@phdthesis{Cicova2016, author = {Cicova, Zdenka}, title = {Characterization of a novel putative factor involved in host adaptation in Trypanosoma brucei}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-142462}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2016}, abstract = {Trypanosomes are masters of adaptation to different host environments during their complex life cycle. Large-scale proteomic approaches provide information on changes at the cellular level in a systematic way. However, a detailed work on single components is necessary to understand the adaptation mechanisms on a molecular level. Here we have performed a detailed characterization of a bloodstream form (BSF) stage-specific putative flagellar host adaptation factor (Tb927.11.2400) identified previously in a SILAC-based comparative proteome study. Tb927.11.2400 shares 38\% amino acid identity with TbFlabarin (Tb927.11.2410), a procyclic form (PCF) stage specific flagellar BAR domain protein. We named Tb927.11.2400 TbFlabarin like (TbFlabarinL) and demonstrate that it is a result of a gene duplication event, which occurred in African trypanosomes. TbFlabarinL is not essential for growth of the parasites under cell culture conditions and it is dispensable for developmental differentiation from BSF to the PCF in vitro. We generated a TbFlabarinL-specific antibody and showed that it localizes in the flagellum. The co-immunoprecipitation experiment together with a biochemical cell fractionation indicated a dual association of TbFlabarinL with the flagellar membrane and the components of the paraflagellar rod.}, subject = {Trypanosoma brucei}, language = {en} } @phdthesis{Gloeckner2001, author = {Gl{\"o}ckner, Herma}, title = {Characterization of a new miniaturized hollow-fiber bioreactor for cultivation of cell lines and primary cells to improve cytostatic drug testing in vitro}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-1181317}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2001}, abstract = {Monolayer or suspension cell cultures are of only limited value as experimental models for human cancer. Therefore, more sophisticated, three-dimensional culture systems like spheroid cultures or histocultures are used, which more closely mimic the tumor in individual patients compared to monolayer or suspension cultures. As tissue culture or tissue engineering requires more sophisticated culture, specialized in vitro techniques may also improve experimental tumor models. In the present work, a new miniaturized hollow-fiber bioreactor system for mammalian cell culture in small volumes (up to 3 ml) is characterized with regard to transport characteristics and growth of leukemic cell lines (chapter 2). Cell and medium compartment are separated by dialysis membranes and oxygenation is accomplished using oxygenation membranes. Due to a transparent housing, cells can be observed by microscopy during culture. The leukemic cell lines CCRF-CEM, HL-60 and REH were cultivated up to densities of 3.5 x 107/ml without medium change or manipulation of the cells. Growth and viability of the cells in the bioreactor were the same or better, and the viable cell count was always higher compared to culture in Transwell{\^a} plates. As shown using CCRF-CEM cells, growth in the bioreactor was strongly influenced and could be controlled by the medium flow rate. As a consequence, consumption of glucose and generation of lactate varied with the flow rate. Influx of low molecular weight substances in the cell compartment could be regulated by variation of the concentration in the medium compartment. Thus, time dependent concentration profiles (e.g. pharmacokinetic profiles of drugs) can be realized as illustrated using glucose as a model compound. Depending on the molecular size cut-off of the membranes used, added growth factors like GM-CSF and IL-3 as well as factors secreted from the cells are retained in the cell compartment for up to one week. Second, a method for monitoring cell proliferation the hollow-fiber bioreactor by use of the Alamar BlueTM dye was developed (chapter 3). Alamar BlueTM is a non-fluorescent compound which yields a fluorescent product after reduction e.g. by living cells. In contrast to the MTT-assay, the Alamar BlueTM-assay does not lead to cell death. However, when not removed from the cells, the Alamar BlueTM dye shows a reversible, time- and concentration-dependent growth inhibition as observed for leukemic cell lines. When applied in the medium compartment of a hollow-fiber bioreactor system, the dye is delivered to the cells across the hollow-fiber membrane, reduced by the cells and released from the cell into the medium compartment back again. Thus, fluorescence intensity can be measured in medium samples reflecting growth of the cells in the cell compartment. This procedure offers several advantages. First, exposure of the cells to the dye can be reduced compared to conventional culture in plates. Second, handling steps are minimized since no sample of the cells needs to be taken for readout. Moreover, for the exchange of medium, a centrifugation step can be avoided and the cells can be cultivated further. Third, the method allows to discriminate between cell densities of 105, 106 and 107 of proliferating HL-60 cells cultivated in the cell compartment of the bioreactor. Measurement of fluorescence in the medium compartment is more sensitive compared to glucose or lactate measurement for cell counts below 106 cells/ml, in particular. In conclusion, the Alamar BlueTM-assay combined with the hollow-fiber bioreactor offers distinct advantages for the non-invasive monitoring of cell viability and proliferation in a closed system. In chapter 4 the use of the hollow-fiber bioreactor as a tool for toxicity testing was investigated, as current models for toxicity as well as efficacy testing of drugs in vitro allow only limited conclusions with regard to the in vivo situation. Examples of the drawbacks of current test systems are the lack of realistic in vitro tumor models and difficulties to model drug pharmacokinetics. The bioreactor proved to be pyrogen free and is steam-sterilizable. Leukemic cell lines like HL-60 and primary cells such as PHA-stimulated lymphocytes can be grown up to high densities of 1-3 x 107 and analyzed during growth in the bioreactor by light-microscopy. The cytostatic drug Ara-C shows a dose-dependent growth inhibition of HL-60 cells and a dose-response curve similar to controls in culture plates. The bioreactor system is highly flexible since several systems can be run in parallel, soluble drugs can be delivered continuously via a perfusion membrane and gaseous compounds via an oxygenation membrane which also allows to control pO2 and pH (via pCO2) during culture in the cell compartment. The modular concept of the bioreactor system allows realization of a variety of different design properties, which may lead to an improved in vitro system for toxicity testing by more closely resembling the in vivo situation. Whereas several distinct advantages of the new system have been demonstrated, more work has to be done to promote in vitro systems in toxicity testing and drug development further and to reduce the need for animal tests.}, subject = {Hohlfaserreaktor}, language = {en} } @phdthesis{Hart2004, author = {Hart, Stefan}, title = {Characterisation of the molecular mechanisms of EGFR signal transactivation in human cancer}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-10067}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2004}, abstract = {In a variety of established tumour cell lines, but also in primary mammary epithelial cells metalloprotease-dependent transactivation of the EGFR, and EGFR characteristic downstream signalling events were observed in response to stimulation with physiological concentrations of GPCR agonists such as the mitogens LPA and S1P as well as therapeutically relevant concentrations of cannabinoids. Moreover, this study reveals ADAM17 and HB-EGF as the main effectors of this mechanism in most of the cancer cell lines investigated. However, depending on the cellular context and GPCR agonist, various different members of the ADAM family are selectively recruited for specific ectodomain shedding of proAR and/or proHB-EGF and subsequent EGFR activation. Furthermore, biological responses induced by LPA or S1P such as migration in breast cancer and HNSCC cells, depend on ADAM17 and proHB-EGF/proAR function, respectively, suggesting that highly abundant GPCR ligands may play a role in tumour development and progression. Moreover, EGFR signal transactivation could be identified as the mechanistic link between cannabinoid receptors and the activation of mitogen activated protein kinases (MAPK) ERK1/2 as well as pro-survival Akt/PKB signalling. Depending on the cellular context, cannabinoid-induced signal cross-communication was mediated by shedding of proAmphiregulin and/or proHB-EGF by ADAM17. Most importantly, our data show that concentrations of THC comparable to those detected in the serum of patients after THC administration accelerate proliferation of cancer cells instead of apoptosis and thereby may contribute to cancer progression in patients.