@phdthesis{Afify2007, author = {Afify, Samar}, title = {Drug targeting delivery systems for treatment of Raf-1 induced lung tumors in mice}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-22249}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2007}, abstract = {The aim of the present study was to design different dosage forms as carrier systems to deliver sorafenib to the lung of BXB-23 transgenic mice using different routes of administration. Three dosage forms were used one of them was an oil-in-water emulsion and the oral route was chosen for this experiment. The other delivery system was a liposome preparation for intratracheal instillation. In this case the oral route was considered as a control experiment. The last dosage form was PLGA microspheres. Before sorafenib administration it was important to develop a HPLC method to assess sorafenib absorption after its administration and to determine its concentrations in mouse serum. The HPLC method allowed sorafenib quantification in small volumes (30 µl) of mouse serum and tissues. The developed HPLC method was validated resulting in satisfactory selectivity, good linearity, good accuracy and precision over the concentration range examined. Sorafenib was successfully incorporated in a fat emulsion (o/w) using a traditional method resulting in a white homogenous emulsion and no particle aggregation was observed. Sorafenib exhibited antitumor activity on the lung adenoma in BXB-23 transgenic mice when administered orally (2 mg sorafenib per mouse) in the emulsion preparation. The determined effect was an approximately 29 \% reduction in the tumor area of the adenoma foci and a proliferation reduction. In order to improve the pharmacological effects of sorafenib on the lung adenoma in BXB-23 mice, the targeting of sorafenib directly to the site of action (the lung) was an attractive concept. For this purpose the intratracheal route was used. Since sorafenib administration by instillation required incorporation of sorafenib in a dosage form suitable for its lipophilic nature, a liposome suspension was the second dosage form used. A lyophilization method was employed for sorafenib liposome preparation utilizing dilauroylphosphatidylcholine (DLPC) which is safe and tolerable for the lung. Incorporation of sorafenib in the liposomes did not influence the particle size and its distribution. The sorafenib liposomes showed high encapsulation efficiency, good stability at 4 °C for one month and satisfactory in vitro release properties and inhibited Raf-1 mediated activation of ERK in cell culture assay. In a pharmacokinetic experiment sorafenib loaded liposomes were instilled directly into the lung. The results revealed that a significant level of sorafenib was achieved in the lung tissues after 2 hours and then reduced after 48 h and remained nearly constant for one week. On the other hand, only traces of sorafenib were found in the mice serum up to 48 h. Subsequently, the pharmacological activity of sorafenib (1 mg per mouse) was studied when delivered in a liposomal suspension intratracheally to treat the lung adenoma of BXB-23 mice. The data of this experiment demonstrated that sorafenib intratracheal instillation resulted in a reduction of tumor area of adenoma foci (67 \%) and an elevation of the percent of apoptotic cells. In contrast, prolongation of the treatment period did not further enhance sorafenib activity on the lung adenoma. This previous finding suggested a development of multidrug resistance (MDR) by the adenoma foci cells against sorafenib instillation, which was examined by immunohistochemistry staining. The percent of MDR positive cells was higher after two and three weeks sorafenib liposome instillation treatment than that after one week treatment. The last dosage form used for sorafenib was microspheres, which were prepared by emulsion-diffusion-evaporation method using biodegradable PLGA 50:50 resulting in a white lyophilized powder. The system was characterized physicochemically and revealed a good microspheres yield, high encapsulation efficiency, a homogenous particle size distribution and slow in vitro release of sorafenib. The other strategy studied in