u}berpr{\"u}ft. Es zeigte nur in der M3H-Analyse, mit pMRAD51D und nativem RAD51B, nach Behandlung mit MMC eine reduzierte Interaktionsst{\"a}rke im Vergleich zum Wildtyp. Dies unter-streicht einmal mehr die als hypomorph beschriebene Mutation des Proteins. Das dritte Projekt, die angestrebte Strukturaufkl{\"a}rung des RAD51C-Proteins erwies sich als schwierig. Eine f{\"u}r eine Kristallisation ausreichende Proteinmenge konnte, weder im E. coli-System noch in Insektenzellen oder in Co-Expression mit seinem Interaktionspartner XRCC3, isoliert und aufgereinigt werden. Elektro-phoretische Mobility Shift Assays des CX3-Proteinkomplexes mit DNA-Strukturen (ssDNA, Open Fork, 3'-/ 5'-{\"U}berhang-Struktur), zeigten eine Bevorzugung des 3'-{\"U}berhang-DNA-Substrates. Diese Art der Analyse k{\"o}nnte in weiterf{\"u}hrenden Analysen zur Absch{\"a}tzung der Auswirkung von Patientenmutationen herangezogen werden. bb}, subject = {Fanconi An{\"a}mie}, language = {de} } @article{BrillMeyerRoessler2015, author = {Brill, Martin F. and Meyer, Anneke and Roessler, Wolfgang}, title = {It takes two—coincidence coding within the dual olfactory pathway of the honeybee}, series = {Frontiers in Physiology}, volume = {6}, journal = {Frontiers in Physiology}, number = {208}, doi = {10.3389/fphys.2015.00208}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-126179}, year = {2015}, abstract = {To rapidly process biologically relevant stimuli, sensory systems have developed a broad variety of coding mechanisms like parallel processing and coincidence detection. Parallel processing (e.g., in the visual system), increases both computational capacity and processing speed by simultaneously coding different aspects of the same stimulus. Coincidence detection is an efficient way to integrate information from different sources. Coincidence has been shown to promote associative learning and memory or stimulus feature detection (e.g., in auditory delay lines). Within the dual olfactory pathway of the honeybee both of these mechanisms might be implemented by uniglomerular projection neurons (PNs) that transfer information from the primary olfactory centers, the antennal lobe (AL), to a multimodal integration center, the mushroom body (MB). PNs from anatomically distinct tracts respond to the same stimulus space, but have different physiological properties, characteristics that are prerequisites for parallel processing of different stimulus aspects. However, the PN pathways also display mirror-imaged like anatomical trajectories that resemble neuronal coincidence detectors as known from auditory delay lines. To investigate temporal processing of olfactory information, we recorded PN odor responses simultaneously from both tracts and measured coincident activity of PNs within and between tracts. Our results show that coincidence levels are different within each of the two tracts. Coincidence also occurs between tracts, but to a minor extent compared to coincidence within tracts. Taken together our findings support the relevance of spike timing in coding of olfactory information (temporal code).}, language = {en} } @phdthesis{Pusch2015, author = {Pusch, Tobias}, title = {The transcription factor NFATc1 mediates cytotoxic T cell function in vitro and in vivo}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-123690}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {While numerous experiments on NFAT were already performed with CD4+ T cells showing defective cytokine release and a reduced T helper cell development, no detailed studies existed for CD8+ T cells. From this point, we wanted to examine the impact of NFATc1 and c2 on the physiological functions of CD8+ T cells in vitro and in vivo. Therefore, we used a murine infection model with the bacteria Listeria monocytogenes and mice in which NFATc1 was specifically depleted in the T cell compartment. Our first in vitro studies showed a typical NFATc1 and c2 nuclear translocation and changes on mRNA levels upon T cell activation similarly in CD4+ as well as in CD8+ T cells extracted from wild type mice. NFAT nuclear translocation is important for target gene activation