}, subject = {Epidermaler Wachstumsfaktor-Rezeptor}, language = {en} } @phdthesis{Schneider2011, author = {Schneider, Matthias}, title = {Characterisation of Metalloprotease-mediated EGFR Signal Transactivation after GPCR Stimulation}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-65105}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2011}, abstract = {In the context of metalloprotease-mediated transactivation of the epidermal growth factor receptor, different monoclonal antibodies against ADAM17 / TACE were characterized for their ability to block the sheddase. Activity of some of them was observed at doses between 2µg/mL and 10µg/mL. Kinetic analyses showed their activity starting at around 30 minutes. In cellular assays performed with the antibodies, especially upon treatment of cells with sphingosine-1-phosphate a reduction in proliferation was observed with some candidates. Moreover this study provides potential new roles for ß-Arrestins. Their involvement in the triple membrane-passing signal pathway of EGFR transactivation was shown. Furthermore, in overexpressing cellular model systems, an interaction between ADAM17 and ß-Arrestin1 could be observed. Detailed analysis discovered that phosphorylation of ß-Arrestin1 is crucial for this interaction. Additionally, the novel mechanism of UV-induced EGFR transactivation was extended to squamous cell carcinoma. The mechanism happens in a dose dependent manner and requires a metalloprotease to shed the proligand Amphiregulin. The involvement of both ADAM9 and ADAM17, being the metalloproteases responsible for this cleavage, was shown for SCC9 cells.}, subject = {Epidermaler Wachstumsfaktor-Rezeptor}, language = {en} } @phdthesis{Laisney2010, author = {Laisney, Juliette Agn{\`e}s Genevi{\`e}ve Claire}, title = {Characterisation and regulation of the Egfr/Egfr ligand system in fish models for melanoma}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-51369}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2010}, abstract = {Fish of the genus Xiphophorus belong to the oldest animal models in cancer research. The oncogene responsible for the generation of spontaneous aggressive melanoma encodes for a mutated epidermal growth factor receptor (Egfr) and is called xmrk for Xiphophorus melanoma receptor kinase. Xmrk constitutive activation mechanisms and subsequent signaling pathways have already been investigated and charaterized but it is still unknown if Egfr ligands may also play a role in Xmrk-driven melanoma formation. To investigate the potential role of Egfr ligands in Xmrk-driven melanoma, I firstly analyzed the evolution of teleost and tetrapod Egfr/Egfr ligand systems. I especially focused on the analysis on the medaka fish, a closely related species to Xiphophorus, for which the whole genome has been sequenced. I could identify all seven Egfr ligands in medaka and could show that the two teleost-specific Egfr copies of medaka display dissimilar expression patterns in adult tissues together with differential expression of Egfr ligand subsets, arguing for subfunctionalization of receptor functions in this fish. Our phylogenetic and synteny analyses supported the hypothesis that only one gene in the chordate ancestor gave rise to the diversity of Egfr ligands found in vertebrate genomes today. I also could show that the Egfr extracellular subdomains implicated in ligand binding are not evolutionary conserved between tetrapods and teleosts, making the use of heterologous ligands in experiments with fish cells debatable. Despite its well understood and straight-forward process, Xmrk-driven melanomagenesis in Xiphophorus is problematic to further investigate in vivo. Our laboratory recently established a new melanoma animal model by generating transgenic mitf::xmrk medaka fishes, a Xiphophorus closely related species offering many more advantages. These fishes express xmrk under the control of the pigment-cell specific Mitf promoter. During my PhD thesis, I participated in the molecular analysis of the stably transgenic medaka and could show that the Xmrk-induced signaling pathways are similar when comparing Xiphophorus with transgenic mitf::xmrk medaka. These data together with additional RNA expression, protein, and histology analyses showed that Xmrk expression under the control of a pigment cell-specific promoter is sufficient to induce melanoma in the transgenic medaka, which develop very stereotyped tumors, including uveal and extracutaneous melanoma, with early onset during larval stages. To further investigate the potential role of Egfr ligands in Xmrk-driven melanoma, I made use of two model systems. One of them was the above mentioned mitf::xmrk medaka, the other was an in-vitro cell culture system, where the EGF-inducible Xmrk chimera HERmrk is stably expressed in murine melanocytes. Here I could show that HERmrk activation strongly induced expression of amphiregulin (Areg) and heparin-binding EGF-like growth factor (Hbegf) in melanocytes. This regulation was dependent on the MAPK and SRC signaling pathways. Moreover, upregulation of Adam10 and Adam17, the two major sheddases of Egfr ligands, was observed. I also could demonstrate the functionality of the growth factors by invitro analyses. Using the mitf::xmrk medaka model I could also show the upregulation of a subset of ligand genes, namely egf, areg, betacellulin (btc) and epigen (epgn) as well as upregulation of medaka egfrb in tumors from fish with metastatic melanoma. All these results converge to support an Xmrk-induced autocrine Egfr ligand loop. Interestingly, my in-vitro experiments with conditioned supernatant from medaka Egf- and Hbegf-producing cells revealed that not only Xiphophorus Egfrb, but also the pre-activated Xmrk could be further stimulated by the ligands. Altogether, I could show with in-vitro and in-vivo experiments that Xmrk is capable of inducing a functional autocrine Egfr ligand loop. These data confirm the importance of autocrine loops in receptor tyrosine kinase (RTK)-dependent cancer development and show the possibility for a constitutively active RTK to strengthen its oncogenic signaling by ligand binding.}, subject = {Schwertk{\"a}rpfling}, language = {en} } @phdthesis{Huenten2005, author = {H{\"u}nten, Peter}, title = {Channel-forming proteins in the cell wall of amino acid-producing Corynebacteria}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-13890}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2005}, abstract = {Corynebacterium glutamicum is together with C. callunae and C. efficiens a member of the diverse group of mycolic-acid containing actinomycetes, the mycolata. These bacteria are potent producer of glutamate, lysine and other amino acids on industrial scale. The cell walls of most actinomycetes contain besides an arabinogalactan-peptidoglycan complex large amounts of mycolic acids. This three-layer envelope is called MAP (mycolyl-arabinogalactan-peptidoglycan) complex and it represents a second permeability barrier beside the cytoplasmic membrane similar to the outer membrane of Gram-negative bacteria. In analogy to the situation in the outer membrane of Gram-negative bacteria, channels are present in the mycolic acid layer of the mycobacterial cell wall for the passage of hydrophilic solutes. Molecular studies have provided far-reaching findings on the amino acid flux and its balance in C. glutamicum in general, but the L-glutamate export still remains unknown. The properties of the outer layers, typical of mycolata, seem to be of major importance in this process, and diffusion seems to play a key role for this part of the cell wall. The major aim of this thesis was to identify and study novel channel-forming proteins of the amino acid producers C. glutamicum, C. callunae and C. efficiens. Cell wall extracts of the organisms were investigated and a novel pore-forming protein, named PorH, that is homologue in all three organisms, was detected and characterized. PorHC.glut was isolated from C. glutamicum cells cultivated in minimal medium. The protein was identified in lipid bilayer experiments and purified to homogeneity by fast-protein liquid chromatography across a HiTrap-Q column. The purified protein forms cation-selective channels with a diameter of about 2.2 nm and an average single-channel conductance of about 2.5 nS in 1 M KCl in the lipid bilayer assay. Organic solvent extracts were used to study the permeability properties of the cell wall of C. callunae and C.efficiens. The cell extracts contained channel-forming activity, the corresponding proteins were purified to homogeneity by fast-protein liquid chromatography across a HiTrap-Q column and named PorHC.call and PorHC.eff. Channels formed by PorHC.call are cation-selective with a diameter of about 2.2 nm and an average single-channel conductance of 3 nS, whereas PorHC.eff forms slightly anion selective channels with an average single-channel conductance of 2.3 nS in 1 M KCl in the lipid bilayer assay. The PorH proteins were partially sequenced and the corresponding genes, which were designated as porH, were identified in the published genome sequence of C. glutamicum and C. efficiens. The chromosome of C. callunae is not sequenced, but PorHC.call shows a high homology to PorHC.eff and PorHC.glut. The proteins have no N-terminal extension, only the inducer methionine, which suggests that secretion of the proteins could be very similar to that of PorAC.glut of C. glutamicum. PorHC.glut is coded in the bacterial chromosome by a gene that is localized in the vincinity of the porAC.glut gene, within a putative operon formed by 13 genes that are encoded by the minus strand. Both porins are cotranscribed and coexist in the cell wall, which was demonstrated in RT-PCR and immunological detection experiments. The arrangement of porHC.glut and porAC.glut on the chromosome is similar to that of porBC.glut and porCC.glut and it was found that PorAC.glut, PorHC.glut, PorBC.glut and PorCC.glut coexist in the cell wall of C. glutamicum. The molecular mass of about 6 kDa of the PorH channel forming proteins is rather small and suggests that the cell wall channels are formed by oligomers. A possibly hexameric form was demonstrated for PorHC.glut in Western blot analysis with anti- PorHC.glut antibodies. Secondary structure predictions for PorHC.glut, PorHC.call and PorHC.eff predict that a stretch of about 42 amino acids of PorHC.glut and 28 amino acids of PorHC.call and PorHC.eff forms amphipathic \&\#61537;-helices with a total length of 6.3 nm and 4.2 nm respectively. This should be sufficient to cross the mycolic acid layer. Another objective of this work was to establish an heterologous expression system for corynebacterial channel-forming proteins, to investigate the channel-forming properties of the up to now only hypothetical porins PorA, PorB, PorC from C. efficiens and PorC from C. glutamicum. We could demonstrate with recombinant expression experiments in E. coli that porBC.eff and porCC.eff encode for channel-forming proteins. They are, like PorBC.glut, anion-selective with a similar single-channel conductance of 1 nS in 1 M KCl.