@article{SinghKingstonGuptaetal.2015, author = {Singh, Amit K. and Kingston, Joseph J. and Gupta, Shishir K. and Batra, Harsh V.}, title = {Recombinant Bivalent Fusion Protein rVE Induces CD4+ and CD8+ T-Cell Mediated Memory Immune Response for Protection Against Yersinia enterocolitica Infection}, series = {Frontiers in Microbiology}, volume = {6}, journal = {Frontiers in Microbiology}, number = {1407}, doi = {10.3389/fmicb.2015.01407}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-136114}, year = {2015}, abstract = {Studies investigating the correlates of immune protection against Yersinia infection have established that both humoral and cell mediated immune responses are required for the comprehensive protection. In our previous study, we established that the bivalent fusion protein (rVE) comprising immunologically active regions of Y pestis LcrV (100-270 aa) and YopE (50-213 aa) proteins conferred complete passive and active protection against lethal Y enterocolitica 8081 challenge. In the present study, cohort of BALB/c mice immunized with rVE or its component proteins rV, rE were assessed for cell mediated immune responses and memory immune protection against Y enterocolitica 8081 rVE immunization resulted in extensive proliferation of both CD4 and CD8 T cell subsets; significantly high antibody titer with balanced IgG1: IgG2a/IgG2b isotypes (1:1 ratio) and up regulation of both Th1 (INF-\(\alpha\), IFN-\(\gamma\), IL 2, and IL 12) and Th2 (IL 4) cytokines. On the other hand, rV immunization resulted in Th2 biased IgG response (11:1 ratio) and proliferation of CD4+ T-cell; rE group of mice exhibited considerably lower serum antibody titer with predominant Th1 response (1:3 ratio) and CD8+ T-cell proliferation. Comprehensive protection with superior survival (100\%) was observed among rVE immunized mice when compared to the significantly lower survival rates among rE (37.5\%) and rV (25\%) groups when IP challenged with Y enterocolitica 8081 after 120 days of immunization. Findings in this and our earlier studies define the bivalent fusion protein rVE as a potent candidate vaccine molecule with the capability to concurrently stimulate humoral and cell mediated immune responses and a proof of concept for developing efficient subunit vaccines against Gram negative facultative intracellular bacterial pathogens.}, language = {en} } @phdthesis{Schneider2015, author = {Schneider, Gudrun}, title = {Effects of adjacent habitats and landscape composition on biodiversity in semi-natural grasslands and biological pest control in oilseed rape fields}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-113549}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {1) Modern European agricultural landscapes form a patchy mosaic of highly fragmented natural and semi-natural habitat remnants embedded in a matrix of intensively managed agricultural land. In those landscapes many organism frequently cross habitat borders including the crop - non-crop boundary, hereby connecting the biotic interactions of multiple habitat types. Therefore biodiversity and ecosystem functions within habitats are expected to depend on adjacent habitat types and the surrounding landscape matrix. In this thesis the biodiversity of non-crop habitats, and ecosystem services and disservices in crop habitats were studied in the human-dominated agricultural landscape in the district Lower Franconia, Bavaria, Germany. First we examined the effect of adjacent habitat type on species composition, diversity and ecosystem functions in semi-natural calcareous grasslands, a biodiversity-rich habitat of high conservation value (chapter 2 and 3). Second we studied the effect of habitat composition in the landscape on herbivory, biological pest control and yield in oilseed rape fields (chapter 4). 2) We examined the effect of adjacent habitat type on the diversity of carabid beetles in 20 calcareous grasslands using pitfall traps. Half of the grasslands were adjacent to a coniferous forest and half to a cereal crop field. We found different species compositions of carabid beetles depending on adjacent habitat type. In addition calcareous grasslands adjacent to crop fields harboured a higher species richness and activity density but a lower evenness of carabid beetles than calcareous grasslands adjacent to forests. These differences can be explained by the spillover of carabid beetles from the adjacent habitats. After crop harvest carabid beetle activity density in crop fields decreased while in parallel the activity density in the calcareous grasslands adjacent to the crop fields increased, indicating an unidirectional carabid beetle spillover. Our results underline that type and management of adjacent habitats affect community composition and diversity in calcareous grasslands. Therefore nature conservation measures, which focused on the improvement of local habitat quality so far, additionally need to consider adjacent habitat type. 3) In addition to carabid beetle communities we also surveyed predation rates of ground-dwelling predators on the same calcareous grasslands in two study periods (June and late August). As ground-dwelling predators of forests or crop fields can move into adjacent calcareous grasslands we expected different predation rates depending on adjacent habitat type. We exposed in total 32.000 lady bird eggs as prey items on the calcareous grasslands in distances of 5 and 20m from the habitat border. We found higher predation rates on calcareous grasslands adjacent to forests than on calcareous grasslands adjacent to crop fields, but only on cool days. On warm days a very high extent (often 100\%) of the exposed prey items were consumed adjacent to both habitat types, which did not allow the detection of possible differences between the adjacent habitat types. Predation rates differed not between the two study periods or the two distances to the habitat edge. The higher predation rates adjacent to forests can be explained by the spillover of ground-dwelling predators from forests into calcareous grasslands. Our results show, that spillover into semi-natural habitats affects ecosystem functioning in addition to species composition and diversity. 4) In chapter 4 of this thesis we examined the effect of spatiotemporal changes in crop cover on pest - natural enemy interactions and crop yields. During two study years we surveyed the abundance of adult and larval pollen beetles, parasitism of pollen beetle larvae by a hymenopteran parasitoid and oilseed rape yields of 36 oilseed rape fields. The surrounding landscape of the fields (1 km radius) differed in the oilseed rape proportion and in the inter-annual change in the oilseed rape proportion since the previous year. We found a dilution effect, i.e. a decreasing abundance with increasing oilseed rape proportions, for pollen beetle larvae and parasitoids in both study years and for adult pollen beetles in one study year. Oilseed rape yields increased with increasing oilseed rape proportions. Inter-annual changes in oilseed rape proportions led to inter-annual crowding and dilution effects for pollen beetles, but had no effect on parasitism or yield. Our results indicate the potential to reduce pest loads and increase yields in intensively managed oilseed rape fields by a coordinated management of the spatiotemporal oilseed rape cover in the landscape. 5) In summary, we showed in this thesis that the biodiversity and functioning of crop and non-crop habitats within agricultural landscapes is affected by the spillover of organisms and thus by the habitat composition in the close surrounding and in the broader landscape context. Spillover affects also ecosystem services and disservices and therefore crop productivity. Thereby the spatial and temporal variation of specific crop types in the landscape can be of particular importance for crop yields. Thus a coordinated landscape wide management can help to optimize both biodiversity conservation and the delivery of ecosystem services and thus crop yields. Future studies integrating landscape effects across several ecosystem functions, multiple taxonomic groups and different crop types are necessary to develop definite landscape management schemes.