and generation of effector functions. Stimulated T cell populations lacking NFATc1 and/or NFATc2 showed a markedly decreased expression of Th1/Tc1 cytokines, as e.g. IL 2 and IFNγ being important for the clearance of intracellular pathogens. From our in vitro model for the generation of allogenically reactive cytotoxic CD8+ T cells, we revealed a decreased killing and lytic granule-release capacity in Nfatc1 inactivated CD8+ T cells whereas NFATc2-/- cytotoxic T cells did not show an altered cytotoxic response compared to wild type cells. Interestingly, we found lytic granules accumulated and mitochondria not getting translocated to the immunological synapse upon re-stimulation in NFATc1-deficient CD8+ T cells. Together with results showing the CsA insensitivity of the CTL killing/degranulation capacities, we assume that some major cellular processes are affected by NFATc1 which are not directly linked to the TCR-induced signal transduction cascade. We also showed the importance of NFATc1 in T cells during intracellular infections with the bacteria Listeria monocytogenes in an in vivo mouse model. After five days, only few bacteria were detected in wt mice whereas high amounts of Listeria particles were extracted from livers of Nfatc1fl/fl x Cd4 cre mice. Although the reactivity towards the pathogen was similar in both groups, a decreased cytokine expression in NFATc1-/- CD8+ T cells was observed together with an altered memory cell generation. Our results show the importance of NFATc1 in CD8+ T cells and give some clue for a possible connection to other basal cellular functions, as e.g. the formation of an immunological synapse.}, subject = {Transkriptionsfaktor}, language = {en} } @phdthesis{Dusik2015, author = {Dusik, Verena}, title = {Immunhistochemische und funktionelle Charakterisierung der Mitogen-aktivierten Proteinkinase p38 in der inneren Uhr von Drosophila melanogaster}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-124636}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Circadianes und Stress-System sind zwei physiologische Systeme, die dem Organismus helfen sich an Ver{\"a}nderungen ihrer Umwelt anzupassen. W{\"a}hrend letzteres spontane und schnelle Antworten auf akute, unvorhersehbare Umweltreize liefert, sagt das circadiane System t{\"a}glich wiederkehrende Ereignisse vorher and bereitet den Organismus so vorzeitig auf diese nahende Umweltver{\"a}nderung vor. Dennoch, trotz dieser unterschiedlichen Reaktionsmechanismen agieren beide Systeme nicht komplett autonom. Studien der vergangen Jahre belegen vielmehr eine Interaktion beider Systeme. So postulieren sie zum einem Unterschiede in der Stressantwort in Abh{\"a}ngigkeit von der Tageszeit zu der der Reiz auftritt und weisen zugleich auf eine Zunahme von gest{\"o}rten biologischen Tagesrhythmen, wie zum Beispiel Schlafst{\"o}rungen, in Folge von unkontrollierten oder exzessiven Stress hin. Ebenso liefern k{\"u}rzlich durchgef{\"u}hrte Studien an Vertebraten und Pilzen Hinweise, dass mit p38, eine Stress-aktivierte Kinase, an der Signalweiterleitung zur inneren Uhr beteiligt ist (Hayashi et al., 2003), sogar durch dieses endogene Zeitmesssystem reguliert wird (Vitalini et al., 2007; Lamb et al., 2011) und deuten damit erstmals eine m{\"o}gliche Verbindung zwischen Stress-induzierten und regul{\"a}ren rhythmischen Anpassungen des Organismus an Umweltver{\"a}nderungen an. Molekulare und zellul{\"a}re Mechanismen dieser Verkn{\"u}pfung sind bisher noch nicht bekannt. W{\"a}hrend die Rolle von p38 MAPK bei der Stress- und Immunantwort in Drosophila melanogaster gut charakterisiert ist, wurden Expression und Funktion von p38 in der inneren Uhr hingegen bislang nicht untersucht. Die hier vorliegende Arbeit hatte daher zum Ziel mittels immunhistochemischer, verhaltensphysiologischer und molekularer Methoden eine m{\"o}gliche Rolle der Stress-aktivierten Kinase im circadianen System der Fliege aufzudecken. Antik{\"o}rperf{\"a}rbungen sowie Studien mit Reporterlinien zeigen deutliche F{\"a}rbesignale in den s-LNv, l-LNv und DN1a und erbringen erstmals einen Nachweis f{\"u}r p38 Expression in den Uhrneuronen der Fliege. Ebenso scheint die Aktivit{\"a}t von p38 MAPK in den DN1a uhrgesteuert zu sein. So liegt p38 vermehrt in seiner aktiven Form in der Dunkelphase vor und zeigt, neben seiner circadian regulierten Aktivierung, zus{\"a}tzlich auch eine Inaktivierung durch Licht. 