}, subject = {Corynebacterium callunae}, language = {en} } @phdthesis{Kronhardt2012, author = {Kronhardt, Angelika}, title = {Channel Formation, Binding and Translocation Properties of Anthrax, CDT and Related Toxins of the AB7 type}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-71559}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2012}, abstract = {The ability to produce toxins is spread among a huge variety of bacterial strains. A very prominent class of bacterial protein toxins is the family of binary AB toxins sharing a common mode of intoxication. A pore forming component B binds and translocates an enzymatic component A into the cytosol of target cells exhibiting a fatal mode of action. These components are supposed to be not toxic themselves but both required for cell toxicity. Anthrax toxin produced by the Gram-positive bacteria Bacillus anthracis is the best studied binary toxin especially since its use as a biological weapon in the context of the attacks of 9/11 in 2001. In contrast to other binary toxins, Anthrax toxin possesses two different enzymatic components, edema factor (EF), a calcium- and calmodulin-dependent adenylat-cyclase and lethal factor (LF), a zinc-dependent metalloprotease. Protective antigen (PA) is the pore-forming component responsible for binding and translocation. Clostridium botulinum possesses in addition to the well known botulinum toxin (Botox) a variety of other toxins, such as the binary C2 toxin. C2 toxin is composed of the binding and translocation moiety C2II and the enzymatic moiety C2I acting as an actin-ADP-ribosyltransferase. In this study, the mode of translocation and the binding kinetics to the enzymatic component were studied in a biophysical experimental setup. In chapter 2, the binding of the N-terminal fractions EFN and LFN to the PA channel are analyzed in artificial bilayer membranes revealing lower binding affinity compared to full-length EF and LF. Other biophysical properties like voltage-dependency and ionic-strength dependency are not influenced. The results suggest that additional forces are involved in the binding process, than those concerning the N-terminus exclusively, as it was supposed previously. As the treatment of an Anthrax infection with antibiotics is often medicated very late due to the lack of early symptoms, tools to prevent intoxication are required. 4-aminoquinolones like chloroquine are known to block the PA channel, thereby inhibiting intoxication but they also lead to severe side-effects. In chapter 3 new promising agents are described that bind to PA in artificial bilayer systems, elucidating common motives and features which are necessary for binding to PA in general. The possible interaction of Anthrax and C2 toxin is investigated by measuring the binding of one enzymatic component to the respective other toxin's pore (chapter 4). Interestingly, in vitro experiments using the black lipid bilayer assay show that PA is able to bind to C2I resulting in half saturation constants in the nanomolar range. Furthermore, in vivo this combination of toxin components exhibits cell toxicity in human cell lines. This is first-time evidence that a heterologous toxin combination is functional in in vitro and in vivo systems. In contrast, C2II is able to bind to EF as well as to LF in vitro, whereas in in vivo studies almost no toxic effect is detected. In the case of PA, an N-terminal His6-tag attached to the enzymatic subunit increased the binding affinity (chapter 5). A His6-tag attached to not related proteins also led to high binding affinities, providing the possibility to establish PA as a general cargo protein. In chapter 6 a set of different molecules and proteins is summarized, which are either related or not related to binary toxins, PA is able to bind. In first line, the presence of positive charges is found to be responsible for binding to PA which is in accordance to the fact that PA is highly cation selective. Furthermore, we present evidence that different cationic electrolytes serve as a binding partner to the PA channel. In the last decade another toxin has aroused public attention as it was found to be responsible for a rising number of nosocomial infections: Clostridium difficile CDT toxin. The mode of action of the enzymatic subunit CDTa is similar to C2I of C2 toxin, acting as an ADP-ribosylating toxin. The channel forming and binding properties of CDT toxin are studied in artificial bilayer membranes (chapter 7). We found that two different types of channels are formed by the B component CDTb. The first channel is similar to that of iota toxin's Ib of Clostridium perfringens with comparable single channel conductance, selectivity and binding properties to the enzymatic subunit CDTa. The formation of this type of channel is cholesterol-dependent, whereas in the absence of cholesterol another kind of channel is observed. This channel has a single channel conductance which is rather high compared to all other binary toxin channels known so far, it is anion selective and does not show any binding affinity to the enzymatic component CDTa. The results reveal completely new insights in channel formation properties and the flexibility of a pore-forming component. Additionally, these findings suggest further possibilities of toxicity of the pore forming component itself which is not known for any other binary toxin yet. Therefore, the pathogenic role of this feature has to be studied in detail.}, subject = {Bacillus anthracis}, language = {en} } @phdthesis{FetivaMora2023, author = {Fetiva Mora, Maria Camila}, title = {Changes in chromatin accessibility by oncogenic YAP and its relevance for regulation of cell cycle gene expression and cell migration}, doi = {10.25972/OPUS-30291}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-302910}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2023}, abstract = {Various types of cancer involve aberrant cell cycle regulation. Among the pathways responsible for tumor growth, the YAP oncogene, a key downstream effector of the Hippo pathway, is responsible for oncogenic processes including cell proliferation, and metastasis by controlling the expression of cell cycle genes. In turn, the MMB multiprotein complex (which is formed when B-MYB binds to the MuvB core) is a master regulator of mitotic gene expression, which has also been associated with cancer. Previously, our laboratory identified a novel crosstalk between the MMB-complex and YAP. By binding to enhancers of MMB target genes and promoting B-MYB binding to promoters, YAP and MMB co-regulate a set of mitotic and cytokinetic target genes which promote cell proliferation. This doctoral thesis addresses the mechanisms of YAP and MMB mediated transcription, and it characterizes the role of YAP regulated enhancers in transcription of cell cycle genes. The results reported in this thesis indicate that expression of constitutively active, oncogenic YAP5SA leads to widespread changes in chromatin accessibility in untransformed human MCF10A cells. ATAC-seq identified that newly accessible and active regions include YAP-bound enhancers, while the MMB-bound promoters were found to be already accessible and remain open during YAP induction. By means of CRISPR-interference (CRISPRi) and chromatin immuniprecipitation (ChIP), we identified a role of YAP-bound enhancers in recruitment of CDK7 to MMB-regulated promoters and in RNA Pol II driven transcriptional initiation and elongation of G2/M genes. Moreover, by interfering with the YAP-B-MYB protein interaction, we can show that binding of YAP to B-MYB is also critical for the initiation of transcription at MMB-regulated genes. Unexpectedly, overexpression of YAP5SA also leads to less accessible chromatin regions or chromatin closing. Motif analysis revealed that the newly closed regions contain binding motifs for the p53 family of transcription factors. Interestingly, chromatin closing by YAP is linked to the reduced expression and loss of chromatin-binding of the p53 family member Np63. Furthermore, I demonstrate that downregulation of Np63 following expression of YAP is a key step in driving cellular migration. Together, the findings of this thesis provide insights into the role of YAP in the chromatin changes that contribute to the oncogenic activities of YAP. The overexpression of YAP5SA not only leads to the opening of chromatin at YAP-bound enhancers which together with the MMB complex stimulate the expression of G2/M genes, but also promotes the closing of chromatin at ∆Np63 -bound regions in order to lead to cell migration.