}, subject = {Landschafts{\"o}kologie}, language = {en} } @article{KuhnGrippFliederetal.2015, author = {Kuhn, Joachim and Gripp, Tatjana and Flieder, Tobias and Dittrich, Marcus and Hendig, Doris and Busse, Jessica and Knabbe, Cornelius and Birschmann, Ingvild}, title = {UPLC-MRM Mass Spectrometry Method for Measurement of the Coagulation Inhibitors Dabigatran and Rivaroxaban in Human Plasma and Its Comparison with Functional Assays}, series = {PLOS ONE}, volume = {10}, journal = {PLOS ONE}, number = {12}, doi = {10.1371/journal.pone.0145478}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-136023}, pages = {e0145478}, year = {2015}, abstract = {Introduction The fast, precise, and accurate measurement of the new generation of oral anticoagulants such as dabigatran and rivaroxaban in patients' plasma my provide important information in different clinical circumstances such as in the case of suspicion of overdose, when patients switch from existing oral anticoagulant, in patients with hepatic or renal impairment, by concomitant use of interaction drugs, or to assess anticoagulant concentration in patients' blood before major surgery. Methods Here, we describe a quick and precise method to measure the coagulation inhibitors dabigatran and rivaroxaban using ultra-performance liquid chromatography electrospray ionization-tandem mass spectrometry in multiple reactions monitoring (MRM) mode (UPLC-MRM MS). Internal standards (ISs) were added to the sample and after protein precipitation; the sample was separated on a reverse phase column. After ionization of the analytes the ions were detected using electrospray ionization-tandem mass spectrometry. Run time was 2.5 minutes per injection. Ion suppression was characterized by means of post-column infusion. Results The calibration curves of dabigatran and rivaroxaban were linear over the working range between 0.8 and 800 mu g/L (r > 0.99). Limits of detection (LOD) in the plasma matrix were 0.21 mu g/L for dabigatran and 0.34 mu g/L for rivaroxaban, and lower limits of quantification (LLOQ) in the plasma matrix were 0.46 mu g/L for dabigatran and 0.54 mu g/L for rivaroxaban. The intraassay coefficients of variation (CVs) for dabigatran and rivaroxaban were < 4\% and 6\%; respectively, the interassay CVs were < 6\% for dabigatran and < 9\% for rivaroxaban. Inaccuracy was < 5\% for both substances. The mean recovery was 104.5\% (range 83.8-113.0\%) for dabigatran and 87.0\%(range 73.6-105.4\%) for rivaroxaban. No significant ion suppressions were detected at the elution times of dabigatran or rivaroxaban. Both coagulation inhibitors were stable in citrate plasma at -20 degrees C, 4 degrees C and even at RT for at least one week. A method comparison between our UPLC-MRM MS method, the commercially available automated Direct Thrombin Inhibitor assay (DTI assay) for dabigatran measurement from CoaChrom Diagnostica, as well as the automated anti-Xa assay for rivaroxaban measurement from Chromogenix both performed by ACL-TOP showed a high degree of correlation. However, UPLC-MRM MS measurement of dabigatran and rivaroxaban has a much better selectivity than classical functional assays measuring activities of various coagulation factors which are susceptible to interference by other coagulant drugs. Conclusions Overall, we developed and validated a sensitive and specific UPLC-MRM MS assay for the quick and specific measurement of dabigatran and rivaroxaban in human plasma.}, language = {en} } @phdthesis{Brockmann2015, author = {Brockmann, Markus}, title = {Inhibition von Aurora-A als neue Therapiestrategie gegen MYCN-amplifizierte Neuroblastome}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-135951}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Im Neuroblastom ist die Amplifikation des MYCN-Gens, das f{\"u}r den Transkriptionsfaktor N-Myc kodiert, der klinisch bedeutendste Faktor f{\"u}r eine schlechte Prognose. Als Mitglied der onkogenen Myc-Familie induziert N-Myc die Expression von Genen, die in vielen biologischen Prozessen wie Metabolismus, Zellzyklusprogression, Zellwachstum und Apoptose eine wichtige Rolle spielen. Die Deregulation der MYCN-Expression f{\"u}hrt zu einem charakteristischen Genexpressionsprofil und einem aggressiven Phenotyp in den Tumorzellen. In normalen neuronalen Vorl{\"a}uferzellen wird N-Myc gew{\"o}hnlich sehr schnell proteasomal abgebaut. W{\"a}hrend der Mitose wird N-Myc an Serin 62 phosphoryliert. Diese Phosphorylierung dient als Erkennungssignal f{\"u}r die Kinase GSK3β, die die Phosphorylierung an Threonin 58 katalysiert. Das Phosphodegron wird von Fbxw7, einer Komponente des E3-Ubiquitinligase-Komplex SCFFbxw7, erkannt. Die anschließende Ubiquitinierung induziert den proteasomalen Abbau des Proteins. Die Reduktion der N-Myc-Proteinlevel erm{\"o}glicht den neuronalen Vorl{\"a}uferzellen den Austritt aus dem Zellzyklus und f{\"u}hrt zu einer terminalen Differenzierung. In einem shRNA Screen konnte AURKA als essentielles Gen f{\"u}r die Proliferation MYCN-amplifizierter Neuroblastomzellen identifiziert werden. Eine Aurora-A-Depletion hatte jedoch keinen Einfluss auf das Wachstum nicht-amplifizierter Zellen. W{\"a}hrend dieser Doktorarbeit konnte gezeigt werden, dass Aurora-A speziell den Fbxw7-vermittelten Abbau verhindert und dadurch N-Myc stabilisiert. F{\"u}r die Stabilisierung ist zwar die Interaktion der beiden Proteine von entscheidender Bedeutung, {\"u}berraschenderweise spielt die Kinaseaktivit{\"a}t von Aurora-A jedoch keine Rolle. Zwei spezifische Aurora-A-Inhibitoren, MLN8054 und MLN8237, sind allerdings in der Lage, nicht nur die Kinaseaktivit{\"a}t zu hemmen, sondern auch die N-Myc-Proteinlevel zu reduzieren. Beide Molek{\"u}le induzieren eine Konformations{\"a}nderung in der Kinasedom{\"a}ne von Aurora-A. Diese ungew{\"o}hnliche strukturelle Ver{\"a}nderung hat zur Folge, dass der N-Myc/Aurora-A-Komplex dissoziiert und N-Myc mit Hilfe von Fbxw7 proteasomal abgebaut werden kann. In MYCN-amplifizierten Zellen f{\"u}hrt diese Reduktion an N-Myc zu einem Zellzyklusarrest in der G1-Phase. Die in vitro Daten konnten in einem transgenen Maus-Modell f{\"u}r das MYCN-amplifizierte Neuroblastom best{\"a}tigt werden. Die Behandlung mit MLN8054 und MLN8237 f{\"u}hrte in den Tumoren ebenfalls zu einer N-Myc-Reduktion. Dar{\"u}ber hinaus konnte ein prozentualer Anstieg an differenzierten Zellen, die vollst{\"a}ndige Tumorregression in der Mehrzahl der Neuroblastome und eine gesteigerte Lebenserwartung beobachtet werden. Insgesamt zeigen die in vitro und in vivo Daten, dass die spezifischen Aurora-A-Inhibitoren ein hohes therapeutisches Potential gegen das MYCN-amplifizierte Neuroblastom besitzen.}, subject = {N-Myc}, language = {de} } @phdthesis{Scholl2015, author = {Scholl, Christina}, title = {Cellular and molecular mechanisms contributing to behavioral transitions and learning in the honeybee}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-115527}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {The honeybee Apis mellifera is a social insect well known for its complex behavior and the ability to learn tasks associated with central place foraging, such as visual navigation or to learn and remember odor-reward associations. Although its brain is smaller than 1mm² with only 8.2 x 105 neurons compared to ~ 20 x 109 in humans, bees still show amazing social, cognitive and learning skills. They express an age - related division of labor with nurse bees staying inside the hive and performing tasks like caring for the brood or cleaning, and foragers who collect food and water outside the hive. This challenges foragers with new responsibilities like sophisticated navigation skills to find and remember food sources, drastic changes in the sensory environment and to communicate new information to other bees. Associated with this plasticity of the behavior, the brain and especially the mushroom bodies (MBs) - sensory integration and association centers involved in learning and memory formation - undergo massive structural and functional neuronal alterations. Related to this background my thesis on one hand focuses on neuronal plasticity and underlying molecular mechanisms in the MBs that accompany the nurse - forager transition. In the first part I investigated an endogenous and an internal factor that may contribute to the nurse - forager phenotype plasticity and the correlating changes in neuronal network in the MBs: sensory exposure (light) and juvenile hormone (JH). Young bees were precociously exposed to light and subsequently synaptic complexes (microglomeruli, MG) in the MBs or respectively hemolymph juvenile hormone (JH) levels were quantified. The results show that light input indeed triggered a significant decrease in MG density, and mass spectrometry JH detection revealed an increase in JH titer. Interestingly light stimulation in young bees (presumably nurse bees) triggered changes in MG density and JH levels comparable to natural foragers. This indicates that both sensory stimuli as well as the endocrine system may play a part in preparing bees for the behavioral transition to foraging. Considering a connection between the JH levels and synaptic remodeling I used gene knockdown to disturb JH pathways and artificially increase the JH level. Even though the knockdown was successful, the results show that MG densities remained unchanged, showing no direct effect of JH on synaptic restructuring. To find a potential mediator of structural synaptic plasticity I focused on the calcium-calmodulin-dependent protein kinase II (CaMKII) in the second part of my thesis. CaMKII is a protein known to be involved in neuronal and behavioral plasticity and also plays an important part in structural plasticity reorganizing synapses. Therefore it is an interesting candidate for molecular mechanisms underlying MG