15-Minuten-Lichtpulse in der subjektiven Nacht f{\"u}hren zu einer signifikanten Reduktion von aktivierter, phosphorylierter p38 MAPK in den DN1a von Canton S Wildtypfliegen im Vergleich zu Fliegen ohne Lichtpuls-Behandlung. Aufzeichnungen der Lokomotoraktivit{\"a}t offenbaren zus{\"a}tzlich die Notwendigkeit von p38 MAPK f{\"u}r wildtypisches Timing der Abendaktivit{\"a}t sowie zum Erhalt von 24-Stunden-Verhaltensrhythmen unter konstanten Dauerdunkel-Bedindungen. So zeigen Fliegen mit reduzierten p38 Level in Uhrneuronen einen verz{\"o}gerten Beginn der Abendaktivit{\"a}t und stark verl{\"a}ngerte Freilaufperioden. In {\"U}bereinstimmung mit Effekten auf das Laufverhalten scheint dar{\"u}ber hinaus die Expression einer dominant-negativen Form von p38b in Drosophila's wichtigsten Uhrneuronen eine versp{\"a}tete nukle{\"a}re Translokation von Period zur Folge zu haben. Westernblots legen zus{\"a}tzlich einen Einfluss von p38 auf den Phosphorylierungsgrad von Period nahe und liefern damit einen m{\"o}gliche Erkl{\"a}rung f{\"u}r den versp{\"a}teten Kerneintritt des Uhrproteins. Abschließende St{\"u}tzung der Westernblotergebnisse bringen in vitro Kinasenassays und deuten auf p38 als eine potentielle „Uhrkinase" hin, welche auch in vivo Period an Serin 661 sowie weiteren potentiellen Phosphorylierungsstellen phosphorylieren k{\"o}nnte. Zusammengenommen deuten die Ergebnisse der hier vorliegenden Arbeit eindeutig auf eine bedeutende Rolle von p38, neben dessen Funkion im Stress-System, auch im circadianen System der Fliege hin und offenbaren damit die M{\"o}glichkeit, dass p38 als Schnittstelle zwischen beider Systeme fungiert.}, subject = {Taufliege}, language = {de} } @phdthesis{Mueller2015, author = {M{\"u}ller, Elisabeth}, title = {Pan-Raf-Inhibition als neue therapeutische Strategie im Multiplen Myelom}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-124666}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Das Multiple Myelom (MM) ist eine durch monoklonale Vermehrung terminal differenzierter Antik{\"o}rper-produzierender B-Lymphozyten (Plasmazellen) im Knochenmark charakterisierte maligne Krankheit, die sich v.a. in osteolytischen Knochendestruktionen, h{\"a}matopoetischer und Niereninsuffizienz {\"a}ußert. Verbesserte Therapieans{\"a}tze wie die Hochdosis-Chemotherapie mit Melphalan und anschließender autologer Stammzelltransplantation sowie die Einf{\"u}hrung neuer pharmakologischer Substanzklassen (Proteasom-Inhibitoren, Cereblon-bindende Thalidomidderivate) f{\"u}hrten zu einer Verl{\"a}ngerung der durchschnittlichen {\"U}berlebenszeit, f{\"u}r die meisten der Patienten ist die Erkrankung jedoch derzeit unheilbar. Die Erforschung neuer potenzieller therapeutischer Angriffspunkte auf Grund pathobiologischer Erkenntnisse bleibt daher unabdingbar. Ein Ansatz zur Verbesserung des Verst{\"a}ndnisses der Pathogenese ist die funktionelle, molekulare und genetische Analyse des Signalnetzwerkes im MM. Im Zusammenhang mit diesem Konzept wurde entdeckt, dass wachstums-regulierende Signalwege in MM Zellen aktiviert oder dereguliert sind und zum {\"U}berleben und der Proliferation des Tumors beitragen. So konnte beispielsweise von unserer Arbeitsgruppe bereits gezeigt werden, dass onkogenes Ras essentiell zum {\"U}berleben der MM Zellen beitr{\"a}gt. Da Ras derzeit mangels spezifischer Inhibitoren pharmakologisch nicht angreifbar ist, stellen weitere funktionelle Bestandteile des Signalweges eine potenzielle therapeutische Zielstruktur dar. W{\"a}hrend die Blockade von MEK1/2 in MM Zellen keinen Einfluss auf das {\"U}berleben hatte, konnte durch die Blockade von Raf in ersten Tests unserer Arbeitsgruppe Apoptose hervorgerufen werden. Aus diesem Grund habe ich in der vorliegenden Arbeit zur Evaluation eines neuen Therapieansatzes die Rolle der Raf-abh{\"a}ngigen Signaltransduktion eingehend untersucht. Als Grundlage diente dabei die