}, subject = {Chromatin}, language = {en} } @phdthesis{Solger2021, author = {Solger, Franziska}, title = {Central role of sphingolipids on the intracellular survival of \(Neisseria\) \(gonorrhoeae\) in epithelial cells}, doi = {10.25972/OPUS-24753}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-247534}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2021}, abstract = {Neisseria gonorrhoeae are Gram-negative bacteria with diplococcal shape. As an obligate human pathogen, it is the causative agent of gonorrhoea, a sexually transmitted disease. Gonococci colonize a variety of mucosal tissues, mainly the urogenital tract in men and women. Occasionally N. gonorrhoeae invades the bloodstream, leading to disseminated gonococcal infection. These bacteria possess a repertoire of virulence factors, which expression patterns can be adapted to the environmental conditions of the host. Through the accumulation of antibiotic resistances and in absence of vaccines, some neisserial strains have the potential to spread globally and represent a major public health threat. Therefore, it is necessary to understand the exact molecular mechanisms underlying the successful infection and progression of gonococci within their host. This deeper understanding of neisserial infection and survival mechanisms is needed for the development of new therapeutic agents. In this work, the role of host-cell sphingolipids on the intracellular survival of N. gonorrhoeae was investigated. It was shown that different classes of sphingolipids strongly interact with invasive gonococci in epithelial cells. Therefore, novel and highly specific clickable sphingolipid analogues were applied to study these interactions with this pathogen. The formation of intra- and extracellular sphingosine vesicles, which were able to target gonococci, was observed. This direct interaction led to the uptake and incorporation of sphingosine into the neisserial membrane. Together with in vitro results, sphingosine was identified as a potential bactericidal reagent as part of the host cell defence. By using different classes of sphingolipids and their clickable analogues, essential structural features, which seem to trigger the bacterial uptake, were detected. Furthermore, effects of key enzymes of the sphingolipid signalling pathway were tested in a neutrophil infection model. In conclusion, the combination of click chemistry and infection biology made it possible to shed some light on the dynamic interplay between cellular sphingosine and N. gonorrhoeae. Thereby, a possible "catch-and-kill" mechanism could have been observed.}, subject = {Neisseria gonorrhoeae}, language = {en} } @phdthesis{Boehme2009, author = {B{\"o}hme, Linda}, title = {Cellular response to double-stranded RNA in Chlamydia trachomatis-infected human host cells}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-46474}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2009}, abstract = {Chlamydien sind Gram-negative, obligat-intrazellul{\"a}re Bakterien, die f{\"u}r ein weites Spektrum an relevanten Krankheiten verantwortlich sind. Auf Grund ihres zweiphasigen Entwicklungszyklusses sind Chlamydien von einer intakten Wirtszelle abh{\"a}ngig, um sich erfolgreich vermehren und im Organismus ausbreiten zu k{\"o}nnen. Daher haben Chlamydien anspruchsvolle Strategien entwickelt, um das Immunsystem des Wirtes auszuschalten oder den programmierten Zelltod ihrer Wirtszelle zu verhindern. In der vorliegenden Arbeit wurde untersucht, ob eine Infektion mit C. trachomatis einen Einfluss auf die zellul{\"a}re Antwort auf dsRNA nehmen kann. Die Synthese von dsRNA ist ein charakteristisches Merkmal der Replikation von Viren, welche sowohl die Apoptose induzieren als auch das Immunsystem aktivieren kann. Um eine chlamydiale und virale Co-Infektion zu simulieren, wurden Chlamydien-infizierte Epithelzellen mit der synthetischen dsRNA Polyinosin-Polycytidins{\"a}ure (polyI:C) transfiziert. Im ersten Teil der Arbeit wurde untersucht, ob Chlamydien die durch dsRNA eingeleitete Apoptose verhindern k{\"o}nnen. Eine signifikante Reduktion der dsRNA-induzierten Apoptose konnte in infizierten Zellen beobachtet werden. Es zeigte sich, dass die Prozessierung der Initiator-Caspase-8 in infizierten Zellen unterblieb. Dies war von der fr{\"u}hen bakteriellen Proteinsynthese abh{\"a}ngig und f{\"u}r die dsRNA-vermittelte Apoptose spezifisch, da der durch TNFalpha bewirkte Zelltod nicht auf der Ebene der Caspase-8 verhindert werden konnte. Die Aktivierung von zellul{\"a}ren Faktoren, die bei der Apoptoseinduzierung eine wichtige Rolle spielen, beispielsweise PKR und RNase L, war in infizierten Zellen jedoch unver{\"a}ndert. Stattdessen konnte durch RNA Interferenz-vermittelte Depletion gezeigt werden, dass der zellul{\"a}re Caspase-8-Inhibitor cFlip eine entscheidende Rolle bei der chlamydialen Blockierung der dsRNA-vermittelten Apoptose spielt. Mittels Co-Immunopr{\"a}zipitation konnte ein erster Hinweis darauf gefunden werden, dass C. trachomatis eine Anreicherung von cFlip im dsRNA-induzierten Komplex von Caspase-8 und FADD bewirkt. Im zweiten Teil der Arbeit wurde untersucht, ob Chlamydien die Immunantwort auf virale Infektionen beeinflussen, welche vor allem die Expression von Interferonen und Interleukinen beinhaltet. Es stellte sich heraus, dass die Aktivierung des Interferon regulatory factor 3 (IRF-3) und des zur Familie von NF-kappaB Trankriptionsfaktoren geh{\"o}renden p65, zwei zentralen Regulatoren der Immunantwort auf dsRNA, in infizierten Epithelzellen ver{\"a}ndert war. Die Degradation von IkappaB-alpha, des Inhibitors von NF-kappaB, war in infizierten Zellen beschleunigt, begleitet von einer Ver{\"a}nderung der Translokation des Transkriptionsfaktors in den Zellkern. Im Gegensatz dazu wurde die nukle{\"a}re Translokation von IRF-3 durch die Infektion signifikant verhindert. Die hier vorgestellten Daten zeigen erstmals, dass eine Infektion mit C. trachomatis die zellul{\"a}re Antwort auf dsRNA signifikant ver{\"a}ndern kann und implizieren einen Einfluss von chlamydialen Infektionen auf den Ausgang von viralen Superinfektionen.}, subject = {Chlamydia trachomatis}, language = {en} } @phdthesis{Blume2009, author = {Blume, Constanze}, title = {Cellular functions of VASP phosphorylations}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-48321}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2009}, abstract = {Members of the enabled/vasodilator-stimulated phosphoprotein (Ena/VASP) family are important regulators of the actin cytoskeleton dynamics. VASP functions as well as its interactions with other proteins are regulated by phosphorylation at three sites - serine157 (S157), serine239 (S239), and threonine278 (T278) in humans. cAMP- and cGMP- dependent protein kinases phosphorylate S157 and S239, respectively. In contrast, the kinase responsible for T278 was as yet unknown and identified in the first part of this thesis. In a screen for T278 phosphorylating kinases using a phospho-specific antibody against phosphorylated T278 AMP-activated protein kinase (AMPK) was identified in endothelial cells. Mutants of AMPK with altered kinase-activity modulate T278-phosphorylation levels in cells. AMPK-driven T278-phosphorylation impaired stress fiber formation and changed cell morphology in living cells. AMPK is a fundamental sensor of cellular and whole body energy homeostasis. Zucker Diabetic Fatty (ZDF) rats, which are an animal model for type II diabetes mellitus, were used to analyze the impact of phosphorylated T278 in vivo. AMPK-activity and T278-phosphorylation were substantially reduced in arterial vessel walls of ZDF rats in comparison to control animals. These findings demonstrate that VASP is a new AMPK substrate, that VASP phosphorylation mediates the effects of metabolic regulation on actin cytoskeleton rearrangements, and that this signaling system becomes down-regulated in diabetic vessel disorders in rats. In the second part of this thesis, a functional analysis of differential VASP phosphorylations was performed. To systematically address VASP phosphorylation patterns, a set of VASP phosphomimetic mutants was cloned. These mutants enable the mimicking of defined phosphorylation patterns and the specific analysis of single kinase-mediated phosphorylations. VASP localization to the cell periphery was increased by S157- phosphorylation and modulated by phosphorylation at S239 and T278. Latter phosphorylations synergistically reduced actin polymerization. In contrast, S157- phosphorylation had no effect on actin-dynamics. Taken together, the results of the second part show that phosphorylation of VASP serves as a fine regulator of localization and actin polymerization activity. In summary, this study revealed the functions of VASP phosphorylations and established novel links between signaling pathways and actin cytoskeleton rearrangement.