reorganization in the MBs in the honeybee. Corresponding to the high abundance of CaMKII in the learning center in vertebrates (hippocampus), CaMKII was shown to be enriched in the MBs of the honeybee. Here I first investigated the function of CaMKII in learning and memory formation as from vertebrate work CaMKII is known to be associated with the strengthening of synaptic connections inducing long term potentiation and memory formation. The experimental approach included manipulating CaMKII function using 2 different inhibitors and a specific siRNA to create a CaMKII knockdown phenotype. Afterwards bees were subjected to classical olfactory conditioning which is known to induce stable long-term memory. All bees showed normal learning curves and an intact memory acquisition, short-term and mid-term memory (1 hour retention). However, in all cases long-term memory formation was significantly disrupted (24 and 72 hour retention). These results suggests the necessity of functional CaMKII in the MBs for the induction of both early and late phases of long-term memory in honeybees. The neuronal and molecular bases underlying long-term memory and the resulting plasticity in behavior is key to understanding higher brain function and phenotype plasticity. In this context CaMKII may be an important mediator inducing structural synaptic and neuronal changes in the MB synaptic network.}, subject = {Biene}, language = {en} } @phdthesis{Konrad2015, author = {Konrad, Tillmann}, title = {Governance of Protected Areas in West Africa - The case of the W-Arly-Pendjari (WAP) Complex in Benin and Burkina Faso}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-115331}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Protected areas are the central strategy for preserving biodiversity in the face of overexploitation and global change. To ensure their long-term survival, however, these areas may not be regarded as last havens of wilderness, but as complex social-ecological systems. Modern approaches of protected area (PA) management support this view by balancing conservation and development issues in a sustainable way and adapted to the local context. However, success of these strategies in achieving their aims so far remains limited. This study therefore aimed at analysing processes and outcomes of PA co-management approaches implemented in a large transfrontier conservation area in West Africa. The W-Arly-Pendjari (WAP) complex spans over more than 30.000 square km in Benin, Burkina Faso and Niger and is composed of approximately 20 subunits. Due to national legal and administrative variety as well as a high diversity of local (project) implementation approaches, the general setting resembled a quasi-experimental design facilitating comparative studies. A mix of quantitative (e.g. survey of 549 households) and qualitative (e.g. expert interviews, literature review) methods was used to evaluate the institutional and organisational differences of PA management approaches implemented in the different parts of WAP belonging to Benin and Burkina Faso. I included an analysis of contextual factors (e.g. land-cover-change) and ecological data, but concentrated on the role of local resource users within the co-management arrangements and the effectiveness of governance regimes to deliver positive socio-economic outputs. Exploring the question whether promotion of development in PA surroundings indeed stipulates conservation success (and vice versa) remained challenging: the lack of sound ecological data, a general mismatch of spatial scale in existing data sets, as well as the high complexity of realities on the ground made me refrain from using simplified proxy indicators and (statistical) modelling approaches. I found that the Sudano-Sahelian context is a very difficult one for the implementation of effective participation approaches in the short-term. Political, demographic, socio-economic as well as ecological factors generated a very dynamic situation characterized by limited financial and natural resources as well as weak institutional and organisational settings. Arenas of interaction were often marked rather by a high degree of distrust and competition than by cooperation among actors. Amid all rhetoric, participation in most cases was hence limited to the transfer of (sparse) information, regulated resource access and financial funds. Options for participation of local resource users in decision-making arenas were generally scarce. Underlying processes were dominated by opacity and often low accountability of actors on all levels. Negative, but also positive affection of local residents by PA existence and management hence was high. Governance regimes of the complex performed very differently with regard to their ability of effectively empowering local village participatory bodies (vpb), generating and distributing benefits to individuals and village communities as well as providing mechanisms of conflict resolution. People around Pendjari enjoyed a relative wealth of high value benefits, while negative impacts caused by human-wildlife conflicts were widespread around the complex. Autochthonous farmers usually were better integrated in incentive schemes than were newcomers or herders. While there was functional separation of actors' roles in all parts of WAP, these roles differed significantly between blocks. Existence and functioning of village participatory bodies ameliorated the situation for local resource users fundamentally, as they acted as cut-points between different networks (governmental hierarchies, private concessionaires and local resource users). Vpbs in the Pendjari region proved to be most advanced in their capacity to push resource users' claims in action arenas on the micro-level. Via their union, these associations also managed to impact arenas on the meso- and the macro scale. Project interventions often had catalyst functions to empower local resource users and their vbps. However, they also contributed to social imbalance and intra-organisational competition. My results represent a snapshot of an ongoing process to establish effective co-governance regimes in the WAP-area. Though I identified a large scope of shortcomings, there were also very promising initiatives underway. This work is therefore meant to foster future research and further positive development by giving guidance scholars and decision-makers form the local to the global level alike.}, subject = {Gesch{\"u}tzte Natur}, language = {en} } @phdthesis{Heidinger2015, author = {Heidinger, Ina M. M.}, title = {Beyond metapopulation theory: Determinants of the dispersal capacity of bush crickets and grasshoppers}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-135068}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Habitat fragmentation and destruction due to anthropogenic land use are the major causes of the increasing extinction risk of many species and have a detrimental impact on animal populations in numerous ways. The long-term survival and stability of spatially structured populations in fragmented landscapes largely depends on the colonisation of habitat patches and the exchange of individuals and genes between patches. The degree of inter-patch dispersal, in turn, depends on the dispersal ability of a species (i.e. the combination of physiological and morphological factors that facilitate dispersal) and the landscape structure (i.e. the nature of the landscape matrix or the spatial configuration of habitat patches). As fragmentation of landscapes is increasing and the number of species is continuously declining, a thorough understanding of the causes and consequences of dispersal is essential for managing natural populations and developing effective conservation strategies. In the context of animal dispersal, movement behaviour is intensively investigated with capture-mark-recapture studies. For the analysis of such experiments, the influence of marking technique, handling and translocation of marked animals on movement pattern is of crucial importance since it may mask the effects of the main research question. Chapter 2 of this thesis presents a capture-mark-recapture study investigating the effect of translocation on the movement behaviour of the blue-winged grasshopper Oedipoda caerulescens. Transferring individuals of this grasshopper species to suitable but unfamilliar sites has a significant influence on their movement behaviour. Translocated individuals moved longer distances, showed smaller daily turning angles, and thus their movements were more directed than those of resident individuals. The effect of translocation was most pronounced on the first day of the experiment, but may persist for longer. On average, daily moved distances of translocated individuals were about 50 \% longer than that of resident individuals because they have been transferred to an unfamiliar habitat patch. Depending on experiment duration, this leads to considerable differences in net displacement between translocated and resident