Hypothese, dass die Raf-Kinasen entscheidende Effektoren der durch onkogenes Ras vermittelten apoptotischen Effekte darstellen. In einem ersten Schritt konnte ich nachweisen, dass alle drei Raf-Isoformen (A-, B- und C-Raf) in humanen MM Zelllinien und in prim{\"a}ren MM Zellen aktiviert sind. Mittels shRNA-vermittelter, Isoform-spezifischer Raf-Knockdown-Experimente konnte ich zeigen, dass nur ein simultaner Knockdown aller Isoformen, d.h. ein Pan-Raf-Knockdown, zu einer De-Phosphorylierung von MEK1/2 und ERK1/2 f{\"u}hrte. Dieser Versuch ließ sich mittels pharmakologischer Raf-Inhibition, bei der ebenfalls nur eine Pan-Raf-Blockade zu einer Herunterregulation von MEK1/2 und ERK1/2 in MM Zellen f{\"u}hrte, best{\"a}tigen. Das MEK/ERK-Modul stellte somit einen hervorragenden Surrogat- und Biomarker f{\"u}r die Pan-Raf-Aktivit{\"a}t dar. Im Gegensatz zur Blockade des MEK/ERK-Moduls f{\"u}hrte eine Hemmung der Pan-Raf-Aktivit{\"a}t mittels shRNA oder pharmakologischer Inhibitoren in allen untersuchten Zelllinien und in der Mehrheit der prim{\"a}ren MM Zellen zu einer starken Induktion von Apoptose. Da das Ansprechen auf eine Pan-Raf-Blockade nicht mit dem Ras-Mutationsstatus korrelierte, k{\"o}nnten die Raf-Kinasen eine von onkogenem Ras unabh{\"a}ngie Qualit{\"a}t als therapeutische Zielstruktur aufweisen. Zur Untersuchung m{\"o}glicher MEK/ERK-unabh{\"a}ngiger Effektormechanismen der Pan-Raf-Inhibition habe ich die mRNA-basierten Genexpressionsprofile von INA-6 Zellen nach pharmakologischer Pan-Raf- oder MEK-Inhibition verglichen. Dabei f{\"u}hrte die Pan-Raf-Inhibition zu einer Regulation von wesentlich mehr Genen, wobei sich auch die Art der regulierten Gene unterschied, darunter Gene mit tumorrelevanten Funktionen wie Regulation von Proliferation, Zellzyklus und Apoptose. F{\"u}r eine dieser Gengruppen, die Gruppe der PI3K-abh{\"a}ngigen, mTOR-assoziierten Gene, konnte ich eine Regulation auch auf der Proteinebene nachweisen: die Phosphorylierungen von mTOR, p70S6K, Rb und AKT und die Expression von CyclinD1 und PDK1 waren nach Pan-Raf-Inhibition, nicht jedoch nach MEK-Blockade herunterreguliert. Dieses Ergebnis deutet auf eine Ko-Regulation der PI3K-abh{\"a}ngigen Signaltransduktion durch die Raf-kinasen hin. Mittels spezifischer PI3K-Inhibitoren ließ sich sowohl bei der Regulation der untersuchten Proteine als auch bei der Induktion von Apoptose eine deutliche Verst{\"a}rkung der Pan-Raf-Inhibition in HMZL und in prim{\"a}ren Zellen erzielen. Zusammengefasst zeigt diese Arbeit, dass die Pan-Raf-Blockade eine neue Therapiem{\"o}glichkeit darstellt, die durch Kombination mit einer PI3K/AKT-Inhibition noch verst{\"a}rkt werden kann.}, subject = {Plasmozytom}, language = {de} } @article{PaschLinkBecketal.2015, author = {Pasch, Elisabeth and Link, Jana and Beck, Carolin and Scheuerle, Stefanie and Alsheimer, Manfred}, title = {The LINC complex component Sun4 plays a crucial role in sperm head formation and fertility}, series = {Biology Open}, volume = {4}, journal = {Biology Open}, doi = {10.1242/bio.015768}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-125212}, pages = {1792-1802}, year = {2015}, abstract = {LINC complexes are evolutionarily conserved nuclear envelope bridges, physically connecting the nucleus to the peripheral cytoskeleton. They are pivotal for dynamic cellular and developmental processes, like nuclear migration, anchoring and positioning, meiotic chromosome movements and maintenance of cell polarity and nuclear shape. Active nuclear reshaping is a hallmark of mammalian sperm development and, by transducing cytoskeletal forces to the nuclear envelope, LINC complexes could be vital for sperm head formation as well. We here analyzed in detail the behavior and function of Sun4, a bona fide testis-specific LINC component. We demonstrate that Sun4 is solely expressed in spermatids and there localizes to the posterior nuclear envelope, likely interacting with Sun3/Nesprin1 LINC components. Our study revealed that Sun4 deficiency severely impacts the nucleocytoplasmic junction, leads to mislocalization of other LINC components and interferes with the formation of the microtubule manchette, which finally culminates in a globozoospermia-like phenotype. Together, our study provides direct evidence for a critical role of LINC complexes in mammalian sperm head formation and male fertility.