}, subject = {Vasodilatator-stimuliertes Phosphoprotein}, language = {en} } @phdthesis{Reinboth2012, author = {Reinboth, Jennifer}, title = {Cellular Factors Contributing to Host Cell Permissiveness in Support of Oncolytic Vaccinia Virus Replication}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-85392}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2012}, abstract = {In initial experiments, the well characterized VACV strain GLV-1h68 and three wild-type LIVP isolates were utilized to analyze gene expression in a pair of autologous human melanoma cell lines (888-MEL and 1936 MEL) after infection. Microarray analyses, followed by sequential statistical approaches, characterized human genes whose transcription is affected specifically by VACV infection. In accordance with the literature, those genes were involved in broad cellular functions, such as cell death, protein synthesis and folding, as well as DNA replication, recombination, and repair. In parallel to host gene expression, viral gene expression was evaluated with help of customized VACV array platforms to get better insight over the interplay between VACV and its host. Our main focus was to compare host and viral early events, since virus genome replication occurs early after infection. We observed that viral transcripts segregated in a characteristic time-specific pattern, consistent with the three temporal expression classes of VACV genes, including a group of genes which could be classified as early-stage genes. In this work, comparison of VACV early replication and respective early gene transcription led to the identification of seven viral genes whose expression correlated strictly with replication. We considered the early expression of those seven genes to be representative for VACV replication and we therefore referred to them as viral replication indicators (VRIs). To explore the relationship between host cell transcription and viral replication, we correlated viral (VRI) and human early gene expression. Correlation analysis revealed a subset of 114 human transcripts whose early expression tightly correlated with early VRI expression and thus early viral replication. These 114 human molecules represented an involvement in broad cellular functions. We found at least six out of 114 correlates to be involved in protein ubiquitination or proteasomal function. Another molecule of interest was the serine-threonine protein kinase WNK lysine-deficient protein kinase 1 (WNK1). We discovered that WNK1 features differences on several molecular biological levels associated with permissiveness to VACV infection. In addition to that, a set of human genes was identified with possible predictive value for viral replication in an independent dataset. A further objective of this work was to explore baseline molecular biological variances associated with permissiveness which could help identifying cellular components that contribute to the formation of a permissive phenotype. Therefore, in a subsequent approach, we screened a set of 15 melanoma cell lines (15-MEL) regarding their permissiveness to GLV-1h68, evaluated by GFP expression levels, and classified the top four and lowest four cell lines into high and low permissive group, respectively. Baseline gene transcriptional data, comparing low and highly permissive group, suggest that differences between the two groups are at least in part due to variances in global cellular functions, such as cell cycle, cell growth and proliferation, as well as cell death and survival. We also observed differences in the ubiquitination pathway, which is consistent with our previous results and underlines the importance of this pathway in VACV replication and permissiveness. Moreover, baseline microRNA (miRNA) expression between low and highly permissive group was considered to provide valuable information regarding virus-host co-existence. In our data set, we identified six miRNAs that featured varying baseline expression between low and highly permissive group. Finally, copy number variations (CNVs) between low and highly permissive group were evaluated. In this study, when investigating differences in the chromosomal aberration patterns between low and highly permissive group, we observed frequent segmental amplifications within the low permissive group, whereas the same regions were mostly unchanged in the high group. Taken together, our results highlight a probable correlation between viral replication, early gene expression, and the respective host response and thus a possible involvement of human host factors in viral early replication. Furthermore, we revealed the importance of cellular baseline composition for permissiveness to VACV infection on different molecular biological levels, including mRNA expression, miRNA expression, as well as copy number variations. The characterization of human target genes that influence viral replication could help answering the question of host cell response to oncolytic virotherapy and provide important information for the development of novel recombinant vaccinia viruses with improved features to enhance replication rate and hence trigger therapeutic outcome.}, subject = {Vaccinia-Virus}, language = {en} } @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{Herrmann2014, author = {Herrmann, Alexander Michael}, title = {CD8+ Lymphozyten mediierter Angriff auf Neuronen des ZNS: Relevanz von Granzym B und Perforin f{\"u}r akute elektrophysiologische Ver{\"a}nderungen}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-109124}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2014}, abstract = {Zytotoxische CD8+ T-Lymphozyten spielen in vielen inflammatorischen, aber auch prim{\"a}r neurodegenerativen Erkrankungen eine wichtige Rolle. Daher besitzt die Fragestellung inwiefern CD8+ ZTL Neurone direkt sch{\"a}digen und ggf. welche mechanistischen Aspekte dieser Sch{\"a}digung zugrunde liegen, eine hohe Relevanz. Um diese Fragestellung eingehender zu beleuchten, wurde mit dem OT-I-System gearbeitet. Dieses gut vorcharakterisierte CD8+ T-Zell-Modell besitzt den Vorteil, dass diese transgenen Zellen nur eine Peptidsequenz des Ovalbumin (OVA) Protein als spezifisches Antigen erkennen. Zun{\"a}chst wurden in der vorliegenden Arbeit Co-Kultivierungs-Experimente durchgef{\"u}hrt. Hierzu wurden akut isolierte murine Hippokampus-Neurone unter verschiedenen Bedingungen mit OT-I Lymphozyten co-kultiviert. Hierbei konnte gezeigt werden, dass unter Antigenpr{\"a}sentation der Neurone signifikant mehr Neurone in die Apoptose/Nekrose gef{\"u}hrt werden, als unter Kontroll-Bedingungen, in denen entweder kein Antigen oder ein Antigen, das nicht von OT-I Lymphozyten erkannt wird, pr{\"a}sentiert wird. Nachdem die Antigen-abh{\"a}ngigen zytotoxischen Effekte auf Neurone gezeigt werden konnten, wurde mithilfe elektrophysiologischer Techniken die mechanistischen und funktionellen Konsequenzen des direkten neuronalen/OT-I-vermittelten Zellkontakts untersucht. Bei diesem experimentellen Ansatz wurde durch elektrisches Auslenken eines Neurons nach Kontakt mit einem OT-I Lymphozyt die passiven elektrischen Parameter der Neuronenmembran gemessen. In diesen Messungen konnte gezeigt werden, dass nach unmittelbarem Kontakt eines Neurons mit einem OT-I Lymphozyt der neuronale Membranwiderstand reduziert wird bzw. die Leitf{\"a}higkeit der Zellmembran erh{\"o}ht wird. Diese {\"A}nderung der neuronalen Membran-Leitf{\"a}higkeit findet in einem Zeitraum von 10 min nach dem Zell-Zell-Kontakt statt. Auch hier konnte gezeigt werden, dass dieser Einfluss von OT-I Lymphozyten auf Neurone strikt Antigen-abh{\"a}ngig ist. Zur Untersuchung des Mechanismus der OT-I T-Lymphozyten auf Neurone wurde das Augenmerk auf verschiedene T-Zell-induzierte Apoptosewegegelegt. Es konnte gezeigt werden, dass durch Blockieren der Fas/FasL-Interaktion mittels eines Antik{\"o}rpers kein Unterschied, weder in der neuronalen Apoptoserate nach Co-Kultivierung, noch eine {\"A}nderung der passiven neuronalen Membran-Leitf{\"a}higkeit auftritt. Weiterhin wurde die Rolle der von T-Zellen sezernierten Granula Perforin und Granzym B untersucht. Um den Einfluss dieser Granula aufzukl{\"a}ren, wurden OT-I Lymphozyten verwendet, die entweder defizient f{\"u}r Perforin oder Granzym B waren. In diesem experimentellen Ansatz wurde gezeigt, dass ausschließlich Perforin f{\"u}r die Erniedrigung des passiven neuronalen Membran-Widerstandes verantwortlich ist. Diese Erh{\"o}hung der neuronalen Membranleitf{\"a}higkeit f{\"u}hrte aber nicht direkt zum neuronalen Zelltod. Vielmehr wurde durch die einhergehende Depolarisation des Neurons die elektrische Aktivit{\"a}t der Zelle vermindert, sodass es zu einem sogenannten „electrical silencing" kommt. Dieser Umstand konnte auch in der Betrachtung der spontanen Netzwerkaktivit{\"a}t von Neuronenkulturen gezeigt werden. Hierf{\"u}r wurden hoch dichte Neuronenkulturen auf MEA-Chips kultiviert. Mit Hilfe dieser MEA konnten die Summenfeldpotentiale der Neuronenkulturen detektiert werden. Hierbei wurde beobachtet, dass nach Beladung der Neuronen mit dem spezifischen OT-I-Antigen und OT-I Zellen eine Verringerung der spontanen Netzwerkaktivit{\"a}t einhergeht. Auch in diesem Effekt konnte eine Antigen-Spezifit{\"a}t nachgewiesen werden. Da der Prozess der zellul{\"a}ren Apoptose mit einem Anstieg der intrazellul{\"a}ren Ca2+-Konzentration einhergeht, und Perforin als Ca2+-durchl{\"a}ssiger unselektiver Porenbildner fungiert, wurden zur {\"U}berpr{\"u}fung der Hypothese calcium imaging-Experimente durchgef{\"u}hrt. Analog zu den elektrophysiologischen Messungen wurde gezeigt, dass nach direktem Zell-Zell-Kontakt zwischen Neuron und OT-I Lymphozyt eine Erh{\"o}hung der intrazellul{\"a}ren Ca2+-Konzentration zu messen ist. Dass diese {\"A}nderung des neuronalen Ca2+-Einstroms durch Perforin-abh{\"a}ngige Membranporen hervorgerufen wird, konnte durch die Verwendung von Perforin-defizienten OT-I Lymphozyten bewiesen werden. Unter Verwendung von Perforin-defizienten OT-I Lymphozyten wurde keine {\"A}nderung der neuronalen Ca2+-Konzentration ermittelt. Weiterhin wurde in diesem experimentellen Ansatz gezeigt, dass auch der OT-I-vermittelte neuronale Ca2+-Anstieg strikt Antigen-abh{\"a}ngig ist.Zusammengefasst konnte in dieser Arbeit gezeigt werden, dass MHC-I/Antigen-vermittelte CD8+ Lymphozyten-Interaktion mit einem Neuron zu „electrical silencing" des Neurons f{\"u}hrt. Dieser Prozess ist klar Perforin-abh{\"a}ngig, f{\"u}hrt jedoch nicht zum unmittelbaren Zelltod des Neurons.