individuals. In summary, the results presented in chapter 2 clearly point out that translocation effects should not be disregarded in future studies on arthropod movement, respectively dispersal. Studies not controlling for possible translocation effects may result in false predictions of dispersal behaviour, habitat detection capability or habitat preferences. Beside direct field observations via capture-mark-recapture methods, genetic markers can be used to investigate animal dispersal. Chapter 3 presents data on the genetic structure of populations of Metrioptera bicolor, a wing-dimorphic bush cricket, in a spatially structured landscape with patches of suitable habitat distributed within a diverse matrix of different habitat types. Using microsatellite markers, the effects of geographic distance and different matrix types on the genetic differentiation among 24 local populations was assessed. The results of this study clearly indicate that for M. bicolor the isolation of local populations severely depends on the type of surrounding matrix. The presence of forest and a river running through the study area was positively correlated with the extent of genetic differentiation between populations. This indicates that both matrix types severely impede gene flow and the exchange of individuals between local populations of this bush cricket. In addition, for a subsample of populations which were separated only by arable land or settlements, a significant positive correlation between pairwise genetic and geographic distances exists. For the complete data set, this correlation could not be found. This is most probably due to the adverse effect of forest and river on gene flow which dominates the effect of geographic distance in the limited set of patches investigated in this study. The analyses in chapter 3 clearly emphasize the differential resistance of different habitat types on dispersal and the importance of a more detailed view on matrix 'quality' in metapopulation studies. Studies that focus on the specific dispersal resistance of different matrix types may provide much more detailed information on the dispersal capacity of species than a mere analysis of isolation by distance. Such information is needed to improve landscape oriented models for species conservation. In addition to direct effects on realised dispersal (see chapter 3), landscape structure on its own is known to act as an evolutionary selection agent because it determines the costs and benefits of dispersal. Both morphological and behavioural traits of individuals and the degree to which a certain genotype responds to environmental variation have heritable components, and are therefore expected to be able to respond to selection pressures. Chapter 4 analyses the influence of patch size, patch connectivity (isolation of populations) and sand dynamics (stability of habitat) on thorax- and wing length as proxies for dispersal ability of O. caerulescens in coastal grey dunes. This study revealed clear and sex-specific effects of landscape dynamics and patch configuration on dispersal-related morphology. Males of this grasshopper species were smaller and had shorter wings if patches were larger and less connected. In addition, both sexes were larger in habitat patches with high sand dynamics compared to those in patches with lower dynamics. The investments in wing length were only larger in connected populations when sand dynamics were low, indicating that both landscape and patch-related environmental factors are of importance. These results are congruent with theoretical predictions on the evolution of dispersal in metapopulations. They add to the evidence that dispersal-related morphology varies and is selected upon in recently structured populations even at small spatial scales. Dispersal involves different individual fitness costs like increased predation risk, energy expenditure, costs of developing dispersal-related traits, failure to find new suitable habitat as well as reproductive costs. Therefore, the decision to disperse should not be random but depend on the developmental stage or the physiological condition of an individual just as on actual environmental conditions (context-dependent dispersal, e.g. sex- and wing morph-biased dispersal). Biased dispersal is often investigated by comparing the morphology, physiology and behaviour of females and males or sedentary and dispersive individuals. Studies of biased dispersal in terms of capture-mark-recapture experiments, investigating real dispersal and not routine movements, and genetic proofs of biased dispersal are still rare for certain taxa, especially for orthopterans. However, information on biased dispersal is of great importance as for example, undetected biased dispersal may lead to false conclusions from genetic data. In chapter 5 of this thesis, a combined approach of morphological and genetic analyses was used to investigate biased dispersal of M. bicolor. The presented results not only show that macropterous individuals are predestined for dispersal due to their morphology, the genetic data also indicate that macropters are more dispersive than micropters. Furthermore, even within the group of macropterous individuals, males are supposed to be more dispersive than females. To get an idea of the flight ability of M. bicolor, the morphological data were compared with that of Locusta migratoria and Schistocerca gregaria, which are proved to be very good flyers. Based on the morphological data presented here, one can assume a good flight ability for macropters of M. bicolor, although flying individuals of this species are seldom observed in natural populations.}, subject = {Heuschrecken <{\"U}berfamilie>}, language = {en} } @phdthesis{MontalbandelBarrio2015, author = {Montalb{\´a}n del Barrio, Itsaso}, title = {Immunosuppressive role of adenosine produced by ectonucleotidases CD39 and CD73 in ovarian cancer, tumor associated macrophages and the host immune system}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-133268}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Eierstockkrebs ist der Tumor mit der schlechtesten Heilungsprognose unter allen gyn{\"a}kologischen Malignomen. Allein in Deutschland verursacht er {\"u}ber 6000 Tote pro Jahr. Patienten mit Ovarialkarzinom zeigen erst in einem sehr fortgeschrittenen Stadium charakteristische Symptome. Die einzig m{\"o}glichen Behandlungsmethoden sind dann die operative Tumorentfernung und die Verabreichung von platinbasierter Chemotherapien sowie von Anthrazyklinen. Da die aktuelle 5-Jahres-{\"U}berlebensrate lediglich 20-40\% betr{\"a}gt, besteht ein dringender Bedarf an neuen therapeutischen Optionen. Seit herausgefunden wurde, dass immunologische Parameter das {\"U}berleben der Patienten beeinflussen, ist Immuntherapie zu einer der vielversprechendsten Behandlungsarten des Eierstockkrebs geworden. Das Ziel unserer Forschung ist die {\"U}berwindung der Immunevasion des Tumors durch ein Verhindern der immun-unterdr{\"u}ckenden Mechanismen des Tumors. Im Speziellen befasst sich diese Arbeit mit dem Einfluss von Adenosin, das durch die Ectonukleotidasen CD39 und CD73 in der Mikroumgebung des Tumors gebildet wird. Die CD39- und CD73-Expression der Zellen f{\"u}hrt zu Immunosuppression da diese Ectonukleotidasen immun-stimulierendes, extrazellul{\"a}res ATP in immunsuppressives Adenosin umwandeln. Dies wurde zuerst als Effektormechanismus f{\"u}r regulatorische T-Zellen beschrieben, kann aber auch im Tumormikromilieu von Bedeutung sein. Mit dem Wissen, dass Tumorzellen von Eierstockkrebs-Patientinnen große Mengen der ATP-unterdr{\"u}ckenden Ectonukleotidasen CD39 und CD73 bilden, analysierten wir die adenosinvermittelte Unterdr{\"u}ckendung von Immunantwortenin der Mikroumgebung der Tumorzellen. Im Vergleich zu regulatorischen T Zellen konnten wir bei Eierstockkrebs-Zelllinien und bei aus Aszites gewonnenen Krebszellen eine 30- bis 60-fache Adenosinproduktion messen. Um diesen mutmaßlichen Immunevasions-Mechanismus zu best{\"a}tigen, untersuchten wir seine Auswirkungen auf mehrere Immunzellenpopulationen. CSFE-basierte Experimente zeigten zum Beispiel eine Hemmung der CD4+ T-Zell-Proliferation durch Adenosin, welches von Eierstockkrebs-Zellen produziert wurde. In diesem Zusammenhang haben wir auch eine in-vitro Methode entwickelt, mit der wir die Beeinflussung von Makrophagen durch Eierstockkrebszellen analysieren und modulieren konnten. Neben seiner suppressiven Wirkung {\"u}bt Adenosin auch chemotaktische Effekte auf menschliche Monozyten aus und lockt wahrscheinlich myeloide Vorl{\"a}uferzellen zum Tumorgewebe. Anschließend differenzieren sich menschliche Monozyten in einer von Eierstockkrebszellen geformten Mikroumgebung zu M2 Makrophagen oder tumor-assoziierten Makrophagen (TAMs), die ihrerseits erhebliche Mengen der Adenosin-produzierenden Ectonukleotidasen CD39 und CD73 bilden. W{\"a}hrend wir die Regulierung der Ectonukleotidasen-Expression untersuchten, entdeckten wir auch, dass klinisch genutzte Techniken zur Behandlung von Eierstockkrebs (zum Beispiel die Anwendung von Doxorubicin oder Bestrahlung) in vitro das CD73- und CD39-Level von Eierstockkrebs- und Immunzellen beeinflussen. In dieser Studie zeigen wir, wie dieser behandlungsbedingte Wechsel des ATP/Adenosine-Verh{\"a}ltnisses die Effektorfunktion verschiedener Immunzellen moduliert. Dar{\"u}ber hinaus untersuchen wir den potentiellen Vorteil von klinisch verf{\"u}gbaren, niedermolekularen Inhibitoren f{\"u}r CD39 und CD73, die die Immunsuppression in der Mikroumgebung des Tumors partiell aufheben k{\"o}nnten, und die vor allem in Kombination mit g{\"a}ngigen Behandlungsschemata von großem Interesse sein k{\"o}nnten.