}, language = {en} } @phdthesis{Grimmig2015, author = {Grimmig, Tanja Maria}, title = {Immunity, Inflammation and Cancer: The role of Foxp3, TLR7 and TLR8 in gastrointestinal cancer}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-125248}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Regulatory T cells (Treg) expressing the transcription factor forkhead box protein P3 (Foxp3) have been demonstrated to mediate evasion from anti-tumor immune responses during tumor progression. Moreover, Foxp3 expression by tumor cells themselves may allow them to counteract effector T cell responses, resulting in a survival benefit of the tumor. For gastrointestinal cancers, in particular pancreatic and colorectal cancer (CRC), the clinical relevance of Foxp3 is not clear to date. Therefore the aim of this study was to analyze its impact in CRC and pancreatic cancer. To determine the relevance of Foxp3 for tumor progression and patient survival, gene and protein analysis of human pancreatic and colon cancer cell lines as well as tumor tissues from patients with CRC was performed. The results derived from the patients with CRC were correlated with clinicopathological parameters and patients' overall survival. Cancer cell mediated Foxp3 expression in vitro was demonstrated in human pancreatic cancer cell lines PANC1, PaCa DD 135, PaCa DD 159 and PaCa DD 185 as well as in human colon cancer cell lines SW480 and SW620. Additionally, Foxp3 expressing cancer cells were found in ex vivo tumor tissue samples of patients with CRC. The percentage of Foxp3+ cancer cells increased from stages UICC I/II to UICC III/IV compared to normal tissue. Moreover, high tumor cell mediated Foxp3 expression was associated with poor prognosis compared to patients with low Foxp3 expression. In contrast, low and high Foxp3 level in tumor infiltrating Treg cells demonstrated no significant differences in patients' overall survival. Correlation analysis demonstrated a significant association of Foxp3 cancer cell expression with the expression of immunosuppressive cytokines IL-10 and TGF-β. These findings suggest that Immunosuppressive cytokines such as IL-10 and TGF-β released by rather Foxp3+ cancer cells than Foxp3+ Treg cells may inhibit the activation of naive T cells, hence limiting antitumor immune responses and favoring tumorigenesis and progression. Chronic inflammation has been shown to be an important epigenetic and environmental factor in numerous tumor entities. Recent data suggest that tumorigenesis and tumor progression may be associated with inflammation-triggered activation of Toll-like receptors (TLR). In this study, the specific impact of both TLR7 and TLR8 expression and signaling on tumor cell proliferation and chemoresistance is analyzed in inflammation linked CRC and pancreatic cancer. By gene and protein expression analysis of human pancreatic and colon cancer cell lines TLR7 and TLR8 expression was determined in vitro. Additionally, expression of TLR7/TLR8 in UICC stage I-IV pancreatic cancer, chronic pancreatitis and normal pancreatic tissue was examined. For in vitro/in vivo studies TLR7/TLR8 overexpressing PANC1 cell lines were generated and analyzed for effects of TLR expression and stimulation on tumor cell proliferation and chemoresistance. Cancer cell mediated TLR7 and TLR8 expression in vitro was demonstrated in human colon cancer cell lines SW480, SW620 and HT-29 as well as in primary pancreatic cancer cell lines PaCa DD 135, PaCa DD 159 and PaCa DD 185. Additionally, TLR7 and TLR8 expressing tumor cells were found in ex vivo tissue samples of patients with pancreatic cancer and chronic pancreatitis. Significantly elevated expression levels of TLR7 and TLR8 were found in advanced tumor stages (UICC III) compared to early tumor stages (UICC II) and chronic pancreatitis. No or occasionally low expression was detected in normal pancreatic tissue. In contrast to the tissues from