}, subject = {Antigen CD8}, language = {de} } @phdthesis{Kibler2002, author = {Kibler, Eike Mathias U.}, title = {Casein-Kinase-2-Beta und neuronale Entwicklungsprozesse}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-4202}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2002}, abstract = {Die Pilzk{\"o}rper von Drosophila melanogaster stellen eine f{\"u}r die Lebensf{\"a}higkeit dieses Organismus entbehrliche Gehirnstruktur dar. Die Entwicklungsprozesse, die der Bildung dieser zentralnerv{\"o}sen Struktur zugrunde liegen, sind gut erforscht. Die neuronalen Stammzellen, die f{\"u}r die Bildung dieser Gehirnstruktur verantwortlich sind, sind identifiziert und experimentell gut zug{\"a}nglich. Daher bietet sich die Drosophila-Pilzk{\"o}rperentwicklung als neurogenetisches Modellsystem an, grundlegende Mechanismen der Gehirnentwicklung durch die Untersuchung von Pilzk{\"o}rperstrukturmutanten zu erforschen. In dieser Arbeit wurde mushroom bodies undersized P1 (mbuP1) als eine durch Transposon- Insertion in den Casein-Kinase-2ß-Genlokus verursachte, hypomorphe Mutation identifiziert, die zu einer starken Verringerung der Anzahl der die Pilzk{\"o}rper bildenden intrinsischen Neurone f{\"u}hrt. Eine Reversion des mbuP1-Pilzk{\"o}rperph{\"a}notyps konnte unter anderem durch die Expression von Casein-Kinase-2ß-(CK2ß)-Transgenen im mbuP1-Hintergrund erzielt werden. Durch Rekombination wurde ein fertiler mbuP1-Stamm etabliert, der nun die Untersuchung der zellul{\"a}ren mbuP1-Defekte erm{\"o}glicht. Eine partielle, letale Deletion der CK2ß-Transkriptionseinheit wurde erzeugt. Die Letalit{\"a}t dieser Deletion konnte sowohl durch ein genomisches CK2ß-Transgen als auch durch die ubiquit{\"a}re Expression einer CK2ß-cDNA gerettet, und hierdurch die essentielle Funktion der CK2ß-Transkriptionseinheit in Drosophila belegt werden. Durch die ubiquit{\"a}re Expression von in vitro-mutagenisierten CK2ß-cDNAs im CK2ß-Letalhintergrund wurde gezeigt, daß die Phosphorylierung der regulatorischen CK2ß-Untereinheit durch die katalytisch aktive CK2\&\#945;-Untereinheit kein lebensnotwendiger Prozess ist. Gleichartige Experimente wurden zur Untersuchung der funktionellen Bedeutung eines CK2ß-Zinkfingermotivs und eines CK2ß-Destruction-Box-Motivs durchgef{\"u}hrt. Diese legen nahe, daß das Zinkfingermotiv im Gegensatz zum Destruction-Box-Motiv f{\"u}r die in vivo-Funktion der CK2ß-Untereinheit essentiell ist. Expression der in vitro-mutagenisierten CK2ß-cDNAs im mbuP1-Hintergrund werden die funktionelle Bedeutung der ausgetauschten Aminos{\"a}uren f{\"u}r die Pilzk{\"o}rperentwicklung zeigen. Eine letale genetische Interaktion von mbuP1 mit einer Mutation des Drosophila-MAP-Kinase-Gens rolled (rlSem) und eine lebensf{\"a}hige Interaktion von mbuP1 mit einer Mutation des Drosophila-S6-Kinase-p90rsk-Gens ignorant (ignP1), bei der Fl{\"u}gel- und Augenent-wicklungsdefekte zu beobachten sind, wurden gefunden. Es wurde zudem gezeigt, daß rlSem als Suppressor des Pilzk{\"o}rperph{\"a}notyps eines schw{\"a}cheren mbu-Allels wirkt. Hierdurch konnte eine Beteiligung der Casein-Kinase-2 an MAP-Kinase-Signal{\"u}bertragungswegen wahrscheinlich gemacht werden.}, subject = {Taufliege}, language = {de} } @phdthesis{BollazziSosa2008, author = {Bollazzi Sosa, Leonardo Martin}, title = {Building behaviour and the control of nest climate in Acromyrmex leaf-cutting ants}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-27610}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2008}, abstract = {This work was aimed at experimentally studying whether climatic variables act as environmental cues for workers' building behaviour in leaf-cutting ants of the genus Acromyrmex, and to what extent building responses account for the maintenance of nest climate in a proper range for the inhabiting colony. Specifically, this work presents independent analysis in different Acromyrmex species with disparate ecology and nesting habits, aimed at understanding to what extent: i) temperature and humidity act as cues for workers' building behaviour, ii) inter- and intraspecific differences in the nesting habits observed in South American Acromyrmex are based on distinct building behaviours and on the variation in regional climate across continent, iii) differences in nest architecture account for the maintenance of nest climate in a proper range for colony members and, iv) climatic variables trigger building responses aimed at controlling short-term changes in nest climate. It is first experimentally shown that soil temperature acts as a cue for workers' digging behaviour. Acromyrmex lundi workers were observed to respond to both soil temperature as well as its changes, and to decide accordingly where to start or whether to stop digging. The soil temperature range preferred by workers to dig, between 20°C and maximally 30.6°C, matches the range at which colony growth is expected to be maximized. Temperature-sensitive digging might therefore lead to the establishment of the fungus chambers in soil layers with a proper range of temperatures for colony growth. Based on that, it was hypothesized that nest depth in Acromyrmex largely depends on the depth at which this temperature range is located across the soil profile, i.e., the higher the temperature in the superficial soil layers, the deeper the nest location, since soil temperature decreases with increasing depth. A bibliographic survey on nesting habits of 21 South American Acromyrmex species confirmed that the warmer the soil temperature at 50 cm depth throughout the South American continent, the higher the number of species presenting subterranean nests, compared with those inhabiting superficial nests. Temperature-sensitive digging in Acromyrmex would therefore explain the geographical distribution of nesting habits observed for this genus in the South American continent, i.e., subterranean in the northern tropical regions, and superficial in the southern temperate ones. In addition, results showed that Acromyrmex colonies from temperate regions indeed achieve thermoregulatory benefits through the determination of nest depth based on thermoregulatory needs. In sympatrically-occurring colonies of the grass-cutting ant A. heyeri, temperature inside superficial thatched nests was higher, and more suitable for colony growth, than that inside subterranean nests. This temperature surplus was even higher in spring, at the time of production of sexual brood, than in winter or summer. It was demonstrated that such temperature surplus was brought about by the low thermal diffusivity of the nest thatch, which prevents diurnal nest overheating by the incoming solar radiation, and avoids losses of the accumulated daily heat into the cold air during night, thus leading to high average nest temperatures. Although highly advantageous for colonies in terms of nest temperature, the determination of nest depth based on thermoregulatory needs may differentially affect nest ventilation and humidity depending on how nest exposition influences the exchange of nest air with the outside air. For instance, colonies with a superficial nesting habit might benefit from improved nest ventilation, but be at risk of desiccation due to their exposition and the consequent humidity losses into the dry outside air. Results demonstrated that in two Acromyrmex species, short-term regulatory building responses triggered and spatially organized by climatic variables occur, and may counteract undesired changes in internal nest humidity. Workers of the thatching grass-cutting ant A. heyeri, for instance, closed a number of nest-thatch openings as a response to desiccation of the outside air, even at a nest temperature that otherwise triggered the response of opening them so as to reduce nest temperature. In the leaf-cutting ant A. ambiguus, the direction of the airflow inside nest tunnels was shown to act as a cue for spatially guiding the building behaviour of plugging nest entrances. However, workers only responded if the humidity content of the circulating air was low, trading therefore nest ventilation for humidity maintenance.