}, subject = {Eierstockkrebs}, language = {en} } @phdthesis{Wiese2015, author = {Wiese, Katrin Evelyn}, title = {Sensing supraphysiological levels of MYC : mechanisms of MIZ1-dependent MYC-induced Apoptosis in Mammary Epithelial Cells}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-132532}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Deregulated MYC expression contributes to cellular transformation as well as progression and maintenance of human tumours. Interestingly, in the absence of additional genetic alterations, potentially oncogenic levels of MYC sensitise cells to a variety of apoptotic stimuli. Hence, MYC-induced apoptosis has long been recognised as a major barrier against cancer development. However, it is largely unknown how cells discriminate physiological from supraphysiological levels of MYC in order to execute an appropriate biological response. The experiments described in this thesis demonstrate that induction of apoptosis in mammary epithelial cells depends on the repressive actions of MYC/MIZ1 complexes. Analysis of gene expression profiles and ChIP-sequencing experiments reveals that high levels of MYC are required to invade low-affinity binding sites and repress target genes of the serum response factor SRF. These genes are involved in cytoskeletal dynamics as well as cell adhesion processes and are likely needed to transmit survival signals to the AKT kinase. Restoration of SRF activity rescues MIZ1- dependent gene repression and increases AKT phosphorylation and downstream function. Collectively, these results indicate that association with MIZ1 leads to an expansion of MYC's transcriptional response that allows sensing of oncogenic levels, which points towards a tumour-suppressive role for the MYC/MIZ1 complex in epithelial cells.}, subject = {Myc}, language = {en} } @phdthesis{Hoecherl2015, author = {H{\"o}cherl, Nicole}, title = {Nesting behaviour of the paper wasp Polistes dominula - with special focus on thermoregulatory mechanisms}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-132681}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Wasps of the genus Polistes comprise over 200 species and are nearly cosmopolitan. They show a lack of physiological caste differentiation and are therefore considered as primitively eusocial. Furthermore, paper wasps are placed between the solitary living Eumenidae and the highly social organized Vespinae. Hence, they are often called a "key genus" for understanding the evolution of sociality. Particularly, Polistes dominula, with its small easy manageable nests and its frequent occurrence and wide distribution range is often the subject of studies. In Europe, the invasion of this species into northern regions is on the rise. Since little was known about the nesting behaviour of P. dominula in Central Europe, the basic principles about nesting were investigated in W{\"u}rzburg, Germany (latitude 49°) by conducting a comprehensive field-study spanning three consecutive years. Furthermore, the thermoregulation of individual wasps in their natural habitat had not yet been investigated in detail. Therefore, their ability to respond to external hazards with elevated thorax temperatures was tested. In addition, different types of nest thermoregulation were investigated using modern methods such as infrared thermography and temperature data logger. In the present work, the investigation of basic nesting principles revealed that foundress groups (1-4 foundresses) and nests are smaller and that the nesting season is shorter in the W{\"u}rzburg area than in other regions. The mean size of newly founded nests was 83 cells and the average nesting season was around 4.6 months. The queens neither preferred single (54\%) nor multiple founding (46\%) in this study. The major benefit of multiple founding is an increased rate of survival. During the three years of observation, only 47\% of single-foundress colonies survived, whereas 100\% of colonies that were built by more than two queens, survived. However, an influence of the number of foundresses on the productivity of colonies in terms of number of cells and pupae per nest has not shown up. However, the length of the nesting season as well as the nest sizes varied strongly depending on the climatic conditions of the preceding winter during the three consecutive years. In order to investigate the thermoregulatory mechanisms of individual adult P. dominula wasps, I presented artificial threats by applying smoke or carbon dioxide simulating fire and predator attacks, respectively, and monitored the thorax temperature of wasps on the nest using infrared thermography. The results clearly revealed that P. dominula workers recognized smoke and CO2 and reacted almost instantaneously and simultaneously with an increase of their thorax temperature. The maximal thorax temperature was reached about 65 s after the application of both stressors, but subsequently the wasps showed a different behaviour pattern. They responded to a longer application of smoke with moving to the exit and fled, whereas in case of CO2 the wasps started flying and circling the nest without trying to escape. No rise of the thorax temperature was detectable after an air blast was applied or in wasps resting on the nest. Additionally, the thorax temperatures of queens were investigated during dominance battles. I found that the thorax temperature of the dominant queens rose up to 5°C compared to that of subordinate queens that attacked the former. The study of active mechanisms for nest thermoregulation revealed no brood incubation or clustering behaviour of P. dominula. Furthermore, I found out that wing fanning for cooling the nest was almost undetectable (4 documented cases). However, I could convincingly record that water evaporation is most effective for nest cooling. By the direct comparison of active (with brood and adults) and non-active (without brood and adults) nests, the start of cooling by water evaporation was detected above maximum outside temperatures of 25°C or at nest temperatures above 35°C. The powerful role of water in nest cooling was manifested by an average decrease of temperature of a single cell of about 8°C and a mean duration of 7 min until the cell reached again its initial temperature. The investigation of passive thermoregulatory mechanisms revealed that the nest site choice as well as nest orientation appears to be essential for P. dominula wasps. Furthermore, I was able to show that the architecture of the nests plays an important role. Based on the presented results, it can be assumed that the vertical orientation of cells helps maintaining the warmth of nests during the night, whereas the pedicel assists in cooling the nest during the day.}, subject = {Franz{\"o}sische Feldwespe}, 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{Gnamlin2015, author = {Gnamlin, Prisca}, title = {Use of Tumor Vasculature for Successful Treatment of Carcinomas by Oncolytic Vaccinia Virus}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-119019}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Tumor-induced angiogenesis is of major interest for oncology research. Vascular endothelial growth factor (VEGF) is the most potent angiogenic factor characterized so far. VEGF blockade was shown to be sufficient for angiogenesis inhibition and subsequent tumor regression in several preclinical tumor models. Bevacizumab was the first treatment targeting specifically tumor-induced angiogenesis through VEGF blockade to be approved by the Food and Drugs Administration (FDA) for cancer treatment. However, after very promising results in preclinical evaluations, VEGF blockade did not show the expected success in patients. Some tumors became resistant to VEGF blockade. Several factors have been accounted responsible, the over-expression of other angiogenic factors, the noxious influence of VEFG blockade on normal tissues, the selection of hypoxia resistant neoplastic cells, the recruitment of hematopoietic progenitor cells and finally the transient nature of angiogenesis inhibition by VEGF blockade. The development of blocking agents against other angiogenic factors like placental growth factor (PlGF) and Angiopoietin-2 (Ang-2) allows the development of an anti-angiogenesis strategy adapted to the profile of the tumor. Oncolytic virotherapy uses the