patients with pancreatic cancer or chronic pancreatitis, established pancreatic tumor cell lines express only very low levels of TLR7 and TLR8. Therefore, for in vitro and xenograft studies TLR7 or TLR8 overexpressing PANC1 cells were generated. Proliferation promoting effects of TLR7 and TLR8 expression and stimulation with R848 were detected in vitro. Additionally, increased tumor growth of TLR expressing PANC1 cells was demonstrated in subcutaneously injected Balb/c nude mice. Interestingly, activation of TLR7 or TLR8 induced not only an increase in tumor cell proliferation but also a strong chemoresistance of PANC1 cells against 5-fluorouracil (5-FU). Moreover, treatment with R848 resulted in elevated expression levels of NF-κB, COX-2 and inflammatory cytokines IL-1β, IL-8 and TNF-α, suggesting TLR7/8 signaling to contribute to an inflammatory, anti-apoptotic and proliferation promoting tumor microenvironment. These findings emphasize the particular role of TLR7 and TLR8 in inflammation related cancers and their relevance as potential targets for cancer therapy.  }, subject = {Bauchspeicheldr{\"u}senkrebs}, language = {en} } @article{Meierjohann2015, author = {Meierjohann, Svenja}, title = {Hypoxia independent drivers of melanoma angiogenesis}, series = {Frontiers in Oncology}, volume = {5}, journal = {Frontiers in Oncology}, number = {120}, doi = {10.3389/fonc.2015.00102}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-125586}, year = {2015}, abstract = {Tumor angiogenesis is a process which is traditionally regarded as the tumor's response to low nutrient supply occurring under hypoxic conditions. However, hypoxia is not a pre-requisite for angiogenesis. The fact that even single tumor cells or small tumor cell aggregates are capable of attracting blood vessels reveals the early metastatic capability of tumor cells. This review sheds light on the hypoxia-independent mechanisms of tumor angiogenesis in melanoma.}, language = {en} } @article{HerterStauchGallantetal.2015, author = {Herter, Eva K. and Stauch, Maria and Gallant, Maria and Wolf, Elmar and Raabe, Thomas and Gallant, Peter}, title = {snoRNAs are a novel class of biologically relevant Myc targets}, series = {BMC Biology}, volume = {13}, journal = {BMC Biology}, number = {25}, doi = {10.1186/s12915-015-0132-6}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-124956}, year = {2015}, abstract = {Background Myc proteins are essential regulators of animal growth during normal development, and their deregulation is one of the main driving factors of human malignancies. They function as transcription factors that (in vertebrates) control many growth- and proliferation-associated genes, and in some contexts contribute to global gene regulation. Results We combine chromatin immunoprecipitation-sequencing (ChIPseq) and RNAseq approaches in Drosophila tissue culture cells to identify a core set of less than 500 Myc target genes, whose salient function resides in the control of ribosome biogenesis. Among these genes we find the non-coding snoRNA genes as a large novel class of Myc targets. All assayed snoRNAs are affected by Myc, and many of them are subject to direct transcriptional activation by Myc, both in Drosophila and in vertebrates. The loss of snoRNAs impairs growth during normal development, whereas their overexpression increases tumor mass in a model for neuronal tumors. Conclusions This work shows that Myc acts as a master regulator of snoRNP biogenesis. In addition, in combination with recent observations of snoRNA involvement in human cancer, it raises the possibility that Myc's transforming effects are partially mediated by this class of non-coding transcripts.