}, subject = {Verhaltens{\"o}kologie}, language = {en} } @phdthesis{Halboth2018, author = {Halboth, Florian}, title = {Building behavior and nest climate control in leaf-cutting ants: How environmental cues affect the building responses of workers of \(Atta\) \(vollenweideri\)}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-161701}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2018}, abstract = {The present work investigates the influence of environmental stimuli on the building behavior of workers of the leaf-cutting ant Atta vollenweideri. It focuses on cues related to the airflow-driven ventilation of their giant underground nests, i.e., air movements and their direction, carbon dioxide concentrations and humidity levels of the nest air. First, it is shown that workers are able to use airflow and its direction as learned orientation cue by performing learning experiments with individual foragers using a classical conditioning paradigm. This ability is expected to allow workers to also navigate inside the nest tunnels using the prevailing airflow directions for orientation, for example during tasks related to nest construction and climate control. Furthermore, the influence of carbon dioxide on the digging behavior of workers is investigated. While elevated CO2 levels hardly affect the digging rate of the ants, workers prefer to excavate at locations with lower concentrations and avoid higher CO2 levels when given a choice. Under natural conditions, shifting their digging activity to soil layers containing lower carbon dioxide levels might help colonies to excavate new or to broaden existing nest openings, if the CO2 concentration in the underground rises. It is also shown that workers preferably transport excavated soil along tunnels containing high CO2 concentrations, when carbon dioxide levels in the underground are elevated as well. In addition, workers prefer to carry soil pellets along outflow tunnels instead of inflow tunnels, at least for high humidity levels of the air. The material transported along tunnels providing outflow of CO2-rich air might be used by workers for the construction of ventilation turrets on top of the nest mound, which is expected to promote the wind-induced ventilation and the removal of carbon dioxide from the underground. The climatic conditions inside the nest tunnels also influence the structural features of the turrets constructed by workers on top the nest. While airflow and humidity have no effect on turret structure, outflow of CO2-rich air from the nest causes workers to construct turrets with additional openings and increased aperture, potentially enhancing the airflow-driven gas exchanges within the nest. Finally, the effect of airflow and ventilation turrets on the gas exchanges in Atta vollenweideri nests is tested experimentally on a physical model of a small nest consisting of a single chamber and two nest tunnels. The carbon dioxide clearance rate from the underground was measured depending on both the presence of airflow in the nest and the structural features of the built turrets. Carbon dioxide is removed faster from the physical nest model when air moves through the nest, confirming the contribution of wind-induced flow inside the nest tunnels to the ventilation of Atta vollenweideri nests. In addition, turrets placed on top of one of the tunnel openings of the nest further enhance the CO2 clearance rate and the effect is positively correlated with turret aperture. Taken together, climatic variables like airflow, carbon dioxide and humidity levels strongly affect the building responses of Atta vollenweideri leaf-cutting ants. Workers use these environmental stimuli as orientation cue in the nest during tasks related to excavation, soil transport and turret construction. Although the effects of these building responses on the microclimatic conditions inside the nest remain elusive so far, the described behaviors are expected to allow ant colonies to restore and maintain a proper nest climate in the underground.}, subject = {Verhalten}, language = {en} } @phdthesis{Stegmann2000, author = {Stegmann, Ulrich E.}, title = {Brutpflege, Lebensgeschichte und Taxonomie s{\"u}dostasiatischer Membraciden (Insecta: Homoptera)}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-2365}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2000}, abstract = {Diese Arbeit untersucht die systematische Verbreitung der Brutpflege bei s{\"u}dostasiatischen Buckelzirpen (Homoptera: Membracidae) sowie verhaltens{\"o}kologische Aspekte dieses Verhaltens bei Pyrgauchenia tristaniopsis. Erg{\"a}nzend dazu wurden Aspekte der Taxonomie, Lebensgeschichte, Reproduktionsbiologie und Morphometrie dieser Art untersucht, deren Kenntnis f{\"u}r die Interpretation des Brutpflegeverhaltens erforderlich waren. Die Ergebnisse (1) widersprechen der starken Version der Semelparitie-Hypothese (ein Fortpflanzungsereignis pro Fortpflanzungsperiode als Voraussetzung f{\"u}r Brutpflege bei Insekten), und sie zeigen, dass (2) Brutpflege bei altweltlichen Centrotinae - entgegen fr{\"u}herer Vermutungen - keine Ausnahme ist. Außerdem konnten erstmals einige grundlegende Aspekte der Biologie eines s{\"u}dostasiatischen Vertreters der Familie Membracidae gekl{\"a}rt werden. Aufsammlungen in der bodennahen Vegetation wurden in 16 Untersuchungsgebieten in West-Malaysia und Sabah (Borneo) von 1996-1998 durchgef{\"u}hrt. Weibliche Brutf{\"u}rsorge in Form von Gelegebewachung wurde bei 11 Arten aus folgenden Gattungen gefunden: Pyrgauchenia, Pyrgonota, Hybandoides, Gigantorhabdus (Hypsaucheniini), Centrochares (Centrocharesini), Ebhul (Ebhuloidesini). Larven dieser Arten lebten in Aggregationen zusammen. Drei Arten werden neu beschrieben (Pyrgauchenia biuni, P. pendleburyi, P. tristaniopsis). Zwei nominelle Arten (P. angulata Funkhouser und P. brunnea Funkhouser) sind Junior-Synonyme von P. colorata Distant. Die Arbeiten zu Pyrgauchenia tristaniopsis fanden im unteren Montanregenwald des Kinabalu Nationalparks (Borneo) statt. Diese Art wurde nur dort gefunden (zwischen 1350 m und 1650 m {\"u}. NN), und sie war polyphag (alle Entwicklungsstadien auf 11 Pflanzenarten aus 8 Familien). Es gab f{\"u}nf Larvenstadien, deren Entwicklungszeit zusammen 63-83 Tage betrug (Embryonalentwicklung: 22 Tage). Larven lebten aggregierend und wurden von Ameisen besucht (insgesamt 4 Morphospecies). Es gab Hinweise, dass frisch geh{\"a}utete Imagines noch etwa 10 Tage in der Aggregation verblieben. Sp{\"a}testens 5 bzw. 10 Tage nach der Imaginalh{\"a}utung waren Weibchen bzw. M{\"a}nnchen zu einer Erstkopulation bereit. Bei der Paarung kletterte das M{\"a}nnchen nach der Kontaktaufnahme auf das Weibchen und blieb dort im Median 138 Sekunden sitzen (Pr{\"a}kopula), worauf eine im Median 116-min{\"u}tige Kopulation folgen konnte. W{\"a}hrend der Pr{\"a}kopula sandte das M{\"a}nnchen Vibrationssignale aus. Die Art war promiskuitiv, und manche Weibchen paarten sich w{\"a}hrend der Gelegebewachung. Das Geschlechterverh{\"a}ltnis war zum Zeitpunkt der Imaginalh{\"a}utung ausgeglichen. Die Eimortalit{\"a}t aufgrund einer Kohortenanalyse betrug 35 Prozent. Pr{\"a}datoren der Larven und Imagines waren besonders Springspinnen (Salticidae). Die Eier wurden von Brachygrammatella sp. (Trichogrammatidae) parasitiert. Eier wurden als Gelege ins Gewebe von Wirtspflanzenzweigen gelegt (Unterseite). Die Anzahl Eier pro Gelege (etwa 57) nahm mit der Bewachungsdauer des Weibchens zu. Bevorzugungen von Gelegepositionen ober- oder unterhalb bereits vorhandener Gelege waren nicht festzustellen. Im Median wurden 3-4 (1998er, 1997er Zensus) Gelege zusammen auf einem Zweig gefunden. Bei einem Wiederfangversuch legte mindestens die H{\"a}lfte aller Weibchen w{\"a}hrend ihres Lebens mindestens zwei Gelege. Zwischen Verlassen des ersten Geleges (auf dem ein Weibchen gefunden wurde) und der Oviposition ihres Folgegeleges vergingen im Median 5 Tage. Folgegelege wurden meist auf derselben Wirtspflanze wie das erste Gelege abgelegt. Der Fettk{\"o}rper vergr{\"o}ßerte sich wieder nach der Oviposition, aber noch w{\"a}hrend der Bewachung des aktuellen Geleges. Weibchen saßen 26-28 Tage lang (nach Beginn der Oviposition) auf ihrem Gelege, d.h. bis zum 5.-8. Tag nach Schlupfbeginn der Larven (die Larven schl{\"u}pften sukzessiv, erst 9 Tage nach Schlupfbeginn waren die meisten LI geschl{\"u}pft). Weibchen kehrten nach experimenteller Vertreibung vom Gelege auf dieses zur{\"u}ck. In Wahlversuchen wurde aber das eigene Gelege gegen{\"u}ber einem fremden nicht pr{\"a}feriert. Weibchen wichen bei St{\"o}rungen stets zur Seite aus und begannen ihre Suche immer mit Seitw{\"a}rtsbewegungen. Experimentell herbeigef{\"u}hrter Kontakt mit dem Eiparasitoid Brachygrammatella sp. gen{\"u}gte, um die Beinabwehr bewachender Weibchen zu erh{\"o}hen. Die H{\"a}ufigkeit von Beinbewegungen war nicht nur vom Vorhandensein eines Geleges, sondern auch von der Tageszeit abh{\"a}ngig. Gelegebewachung f{\"o}rderte das {\"U}berleben der Eier: Die Eimortalit{\"a}t stieg mit experimenteller Verk{\"u}rzung der weiblichen Bewachungsdauer an (unabh{\"a}ngig von der Gelegegr{\"o}ße). Gelegebewachung verz{\"o}gerte die Ablage von Folgegelegen, wie durch experimentelles Verk{\"u}rzen der Bewachungsdauer aktuell bewachter Gelege gezeigt wurde. Abgebrochene pronotale Dorsaldornen minderten nicht die Paarungswahrscheinlichkeit: Die H{\"a}ufigkeit kopulierender M{\"a}nnchen und Weibchen mit abgebrochenem Dorn wich nicht von ihrer jeweiligen H{\"a}ufigkeit in der Population ab. Bei 52 Prozent aller Gelege bewachenden Weibchen war der Dorsaldorn abgebrochen. Weibchen waren l{\"a}nger und schwerer als M{\"a}nnchen, und einige pronotale Merkmale (z.B. der Caudaldorn) waren ebenfalls bei den Weibchen l{\"a}nger. Dorsaldorn und Distallobus waren dagegen bei M{\"a}nnchen l{\"a}nger, und zwar bei gleicher K{\"o}rpergr{\"o}ße. Geschwister {\"a}hnelten sich besonders hinsichtlich Gewicht sowie K{\"o}rper- und Dorsaldornl{\"a}nge, was durch große Heritabilit{\"a}t, gleiche Umweltbedingungen und Inzucht erkl{\"a}rt werden k{\"o}nnte.