the present research project was gene delivery to target the lung bearing tumor of BXB-23 mice using a non-viral vector (polyethylenimine). Polyethylenimine (PEI) was used to investigate its efficiency in transfecting lung bearing tumor of BXB-23 mice model and its ability to transfect the adenoma foci cells. LacZ, which encodes Beta-galactosidase was used in the present study as a reporter gene and was complexed with PEI before delivered intravenously. A high LacZ expression in the alveolar region with some expression in the adenoma foci was observed. On contrary, a low LacZ expression in the alveoli and in the adenoma foci was achieved after instillation of the same polyplex intratracheally.}, subject = {Maus}, language = {en} } @phdthesis{Alrefai2014, author = {Alrefai, Hani Gouda Alsaid}, title = {Molecular Characterization of NFAT Transcription Factors in Experimental Mouse Models}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-97905}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2014}, abstract = {In this work we wanted to investigate the role of NFATc1 in lymphocyte physiology and in pathological conditions (eg. psoriasis). NFATc1 is part of the signal transduction pathways that regulates B cells activation and function. NFATc1 has different isoforms that are due to different promoters (P1 and P2), polyadenylation and alternative splicing. Moreover, we tried to elucidate the points of interactions between the NFAT and the NF-κB pathways in activated B-cell fate. NFAT and NF-κB factors share several properties, such as a similar mode of induction and architecture in their DNA binding domain. We used mice which over-express a constitutive active version of NFATc1/α in their B cells with -or without- an ablated IRF4. IRF4 inhibits cell cycle progression of germinal center B cell-derived Burkitt's lymphoma cells and induces terminal differentiation toward plasma cells. Our experiments showed that a 'double hit' in factors affecting B cell activation (NFATc1 in this case) and late B cell Differentiation (IRF4 in this case) alter the development of the B cells, lead to increase in their numbers and increase in stimulation induced proliferation. Therefore, the overall picture indicates a link between these 2 genes and probable carcinogenic alterations that may occur in B cells. We also show that in splenic B cells, c-Rel (of the NF-κB canonical pathway) Support the induction of NFATc1/αA through BCR signals. We also found evidence that the lack of NFATc1 affects the expression of Rel-B (of the NF-κB non-canonical pathway). These data suggest a tight interplay between NFATc1 and NF-κB in B cells, influencing the competence of B cells and their functions in peripheral tissues. We also used IMQ-induced psoriasis-like inflammation on mice which either lack NFATc1 from B cell. Psoriasis is a systemic chronic immunological disease characterized primarily by abnormal accelerated proliferation of the skin keratinocytes. In psoriasis, the precipitating event leads to immune cell activation. Our experiments showed that NFATc1 is needed for the development of psoriasis. It also showed that IL-10 is the link that enables NFAT from altering the B cell compartment (eg Bregs) in order to affect inflammation. The important role of B cell in psoriasis is supported by the flared up psoriasis-like inflammation in mice that lack B cells. Bregs is a special type of B cells that regulate other B cells and T cells; tuning the immunological response through immunomodulatory cytokines.}, subject = {Schuppenflechte}, language = {en} } @phdthesis{Araragi2013, author = {Araragi, Naozumi}, title = {Electrophysiological investigation of two animal models for emotional disorders - serotonin transporter knockout mice and tryptophan hydroxylase 2 knockout mice}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-83265}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2013}, abstract = {Serotonin (5-HT) has been implicated in the regulation of emotions as well as in its pathological states, such as anxiety disorders and depression. Mice with targeted deletion of genes encoding various mediators of central serotonergic neurotransmission therefore provides