}, language = {en} } @article{SickelAnkenbrandGrimmeretal.2015, author = {Sickel, Wiebke and Ankenbrand, Markus J. and Grimmer, Gudrun and Holzschuh, Andrea and H{\"a}rtel, Stephan and Lanzen, Jonathan and Steffan-Dewenter, Ingolf and Keller, Alexander}, title = {Increased efficiency in identifying mixed pollen samples by meta-barcoding with a dual-indexing approach}, series = {BMC Ecology}, volume = {15}, journal = {BMC Ecology}, number = {20}, doi = {10.1186/s12898-015-0051-y}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-125730}, year = {2015}, abstract = {Background Meta-barcoding of mixed pollen samples constitutes a suitable alternative to conventional pollen identification via light microscopy. Current approaches however have limitations in practicability due to low sample throughput and/or inefficient processing methods, e.g. separate steps for amplification and sample indexing. Results We thus developed a new primer-adapter design for high throughput sequencing with the Illumina technology that remedies these issues. It uses a dual-indexing strategy, where sample-specific combinations of forward and reverse identifiers attached to the barcode marker allow high sample throughput with a single sequencing run. It does not require further adapter ligation steps after amplification. We applied this protocol to 384 pollen samples collected by solitary bees and sequenced all samples together on a single Illumina MiSeq v2 flow cell. According to rarefaction curves, 2,000-3,000 high quality reads per sample were sufficient to assess the complete diversity of 95\% of the samples. We were able to detect 650 different plant taxa in total, of which 95\% were classified at the species level. Together with the laboratory protocol, we also present an update of the reference database used by the classifier software, which increases the total number of covered global plant species included in the database from 37,403 to 72,325 (93\% increase). Conclusions This study thus offers improvements for the laboratory and bioinformatical workflow to existing approaches regarding data quantity and quality as well as processing effort and cost-effectiveness. Although only tested for pollen samples, it is furthermore applicable to other research questions requiring plant identification in mixed and challenging samples.}, language = {en} } @article{SalatWinklerUrlaubetal.2015, author = {Salat, Daniela and Winkler, Anja and Urlaub, Henning and Gessler, Manfred}, title = {Hey bHLH Proteins Interact with a FBXO45 Containing SCF Ubiquitin Ligase Complex and Induce Its Translocation into the Nucleus}, series = {PLoS One}, volume = {10}, journal = {PLoS One}, number = {6}, doi = {10.1371/journal.pone.0130288}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-125769}, pages = {e0130288}, year = {2015}, abstract = {The Hey protein family, comprising Hey1, Hey2 and HeyL in mammals, conveys Notch signals in many cell types. The helix-loop-helix (HLH) domain as well as the Orange domain, mediate homo- and heterodimerization of these transcription factors. Although distinct interaction partners have been identified so far, their physiological relevance for Hey functions is still largely unclear. Using a tandem affinity purification approach and mass spectrometry analysis we identified members of an ubiquitin E3-ligase complex consisting of FBXO45, PAM and SKP1 as novel Hey1 associated proteins. There is a direct interaction between Hey1 and FBXO45, whereas FBXO45 is needed to mediate indirect Hey1 binding to SKP1. Expression of Hey1 induces translocation of FBXO45 and PAM into the nucleus. Hey1 is a short-lived protein that is degraded by the proteasome, but there is no evidence for FBXO45-dependent ubiquitination of Hey1. On the contrary, Hey1 mediated nuclear translocation of FBXO45 and its associated ubiquitin ligase complex may extend its spectrum to additional nuclear targets triggering their ubiquitination. This suggests a novel mechanism of action for Hey bHLH factors.}, language = {en} } @article{FalibeneRocesRoessler2015, author = {Falibene, Agustina and Roces, Flavio and R{\"o}ssler, Wolfgang}, title = {Long-term avoidance memory formation is associated with a transient increase in mushroom body synaptic complexes in leaf-cutting ants}, series = {Frontiers in Behavioral Neuroscience}, volume = {9}, journal = {Frontiers in Behavioral Neuroscience}, number = {84}, doi = {10.3389/fnbeh.2015.00084}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-125522}, year = {2015}, abstract = {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.}, language = {en} }