}, subject = {S{\"u}dostasien}, language = {de} } @phdthesis{Muellner2004, author = {M{\"u}llner, Antje}, title = {Breeding ecology and related life-history traits of the hoatzin, Opisthocomus hoazin, in a primary rainforest habitat}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-13239}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2004}, abstract = {The hoatzin (Opisthocomus hoazin) is an enigmatic bird that lives in the riparian lowlands of northern South America. Among its peculiar attributes are 1) microbial foregut fermentation, unique in birds, to convert plant cellulose in the foliage which it consumes into simple sugars, 2) an ongoing debate about the puzzling taxonomic position, although a relationship to the Cuculiformes appears likely, 3) adaptive wing claws in the young which are used for climbing, and 4) co-operative breeding behaviour. Despite the information available on digestive mode and taxonomy little has been published on its breeding biology and behaviour and until now almost all knowledge was based on a study in the savannah of Venezuela. This is the first detailed study of the hoatzin's nesting ecology in a rainforest habitat. From 1995-1998 and in 2000 I monitored a hoatzin population which consisted of approximately 700 individuals in an Amazonian rainforest in Ecuador situated in the Cuyabeno Wildlife Reserve (between 0°02' N, 76°0' W, 0°03' S, and 76°14' W). The area is composed of various black water lagoons and small rivers, flooded forests and terra firme forest. Primarily, I examined group composition and breeding pattern and success related to traits such as clutch and egg size, offspring sex ratio and the number of parents involved in a common breeding attempt. Apart from standardised observations and monitoring I took blood samples from chicks, which were later used for molecular sexing and for DNA fingerprints. Food plants were collected and determined and a rough habitat mapping was conducted. Since the impacts of boat tourism in the area became apparent I investigated the interactions of adult and young hoatzins with tourists and measured the plasma concentration of the hormone corticosterone in chicks as an indicator of stress. Each chapter has its own introduction to the specific topic and can be read independently. The main findings of this study are: The reproduction of the hoatzin was timed strictly following the bimodal rainy pattern in the area. There was only one breeding attempt per year. Only 18\% of breeding attempts ended successfully with at least one fledgling. Incubation started with the first egg laid and led to hatching asynchrony. In most cases only the A-chick survived and there is evidence for a brood reduction strategy. I observed egg size variation patterns both within the clutches and between the clutches. Approximately 80\% of breeding attempts were carried out with auxiliaries. Units with alloparentals had a higher breeding success than single pairs. The results indicate a trade-off between helping and group size. DNA band-sharing comparisons revealed the existence of joint-nests, where several females laid their eggs in one single nest. The clutches of these joint-nests suffered severe egg loss during all stages of incubation. Breeding success did not differ between single- and joint-nests. The primary offspring sex ratio was biased towards daughters. There was no differential mortality between the sexes until fledging. Individual breeding units employed an adaptive production of offspring of each sex according to their current group size. Rainforest tourism negatively influenced the survival and growth of young, not yet fledged hoatzins. In addition tourist-exposed young showed a stronger hormonal stress response than their conspecifics from undisturbed sites. In contrast, breeding adults appear to have habituated to tourist boats and exposure to observers.}, subject = {Hoatzins}, language = {en} } @phdthesis{Kotzsch2008, author = {Kotzsch, Alexander}, title = {BMP Ligand-Rezeptor-Komplexe: Molekulare Erkennung am Beispiel der Spezifischen Interaktion zwischen GDF-5 und BMPR-IB}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-31040}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2008}, abstract = {Knochenwachstumsfaktoren (Bone Morphogenetic Proteins, BMPs) sind ubiquit{\"a}re, sekretierte Proteine mit vielf{\"a}ltigen biologischen Funktionen. Die Vielfalt an zellul{\"a}ren Prozessen, die durch BMPs reguliert werden, von der Knochenentwicklung und Organhom{\"o}ostase bis hin zur Neurogenese, erstaunt - und wirft angesichts von teils redundanten, teils spezifischen Funktionen der BMPs Fragen zu den Mechanismen ihrer Signal{\"u}bermittlung auf. Die Signaltransduktion von BMPs erfolgt wie bei den strukturell verwandten TGF-\&\#946;s und Activinen durch die ligandeninduzierte Oligomerisierung von transmembranen Serin/Threonin-Kinaserezeptoren, von denen zwei Typen - Typ I und Typ II - existieren. Einer Vielzahl von mehr als 18 BMP-Liganden stehen nach derzeitigem Erkenntnisstand nur vier Typ I und drei Typ II Rezeptorsubtypen f{\"u}r die Bildung von heteromeren Rezeptorkomplexen zur Verf{\"u}gung. Ein BMP-Ligand kann hochspezifisch nur einen bestimmten Rezeptorsubtyp oder in einer promisken Art und Weise mehrere Rezeptorsubtypen binden. Trotz dieser Bindungspromiskuit{\"a}t {\"u}ben BMPs ihre biologische Funktion {\"u}berwiegend hochspezifisch aus, d.h. abh{\"a}ngig vom Liganden werden spezifische zellul{\"a}re Prozesse reguliert. Somit stellt sich die Frage, wie die Bildung von heteromeren Ligand-Rezeptor-Komplexen und die Aktivierung definierter intrazellul{\"a}rer Signalkaskaden zusammenh{\"a}ngen und wie letztlich ein bestimmtes BMP-Signal durch einen „Flaschenhals", repr{\"a}sentiert durch die begrenzte Anzahl an Rezeptorsubtypen, in das Zellinnere {\"u}bermittelt wird. Die Interaktionen zwischen BMP-2 / GDF-5 und den Typ I Rezeptoren BMPR-IA / BMPR-IB sind ein Paradebeispiel f{\"u}r Bindungspromiskuit{\"a}t und -spezifit{\"a}t. W{\"a}hrend BMP-2 beide Rezeptoren BMPR-IA und BMPR-IB mit gleicher Bindungsaffinit{\"a}t bindet („promiske Interaktion"), zeigt GDF-5 eine 15-20fach h{\"o}here Bindungsaffinit{\"a}t zu BMPR-IB („spezifische" Interaktion). Dieser Unterschied ist scheinbar gering, aber physiologisch {\"u}beraus relevant. Um Einblick in die Mechanismen der molekularen Erkennung zwischen den Bindungspartnern zu gewinnen, wurden bin{\"a}re und tern{\"a}re Komplexe aus den Liganden BMP-2 oder GDF-5, den extrazellul{\"a}ren Dom{\"a}nen der Typ I Rezeptoren BMPR-IA oder BMPR-IB sowie der extrazellul{\"a}ren Dom{\"a}ne des Typ II Rezeptors ActR-IIB untersucht. Die hier vorliegende Arbeit beschreibt die strukturelle und funktionelle Analyse dieser Ligand-Rezeptor-Komplexe. Um den Einfluss struktureller Flexibilit{\"a}t auf die BMP Typ I Rezeptor Erkennung n{\"a}her zu analysieren, wurde zudem die Struktur von BMPRIA in freiem Zustand mittels NMR-Spektroskopie aufgekl{\"a}rt. Aus Mutagenesedaten und der Kristallstruktur des GDF-5•BMPR-IB-Komplexes lassen sich im Vergleich zu bekannten Kristallstrukturen Merkmale ableiten, mit denen die Ligand-Rezeptor-Bindung und -Erkennung charakterisiert werden kann: (1) Die Hauptbindungsdeterminanten in Komplexen von BMPR-IA und BMPR-IB mit ihren Liganden sind unterschiedlich. W{\"a}hrend in Komplexen mit BMPR-IB ein hydrophobes Motiv die Bindungsaffinit{\"a}t bestimmt, tr{\"a}gt in Komplexen mit BMPR-IA eine polare Interaktion signifikant zur Bindungsenergie bei. Ein Vergleich der Strukturen von freien und gebundenen Liganden und Typ I Rezeptoren zeigt, dass interessanterweise diese Hauptbindemotive erst bei der Ligand-Rezeptor-Interaktion entstehen, sodass ein „induced fit" vorliegt und die Molek{\"u}le entsprechend „aufeinander falten". (2) Die Bindungsspezifit{\"a}t wird durch periphere Schleifen in den Typ I Rezeptoren bestimmt. Wie Untersuchungen von Punktmutationen in BMPR-IA zeigen, die einer krebsartigen Darmerkrankung (Juvenile Polyposis) zugrunde liegen, f{\"u}hrt erst die „richtige" Kombination aus Flexibilit{\"a}t in den Schleifen und Rigidit{\"a}t des Rezeptorgrundger{\"u}sts zu signalaktiven Typ I Rezeptoren mit einer potentiell den Liganden komplement{\"a}ren Oberfl{\"a}che. Die mangelnde sterische Komplementarit{\"a}t von Ligand- und Rezeptoroberfl{\"a}chen f{\"u}hrt zu der niedrigeren Bindungsaffinit{\"a}t von GDF-5 zu BMPR-IA im Vergleich zu BMPR-IB. Interessanterweise zeigen die hier vorgestellten, hochaufgel{\"o}sten Strukturdaten, dass die Orientierungen/Positionen der Typ I Rezeptoren BMPR-IA und BMPR-IB in den Bindeepitopen der Liganden BMP-2 und GDF-5 variieren. Unter der Voraussetzung, dass die extrazellul{\"a}re Dom{\"a}ne, das Transmembransegment und die intrazellul{\"a}re Dom{\"a}ne der Typ I Rezeptoren ein starres Element bilden, sollte sich die unterschiedliche Orientierung der extrazellul{\"a}ren Dom{\"a}nen der Typ I Rezeptoren in der Anordnung der Kinasedom{\"a}nen widerspiegeln und sich auf die Signaltransduktion auswirken. M{\"o}glicherweise ist eine bestimmte Anordnung der Kinasedom{\"a}nen der Typ I und Typ II Rezeptoren f{\"u}r eine effiziente Phosphorylierung bzw. Signaltransduktion erforderlich. Der Vergleich mehrerer Ligand-Typ I Rezeptor-Komplexe zeigt, dass die unterschiedliche Orientierung dieser Rezeptoren m{\"o}glicherweise vom Liganden abh{\"a}ngt. Angesichts der Bindungspromiskuit{\"a}t unter BMP-Liganden und -Rezeptoren k{\"o}nnten so spezifische Signale {\"u}bermittelt und spezifische biologische Funktionen reguliert werden. Die in dieser Arbeit vorgestellten Erkenntnisse tragen wesentlich zur strukturellen Charakterisierung der Ligand-Rezeptor-Erkennung in der BMP-Familie bei. Die Frage, warum trotz strukturell hoch homologer Liganden und Rezeptoren und weitgehend konservierten Bindeepitopen eine teils promiske und teils spezifische Interaktion m{\"o}glich ist, kann nun f{\"u}r die Liganden BMP-2 und GDF-5 sowie den beiden Typ I Rezeptoren BMPR-IA und BMPR-IB beantwortet werden.}, subject = {Cytokine}, language = {de} }