a powerful tool in understanding contributions of such mediators to homeostatic mechanisms as well as to the development of human emotional disorders. Within this thesis a battery of electrophysiological recordings were conducted in the dorsal raphe nucleus (DRN) and the hippocampus of two murine knockout lines with deficient serotonergic systems. Serotonin transporter knockout mice (5-Htt KO), which lack protein responsible for reuptake of 5-HT from the extracellular space and tryptophan hydroxylase 2 knockout (Tph2 KO) mice, which lack the gene encoding the neuronal 5-HT-synthesising enzyme. First, 5-HT1A receptor-mediated autoinhibition of serotonergic neuron firing in the DRN was assessed using the loose-seal cell-attached configuration. Stimulation of 5-HT1A receptors by a selective agonist, R-8-hydroxy-2-(di-n-propylamino)tetralin (R-8-OH-DPAT), showed a mild sensitisation and a marked desensitisation of these receptors in Tph2 KO and 5-Htt KO mice, respectively. While application of tryptophan, a precursor of 5-HT and a substrate of Tph2, did not cause autoinhibition in Tph2 KO mice due to the lack of endogenously produced 5-HT, data from 5-Htt KO mice as well as heterozygous mice of both KO mice lines demonstrated the presence of autoinhibitory mechanisms as normal as seen in wildtype (WT) controls. When the Tph2-dependent step in the 5-HT synthesis pathway was bypassed by application of 5-hydroxytryptophan (5-HTP), serotonergic neurons of both Tph2 KO and 5-Htt KO mice showed decrease in firing rates at lower concentrations of 5-HTP than in WT controls. Elevated responsiveness of serotonergic neurons from Tph2 KO mice correspond to mild sensitisation of 5-HT1A receptors, while responses from 5-Htt KO mice suggest that excess levels of extracellular 5-HT, created by the lack of 5-Htt, stimulates 5-HT1A receptors strong enough to overcome desensitisation of these receptors. Second, the whole-cell patch clamp recording data from serotonergic neurons in the DRN showed no differences in basic electrophysiological properties between Tph2 KO and WT mice, except lower membrane resistances of neurons from KO mice. Moreover, the whole-cell patch clamp recording from CA1 pyramidal neurons in the hippocampus of 5-Htt KO mice showed increased conductance both at a steady state and at action potential generation. Lastly, magnitude of long-term potentiation (LTP) induced by the Schaffer collateral/commissural pathway stimulation in the ventral hippocampus showed no differences among Tph2 KO, 5-Htt KO, and WT counterparts. Taken together, lack and excess of extracellular 5-HT caused sensitisation and desensitisation of autoinhibitory 5-HT1A receptors, respectively. However, this may not directly translate to the level of autoinhibitory regulation of serotonergic neuron firing when these receptors are stimulated by endogenously synthesised 5-HT. In general, KO mice studied here showed an astonishing level of resilience to genetic manipulations of the central serotonergic system, maintaining overall electrophysiological properties and normal LTP inducibility. This may further suggest existence of as-yet-unknown compensatory mechanisms buffering potential alterations induced by genetic manipulations.}, subject = {Serotonin}, language = {en} } @phdthesis{Auth2021, author = {Auth, Charlotte Sophie}, title = {Die Auswirkungen von Tph2-Defizienz und negativen fr{\"u}hen Umwelterfahrungen auf Angstverhalten in weiblichen M{\"a}usen}, doi = {10.25972/OPUS-23948}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-239488}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2021}, abstract = {Angsterkrankungen geh{\"o}ren zu den am weitesten verbreiteten psychischen Erkrankungen und stellen eine betr{\"a}chtliche soziale und wirtschaftliche Herausforderung f{\"u}r unsere Gesellschaft dar. Aversive fr{\"u}he Erfahrungen sind ein bekannter Risikofaktor f{\"u}r die Entwicklung verschiedener psychischer Erkrankungen, insbesondere Angstst{\"o}rungen. W{\"a}hrend der fr{\"u}hen Entwicklung findet die Programmierung der Hypothalamus-Hypophysen-Nebennierenrinden- (HHN)-Achse, die die Aussch{\"u}ttung des Stresshormons Cortisol in Menschen bzw. Corticosteron