natural propensity of viruses to colonize tumors to treat cancer. The recombinant vaccinia virus GLV-1h68 was shown to infect, colonize and lyse several tumor types. Its descendant GLV-1h108, expressing an anti-VEGF antibody, was proved in previous studies to inhibit efficiently tumor induced angiogenesis. Additional VACVs expressing single chain antibodies (scAb) antibodies against PlGF and Ang-2 alone or in combination with anti VEGF scAb were designed. In this study, VACV-mediated anti-angiogenesis treatments have been evaluated in several preclinical tumor models. The efficiency of PlGF blockade, alone or in combination with VEGF, mediated by VACV has been established and confirmed. PlGF inhibition alone or with VEGF reduced tumor burden 5- and 2-folds more efficiently than the control virus, respectively. Ang-2 blockade efficiency for cancer treatment gave controversial results when tested in different laboratories. Here we demonstrated that unlike VEGF, the success of Ang-2 blockade is not only correlated to the strength of the blockade. A particular balance between Ang-2, VEGF and Ang-1 needs to be induced by the treatment to see a regression of the tumor and an improved survival. We saw that Ang-2 inhibition delayed tumor growth up to 3-folds compared to the control virus. These same viruses induced statistically significant tumor growth delays. This study unveiled the need to establish an angiogenic profile of the tumor to be treated as well as the necessity to better understand the synergic effects of VEGF and Ang-2. In addition angiogenesis inhibition by VACV-mediated PlGF and Ang-2 blockade was able to reduce the number of metastases and migrating tumor cells (even more efficiently than VEGF blockade). VACV colonization of tumor cells, in vitro, was limited by VEGF, when the use of the anti-VEGF VACV GLV-1h108 drastically improved the colonization efficiency up to 2-fold, 72 hours post-infection. These in vitro data were confirmed by in vivo analysis of tumors. Fourteen days post-treatment, the anti-VEGF virus GLV-1h108 was colonizing 78.8\% of the tumors when GLV-1h68 colonization rate was 49.6\%. These data confirmed the synergistic effect of VEGF blockade and VACV replication for tumor regression. Three of the tumor cell lines used to assess VACV-mediated angiogenesis inhibition were found, in certain conditions, to mimic either endothelial cell or pericyte functions, and participate directly to the vascular structure. The expression by these tumor cells of e-selectin, p-selectin, ICAM-1 and VCAM-1, normally expressed on activated endothelial cells, corroborates our findings. These proteins play an important role in immune cell recruitment, and there amount vary in presence of VEGF, PlGF and Ang-2, confirming the involvement of angiogenic factors in the immuno-modulatory abilities of tumors. In this study VACV-mediated angiogenesis blockade proved its potential as a therapeutic agent able to treat different tumor types and prevent resistance observed during bevacizumab treatment by acting on different factors. First, the expression of several antibodies by VACV would prevent another angiogenic factor to take over VEGF and stimulate angiogenesis. Then, the ability of VACV to infect tumor cells would prevent them to form blood vessel-like structures to sustain tumor growth, and the localized delivery of the antibody would decrease the risk of adverse effects. Next, the blockade of angiogenic factors would improve VACV replication and decrease the immune-modulatory effect of tumors. Finally the fact that angiogenesis blockade lasts until total regression of the tumor would prevent the recovery of the tumor-associated vasculature and the relapse of patients.}, subject = {Vaccinia-Virus}, 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{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} } @phdthesis{Czakai2015, author = {Czakai, Kristin Bernadette}, title = {Interaktionen des humanpathogenen Pilzes Aspergillus fumigatus mit dem angeborenen Immunsystem und Thrombozyten}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-117496}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Pilze sind in unserer Umwelt allgegenw{\"a}rtig und besiedeln im Fall von Candida albicans (C. albicans) sogar bei {\"u}ber 50\% der Menschen die Schleimh{\"a}ute, w{\"a}hrend Sporen von Aspergillus fumigatus (A. fumigatus) t{\"a}glich {\"u}ber die Atmung in die Lunge des Menschen gelangen. Dennoch sind Erkrankungen, die durch diese zwei Pilze ausgel{\"o}st werden, bei gesunden Menschen selten. Ist jedoch das Immunsystem beeintr{\"a}chtigt, k{\"o}nnen diese Pilze zu systemischen und damit lebensbedrohlichen Erkrankungen wie der invasiven Aspergillose und der systemischen Candidiasis f{\"u}hren. F{\"u}r eine Verbesserung der Behandlung solcher Infektionen ist das genaue Verst{\"a}ndnis der Immunabwehrmechanismen entscheidend. Da A. fumigatus {\"u}ber die Lunge in den K{\"o}rper gelangt, wurden in dieser Arbeit die h{\"a}ufigsten Immunzellen der Lunge, die Makrophagen, und deren Immunantwort auf A. fumigatus untersucht. Parallel hierzu wurden dendritische Zellen (DCs) verwendet, die als Br{\"u}cke zwischen dem angeborenen und adaptiven Immunsystem wirken. Ein besonderes Augenmerk wurde hierbei auf A. fumigatus induzierte Genexpressions{\"a}nderungen und deren Regulationsmechanismen gelegt. Dabei wurden kurze, regulatorische RNAs, die sogenannten miRNAs, untersucht, die eine wichtige Rolle in der post-transkriptionalen Genregulation spielen. Bislang ist nur wenig {\"u}ber die miRNA-abh{\"a}ngigen Genregulationen in DCs, die auf eine Infektion mit A. fumigatus oder C. albicans reagieren, bekannt. Um alle durch A. fumigatus und C. albicans regulierten miRNAs zu identifizieren, wurden DCs mit A. fumigatus und C. albicans ko-kultiviert und anschließend eine Komplettsequenzierung der kurzen RNAs durchgef{\"u}hrt. Die Pilz-spezifische Induktion der miRNA-Regulation wurde zudem mit der miRNA-Regulation durch den bakteriellen Zellwandbestandteil Lipopolysaccharid verglichen. Durch die Stimulation mit Keimschl{\"a}uchen von A. fumigatus wurden die miRNAs miR-132-3p/5p, miR-155-5p, miR129-2-3p, miR-129-5p, miR-212-3p/5p und miR-9-5p in DCs induziert. Diese wurden ebenfalls durch C. albicans induziert, zudem noch die miRNAs miR-147a und miR-147b. Spezifisch f{\"u}r A. fumigatus war die Regulation der miR-129-2-3p. Neben dem miRNA-Profiling wurde auch das mRNA-Transkriptom {\"u}ber Microarrays analysiert und dadurch 18 potentielle Zielgene der Pilz-induzierten miRNAs identifiziert. Neben den Elementen der Translationsregulation wurden auch die Transkriptionsfaktoren untersucht. Als einziger unter den 60 regulierten Transkriptionsfaktoren zeigte KLF4 eine ver{\"a}nderte Expressionsrichtung in DCs, die mit Pilzen oder LPS behandelt waren. W{\"a}hrend die Stimulation mit LPS die Expression von KLF4 induzierte, wurde es durch die Pilze A. fumigatus und C. albicans reprimiert. In einer Untersuchung der unterschiedlichen A. fumigatus-Rezeptoren, wurde deren Einfluss auf die KLF4-Regulation gezeigt. W{\"a}hrend TLR4-Liganden KLF4 induzierten, f{\"u}hrten Liganden, die an die Rezeptoren TLR2/TLR1 und Dectin-1 binden, zu einer Reduktion von KLF4. Nach einem erfolgreich etablierten KLF4-knock-down mittels RNA-Interferenz wurden KLF4-Zielgene untersucht. W{\"a}hrend kein bzw. nur ein geringer Effekt auf die Genexpression von CCL2, RANTES, CXCL10 und TNF beobachtet wurde, sorgte der KLF4 knock-down f{\"u}r eine hoch signifikante Reduktion der IL6-Genexpression in LPS-stimulierten DCs. Um die KLF4-Regulation weiter zu untersuchen, wurde zudem eine weitere Zellpopulation des angeborenen Immunsystems, die Makrophagen, verwendet. Auch hier wurde die Immunantwort gegen A. fumigatus analysiert. Zudem wurde die Rolle der Thrombozyten als Immunmediatoren betrachtet. Zuerst wurde ein Zytokinprofil des pl{\"a}ttchenreichen Plasmas (PRP), das mit A. fumigatus stimuliert wurde, erstellt. In diesem konnte nur RANTES in hoher Konzentration nachgewiesen werden. Daraufhin wurde der Einfluss von PRP auf die Reifung von DCs, die Phagozytosef{\"a}higkeit von Makrophagen und DCs sowie der Einfluss von DCs und Makrophagen auf die metabolische Aktivit{\"a}t von A. fumigatus in An- und Abwesenheit von pl{\"a}ttchenreichem Plasma untersucht. Es konnte eine gering verst{\"a}rkte Reifung der DCs durch PRP gezeigt werden. Isolierte Thrombozyten konnten die Phagozytose von DCs steigern, w{\"a}hrend Makrophagen durch PRP verst{\"a}rkt Konidien phagozytierten. In einem genomweiten Transkriptomprofiling wurde die Immunantwort von DCs und Makrophagen verglichen. Zudem wurde untersucht, wie PRP die Immunantwort dieser Immunzellen beeinflusst. Es wurden 2 bzw. 24 Gene identifiziert, die signifikant in A. fumigatus-stimulierten DCs und Makrophagen reguliert waren. Hierbei wurde gezeigt, dass KLF4 durch die Zugabe von PRP herabreguliert wurde. Das zuvor beschriebene Zielgen IL6 wurde durch PRP in A. fumigatus-stimulierten DCs gegen{\"u}ber stimulierten DCs ohne PRP deutlich reduziert, wodurch sich eine immunmodulatorische F{\"a}higkeit des PRP zeigte. Die Induktion von IL-6, weiteren Zytokinen und der Reifemarker durch A. fumigatus in DCs wurden zudem in einem Booleschen Modell simuliert. Dieses Modell soll in Zukunft Vorhersagen {\"u}ber experimentelle Ergebnisse und dadurch eine optimale Versuchsvorbereitung erm{\"o}glichen.}, subject = {Aspergillus fumigatus}, language = {de} } @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{Bruttel2015, author = {Bruttel, Valentin Stefan}, title = {Soluble HLA-G binds to dendritic cells which likely suppresses anti-tumour immune responses in regional lymph nodes in ovarian carcinoma}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-127252}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Zusammenfassung Einleitung HLA-G, ein nicht-klassisches HLA bzw. MHC Klasse Ib Molek{\"u}l, kann sowohl als membrangebundenes als auch als l{\"o}sliches Molek{\"u}l verschiedenste Immunzellpopulationen effektiv inhibieren. Unter physiologischen Bedingungen wird HLA-G vor allem in der Plazenta exprimiert, wo es dazu beitr{\"a}gt den semiallogenen Embryo vor einer Abstoßung durch das m{\"u}tterliche Immunsystem zu besch{\"u}tzen. Außerdem wird HLA-G in einer Vielzahl von Tumoren wie zum Beispiel in Ovarialkarzinomen {\"u}berexprimiert. Ziel dieser Arbeit war es besonders die Rolle von l{\"o}slichem HLA-G im Ovarialkarzinom und die Expression von HLA-G in verschiedenen Subtypen des Ovarialkarzinoms genauer zu untersuchen. Ergebnisse Anhand eines Tissue Microarrays wurde best{\"a}tigt dass HLA-G unter physiologischen Bedingungen nur in sehr wenigen Geweben wie Plazenta oder Testes exprimiert wird. Außerdem wurden erstmals auch im Nebennierenmark hohe Expressionslevel detektiert. Im Gegensatz zur physiologischen Expression wurde HLA-G in ser{\"o}sen, muzin{\"o}sen, endometrioiden und Klarzellkarzinomen und somit in Tumoren aller untersuchten Subtypen des Ovarialkarzinoms detektiert. Am h{\"a}ufigsten war HLA-G in hochgradigen ser{\"o}sen Karzinomen {\"u}berexprimiert. Hier konnte gezeigt werden dass auf Genexpressionslevel in Ovarialkarzinomen die Expression des immunsuppressiven HLA-G mit der Expression von klassischen MHC Molek{\"u}len wie HLA-A, -B oder -C hochsignifikant korreliert. Außerdem konnte in Aszitesproben von Patientinnen mit Ovarialkarzinomen hohe Konzentrationen von l{\"o}slichem HLA-G nachgewiesen werden. Auch auf metastasierten Tumorzellen in regionalen Lymphknoten war HLA-G nachweisbar. {\"U}berraschenderweise wurde aber besonders viel HLA-G auf Dendritischen Zellen in Lymphknoten detektiert. Da in Monozyten und Dendritischen Zellen von gesunden Spendern durch IL-4 oder IL-10 im Gegensatz zu Literatur keine Expression von HLA-G induzierbar war, untersuchten wir ob Dendritische Zellen l{\"o}sliches HLA-G binden. Es konnte gezeigt werden, dass besonders Dendritische Zellen die in Gegenwart von IL-4, IL-10 und GM-CSF aus Monozyten generiert wurden (DC-10) effektiv l{\"o}sliches HLA-G {\"u}ber ILT Rezeptoren binden. In Abh{\"a}ngigkeit von ihrer Beladung mit HLA-G hemmen auch fixierte DC-10 Zellen noch die Proliferation von zytotoxischen CD8+ T Zellen. Zudem wurden regulatorische T Zellen induziert. Schlussfolgerungen Besonders in den am h{\"a}ufigsten diagnostizierten hochgradigen ser{\"o}sen Ovarialkarzinomen ist HLA-G in den meisten F{\"a}llen {\"u}berexprimiert. Durch die Expression immunsuppressiver MHC Klasse Ib Molek{\"u}le wie HLA-G k{\"o}nnen wahrscheinlich auch Tumore wachsen, die noch klassische MHC Molek{\"u}le exprimieren und aufgrund ihrer Mutationslast eigentlich vom Immunsystem erkannt und eliminiert werden m{\"u}ssten. L{\"o}sliches HLA-G k{\"o}nnte zudem lokal Immunantworten gegen Tumorantigene unterdr{\"u}cken indem es an Dendritische Zellen in regionalen Lymphknoten bindet. Diese Zellen pr{\"a}sentieren nomalerweise zytotoxischen T Zellen Tumorantigene und spielen daher eine entscheidende Rolle in der Entstehung von protektiven Immunantworten. Mit l{\"o}slichem HLA-G beladene Dendritische Zellen hemmen jedoch die Proliferation von CD8+ T Zellen und induzieren regulatorische T Zellen. Dadurch k{\"o}nnten Ovarialkarzinome "aus der Ferne" auch in metastasenfreien Lymphknoten die Entstehung von gegen den Tumor gerichteten Immunantworten unterdr{\"u}cken. Dieser erstmals beschriebene Mechanismus k{\"o}nnte auch in anderen malignen Erkrankungen eine Rolle spielen, da l{\"o}sliches HLA-G in einer Vielzahl von Tumorindikationen nachgewiesen wurde.}, subject = {HLA-G}, language = {en} } @phdthesis{Kuger2015, author = {Kuger, Sebastian}, title = {Radiosensibilisierung humaner Tumorzelllinien unterschiedlicher Entit{\"a}ten durch den dualen PI3K/mTOR-Inhibitor NVP-BEZ235 alleine oder in Kombination mit dem MEK-Inhibitor AZD6244: Einfluss des Behandlungsschemas und der Hypoxie}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-126715}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2015}, abstract = {Eine wichtige Standardtherapie in der modernen Behandlung von Krebserkrankungen ist die Strahlentherapie, in welcher Tumorzellen mittels ionisierender Strahlung gesch{\"a}digt und abget{\"o}tet werden. Dabei soll die Sch{\"a}digung des umgebenden Normalgewebes m{\"o}glichst gering gehalten und trotzdem eine maximale Sch{\"a}digung des Tumorgewebes erreicht werden. Deshalb sind neue Strategien zur Steigerung der Radiosensitivit{\"a}t des Tumorgewebes sehr wichtig, die es erlauben, bei gleicher Dosis eine verst{\"a}rkte Strahlenantwort im Tumorgewebe zu erreichen. Hier kommen zunehmend sog. Radiosensibilisatoren zum Einsatz, die unter anderem onkogene Signalwege in den Tumorzellen inhibieren. Der PI3K/Akt/mTOR Signalweg stellt hierbei einen wichtigen Ansatzpunkt dar, da er in vielen Tumorentit{\"a}ten dereguliert vorliegt und diese Signalkaskade bekanntermaßen einen Einfluss auf die zellul{\"a}re Strahlensensitivit{\"a}t hat. Obwohl es f{\"u}r diesen Signalweg schon eine Reihe von Inhibitoren gibt, f{\"u}r die bereits neben einer anti-proliferativen Wirkung auch ein radiosensibilisierender Effekt nachgewiesen wurde (z.B. Wortmannin und Rapamycin), machten eine geringe Spezifit{\"a}t, starke Nebenwirkungen und negative R{\"u}ckkopplungsmechanismen im Signalweg, die die Wirkung des Inhibitors kompensieren, die Entwicklung neuer Inhibitoren notwendig. Das Imidazoquinolinderivat NVP-BEZ235 inhibiert den PI3K/Akt/mTOR Signalweg an mehreren Stellen gleichzeitig, indem es kompetitiv zu ATP das katalytische Zentrum von PI3K und mTOR blockiert. F{\"u}r diesen kleinmolekularen, dualen Inhibitor gibt es bereits erste vielversprechende Forschungsergebnisse hinsichtlich einer radiosensibilisierenden Wirkung, allerdings sind die zugrunde liegenden molekularbiologischen Mechanismen noch nicht vollst{\"a}ndig gekl{\"a}rt. Deshalb war das Ziel der vorliegenden Dissertation, in drei Teilprojekten mehrere Aspekte der NVP-BEZ235-induzierten Radiosensibilisierung aufzukl{\"a}ren: a) Einfluss des Behandlungsschemas f{\"u}r NVP-BEZ235 in vier Glioblastomzelllinien mit unterschiedlichem PTEN und TP53 Mutationsstatus, b) Einfluss der Sauerstoffversorgung (Hypoxie, Normoxie, reoxygeniert nach Bestrahlung) auf die strahlensensibilisierende Wirkung von NVP-BEZ235 in zwei Mammakarzinomzelllinien, c) gleichzeitige Inhibierung des MAPK Signalwegs durch AZD6244 und der PI3K/Akt/mTOR Signalkaskade durch NVP-BEZ235 in zwei Zelllinien mit unter-schiedlichem Mutationsstatus aus verschiedenen Tumorentit{\"a}ten, um synergistische Effekte zu untersuchen. Um diese Fragestellungen zu beantworten, wurde im Rahmen - 142 - der Dissertation eine Auswahl an humanen Tumorzelllinien mit unterschiedlich deregulierten Signalwegen bearbeitet. Dabei wurde die Expression von Schl{\"u}sselproteinen der MAPK/Erk und der PI3K/Akt/mTOR Signalwege analysiert und mit zellbiologischen Daten verschiedener ph{\"a}notypischer Endpunkte nach Inhibitor Behandlung und Bestrahlung integriert (Proliferationsrate, klonogenes {\"U}berleben, Zellzyklusaberrationen, DNS-Sch{\"a}den und -Reparatur, Zelltod und Autophagie). Im Teilprojekt zum Behandlungsschema der NVP-BEZ235 Inhibierung und Bestrahlung konnte in vier Glioblastomzelllinien mit Behandlungsschema I (NVP-BEZ235 Behandlung 24 Stunden vor Bestrahlung) kein radiosensibilisierender Effekt hinsichtlich klonogenem {\"U}berleben nachgewiesen werden, wohingegen Behandlungsschema II (NVP-BEZ235 Behandlung 1 h vor und im Anschluss an die Bestrahlung) unabh{\"a}ngig vom Mutationsstatus in allen vier Zelllinien eine starke Radiosensibilisierung bewirkte. Auf molekularer Ebene war zwischen beiden Behandlungsschemata f{\"u}r das antiapoptotische Protein Akt ein großer Unterschied zu beobachten, welches bei Behandlung nach Schema I zum Zeitpunkt der Bestrahlung {\"u}beraktiviert, nach Behandlung mit Schema II hingegen inhibiert war. Weiterhin resultierte Behandlungsschema I in einem erh{\"o}hten Anteil der Zellen in der radioresistenteren G1-Phase des Zellzyklus zum Zeit-punkt der Bestrahlung. Behandlungsschema II f{\"u}hrte hingegen nach Bestrahlung zu einer verminderten Expression des Reparaturproteins Rad51 und damit zu verminderter DNS-Schadensreparatur und schließlich zu einem stabilen Arrest in der G2/M-Phase des Zellzyklus sowie zu verst{\"a}rkter Apoptose (erh{\"o}hte Spaltung von PARP, erh{\"o}hter Anteil hypodiploider Zellen). Somit zeigen diese Ergebnisse, dass unabh{\"a}ngig vom PTEN und TP53 Mutationsstatus eine Radiosensibilisierung nur durch das Behandlungsschema II erreicht werden konnte. Ferner deuten die Ergebnisse der Proteinexpression darauf hin, dass durch NVP-BEZ235 ein negativer R{\"u}ckkopplungsmechanismus ausgel{\"o}st wird, wodurch die PI3K/Akt/mTOR Signalkaskade 24h nach Zugabe des Inhibitors aktiviert und synergistische Effekte mit ionisierender Bestrahlung aufgehoben wurden. Im Teilprojekt zur Abh{\"a}ngigkeit der NVP-BEZ235 Inhibition vom Sauerstoffgehalt wurden in den beiden Brustkrebszelllinien MCF-7 (ER-positiv) und TN MDA-MB-231 (TP53 mutiert) normoxische, hypoxische und nach Bestrahlung reoxygenierte Kulturbedingungen im Hinblick auf die Koloniebildungsf{\"a}higkeit nach NVP-BEZ235 Behandlung und Bestrahlung untersucht. Die beobachtete Radiosensibilisierung war unter allen getesteten Bedingungen auf gleichem Niveau. In beiden Zelllinien bewirkte NVP-BEZ235 eine Inhibition des antiapoptotischen HIF-1α Proteins, eine stabile Inaktivierung des PI3K/Akt/mTOR Signalweges und eine Aktivierung der Autophagie. Nach Bestrahlung waren zudem erh{\"o}hte residuale DNS-Sch{\"a}den und ein stabiler Arrest in der G2/M-Phase des Zellzyklus unter allen Oxygenierungsbedingungen in beiden Zelllinien zu beobachten. Eine Apoptose Induktion (Spaltung von PARP, hypodiploide Zellen) trat nur in der TP53 wildtypischen MCF-7 Zelllinie nach NVP-BEZ235 Behandlung auf. Somit konnte in beiden Zelllinien in allen pathophysiologisch relevanten Oxygenierungszust{\"a}nden eine sauerstoffunabh{\"a}ngige Radiosensibilisierung durch NVP-BEZ235 gezeigt werden. Der bisher nicht erforschte Aspekt zur synergistischen Wirkung des MEK Inhibitors AZD6244 und des dualen PI3K/Akt/mTOR Inhibitors NVP-BEZ235 nach Bestrahlung wurde an der Glioblastomzelllinie SNB19 und der Lungenkarzinomzelllinie A549 anhand der Koloniebildungsf{\"a}higkeit der behandelten Zellen untersucht. Eine Behandlung mit dem MEK Inhibitor bewirkte lediglich eine moderate Radiosensibilisierung, wohin-gegen der duale PI3K/Akt/mTOR Inhibitor beide Zelllinien in st{\"a}rkerem Maße sensibilisierte. Eine Kombination beider Inhibitoren resultierte bei keiner Zelllinie in einer Verst{\"a}rkung der durch NVP-BEZ235 induzierten Radiosensibilisierung. Eine m{\"o}gliche Erkl{\"a}rung f{\"u}r die fehlende Synergie im Bezug auf die Radiosensibilisierung k{\"o}nnen die gegens{\"a}tzlichen Effekte der beiden Inhibitoren auf den Zellzyklus sein. Auf Proteinebene f{\"u}hrte eine simultane Behandlung mit beiden Substanzen zur Inhibition beider Signalwege. Dar{\"u}ber hinaus war in SNB19 Zellen eine verst{\"a}rkte Dephosphorylierung von Rb und ein erh{\"o}hter Anteil an G1-Phase Zellen bei kombinierter Gabe der Inhibitoren zu beobachten. Im Rahmen dieser Arbeit konnte somit die radiosensibilisierende Wirkung von NVP-BEZ235 in Abh{\"a}ngigkeit vom Behandlungsschema gezeigt werden. Ferner wurde nachgewiesen, dass die Radiosensibilisierung unabh{\"a}ngig von der Sauerstoffversorgung sowie von den PTEN und TP53 Mutationsstatus der Tumorzellen ist. Die kombinierte Inhibition der MAPK und PI3K/Akt/mTOR Signalwege resultierte zwar in einem verst{\"a}rkten zytostatischen, aber nicht in einem verst{\"a}rkten radiosensibilisierenden Effekt. Da allerdings eine große Anzahl verschiedener Inhibitoren der MAPK/Erk und der PI3K/Akt/mTOR Signalkaskade verf{\"u}gbar sind, sollte die kombinatorische Inhibition dieser Signalwege systematisch weiter verfolgt werden. Die vorliegende Arbeit liefert auch weitere grundlegende Erkenntnisse zu den molekularen Mechanismen der Radiosensibilisierung durch NVP-BEZ235, die auch auf Verkn{\"u}pfungen und Wechselwirkungen mit anderen als den bisher bekannten Proteinen hindeuten, die f{\"u}r jeden Inhibitor aufgekl{\"a}rt werden m{\"u}ssen, um eine effektive radiosensibilisierende Wirkung vorher-sagen zu k{\"o}nnen.}, subject = {Strahlensensibilisator}, language = {de} } @article{StrubeBlossBrownSpaetheetal.2015, author = {Strube-Bloss, Martin F. and Brown, Austin and Spaethe, Johannes and Schmitt, Thomas and R{\"o}ssler, Wolfgang}, title = {Extracting the Behaviorally Relevant Stimulus: Unique Neural Representation of Farnesol, a Component of the Recruitment Pheromone of Bombus terrestris}, series = {PLoS One}, volume = {10}, journal = {PLoS One}, number = {9}, doi = {10.1371/journal.pone.0137413}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-125875}, pages = {e0137413}, year = {2015}, abstract = {To trigger innate behavior, sensory neural networks are pre-tuned to extract biologically relevant stimuli. Many male-female or insect-plant interactions depend on this phenomenon. Especially communication among individuals within social groups depends on innate behaviors. One example is the efficient recruitment of nest mates by successful bumblebee foragers. Returning foragers release a recruitment pheromone in the nest while they perform a 'dance' behavior to activate unemployed nest mates. A major component of this pheromone is the sesquiterpenoid farnesol. How farnesol is processed and perceived by the olfactory system, has not yet been identified. It is much likely that processing farnesol involves an innate mechanism for the extraction of relevant information to trigger a fast and reliable behavioral response. To test this hypothesis, we used population response analyses of 100 antennal lobe (AL) neurons recorded in alive bumblebee workers under repeated stimulation with four behaviorally different, but chemically related odorants (geraniol, citronellol, citronellal and farnesol). The analysis identified a unique neural representation of the recruitment pheromone component compared to the other odorants that are predominantly emitted by flowers. The farnesol induced population activity in the AL allowed a reliable separation of farnesol from all other chemically related odor stimuli we tested. We conclude that the farnesol induced population activity may reflect a predetermined representation within the AL-neural network allowing efficient and fast extraction of a behaviorally relevant stimulus. Furthermore, the results show that population response analyses of multiple single AL-units may provide a powerful tool to identify distinct representations of behaviorally relevant odors.}, language = {en} } @article{LichtensteinSommerlandtSpaethe2015, author = {Lichtenstein, Leonie and Sommerlandt, Frank M. J. and Spaethe, Johannes}, title = {Dumb and Lazy? A Comparison of Color Learning and Memory Retrieval in Drones and Workers of the Buff-Tailed Bumblebee, Bombus terrestris, by Means of PER Conditioning}, series = {PLoS One}, volume = {10}, journal = {PLoS One}, number = {7}, doi = {10.1371/journal.pone.0134248}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-125832}, pages = {e0134248}, year = {2015}, abstract = {More than 100 years ago, Karl von Frisch showed that honeybee workers learn and discriminate colors. Since then, many studies confirmed the color learning capabilities of females from various hymenopteran species. Yet, little is known about visual learning and memory in males despite the fact that in most bee species males must take care of their own needs and must find rewarding flowers to obtain food. Here we used the proboscis extension response (PER) paradigm to study the color learning capacities of workers and drones of the bumblebee, Bombus terrestris. Light stimuli were paired with sucrose reward delivered to the insects' antennae and inducing a reflexive extension of the proboscis. We evaluated color learning (i.e. conditioned PER to color stimuli) in absolute and differential conditioning protocols and mid-term memory retention was measured two hours after conditioning. Different monochromatic light stimuli in combination with neutral density filters were used to ensure that the bumblebees could only use chromatic and not achromatic (e.g. brightness) information. Furthermore, we tested if bees were able to transfer the learned information from the PER conditioning to a novel discrimination task in a Y-maze. Both workers and drones were capable of learning and discriminating between monochromatic light stimuli and retrieved the learned stimulus after two hours. Drones performed as well as workers during conditioning and in the memory test, but failed in the transfer test in contrast to workers. Our data clearly show that bumblebees can learn to associate a color stimulus with a sugar reward in PER conditioning and that both workers and drones reach similar acquisition and mid-term retention performances. Additionally, we provide evidence that only workers transfer the learned information from a Pavlovian to an operant situation.}, language = {en} }