in M{\"a}usen steuert, statt. Wenn Individuen in dieser kritischen Phase Stress ausgesetzt sind, wird die regelrechte Ausbildung der HHN-Achse gest{\"o}rt, was zu dysregulierten Verhaltensantworten auf Stressreize im sp{\"a}teren Leben f{\"u}hren kann. Das Serotonin (5-HT)-System als eines der ausgedehntesten Neurotransmittersysteme ist an der Vermittlung der Effekte von fr{\"u}her Stressexposition auf angst{\"a}hnliche Verhaltensweisen beteiligt. Das Ziel dieser Studie ist es, die Interaktion zwischen genetischer Pr{\"a}disposition und negativen Einfl{\"u}ssen in fr{\"u}hen Entwicklungsstadien auf die Ausbildung von Angstverhalten im Erwachsenenalter n{\"a}her zu beleuchten. In dieser Studie wurden Tryptophanhydroxylase 2 (Tph2)-defiziente weibliche M{\"a}use als Modell f{\"u}r ein lebenslanges konstitutives 5-HT Synthesedefizit im zentralen Nervensystem verwendet. Nachkommen dieser Mauslinie wurden im fr{\"u}hen Lebensalter Maternaler Separation (MS), d.h. einem m{\"u}tterlichen Trennungsparadigma, unterzogen und im Erwachsenenalter im „Open field" (OF) oder in der „Dark-light box" (DLB) getestet. Im Anschluss an die Verhaltensexperimente wurde die neuronale Aktivierung immunhistochemisch durch Darstellung des fr{\"u}hzeitig auftretenden Genprodukts c-Fos bestimmt. In der DLB zeigten homozygot Tph2-defiziente M{\"a}use eine verringerte motorische Aktivit{\"a}t im hellen Kompartiment, und dieser Effekt konnte durch MS normalisiert werden. Zus{\"a}tzlich verst{\"a}rkte MS bei diesem Genotyp das Auftreten von fluchtartigen Spr{\"u}ngen. Im OF hat MS fluchtartige Verhaltensweisen in homo- und heterozygoten Tph2-defizienten M{\"a}usen bef{\"o}rdert. Beide Verhaltenstests f{\"u}hrten zu spezifischen neuronalen Aktivierungsmustern, die mithilfe von c-Fos- Immunhistochemie ausgewertet wurden. Die Durchf{\"u}hrung des DLB-Tests f{\"u}hrte in Abh{\"a}ngigkeit vom Vorhandensein von Tph2 zur Aktivierung des paraventrikul{\"a}ren Kerns des Hypothalamus (PVN) und der basolateralen Amygdala (BL), wohingegen die Exposition gegen{\"u}ber dem OF-Test zu einer Aktivierung der lateralen Amygdala (La) in Tieren, die einem m{\"u}tterlichen Trennungsparadigma unterzogen wurden, sowie einer Aktivierung des ventrolateralen (VLPAG) und dorsolateralen (DLPAG) periaqu{\"a}duktalen H{\"o}hlengraus in Abh{\"a}ngigkeit von Tph2 und MS f{\"u}hrte. Zusammenfassend weisen die Ergebnisse dieser Studie darauf hin, dass MS aktive Verhaltensantworten auf aversive Reize in Abh{\"a}ngigkeit vom Vorhandensein von 5-HT im Gehirn f{\"o}rdert. Diese Effekte k{\"o}nnten durch die spezifische Aktivierung von mit Angstverhalten in Zusammenhang stehenden Gehirnregionen w{\"a}hrend der Verhaltensexperimente vermittelt werden.}, subject = {Angst}, language = {de} } @phdthesis{Auth2005, author = {Auth, Tanja}, title = {Funktionelle Analyse der Interaktion und Lokalisation von Replikationsfaktoren und replikationsrelevanten Proteinen in Mauszellen}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-13082}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2005}, abstract = {Zeil dieser Arbeit war die Identifikation von Proteinen, die mit Bestandteilen des f{\"u}r die DNA-Replikation essentiellen pr{\"a}replikativen Komplexes in der Maus wechselwirken. Hierbei konnten Interkationen des Heterochromatin Proteins 1a mit den Replikationsfaktoren ORC1, ORC2 und CDC6 sowohl in Two Hybrid-Studien als auch in Immunpr{\"a}zipitationen gezeigt werden. Dar{\"u}berhinaus konnten signifikante Kolokalisationen dieser Proteine mit HP1a an heterochromatischen Regionen in murinen NIH3T3-Zellen nachgewiesen werden. Ebenfalls konnte hier erstmals eine Lokalisation von HP1a am Centrosom demonstriert werden. Ein siRNA-vermittelter Knock Down von HP1a zeigte jedoch keinen direkten Einfluß auf die Replikation. Es konnte hingegen gezeigt werden, daß ein Knock Down von HP1a in signifikatnen Defekten in der Cytokinese und einer deutlich verlangsamten Zellproliferation resultiert. So konnten h{\"a}ufig multinukle{\"a}re Zellen und eine Arretierung in der G1-Phase beobachtet werden. Weiterhin wurde der Einfluß der Phosphorylierung von HP1a durch die Casein Kinase II mithilfe von Phosphorylierungsmutanten untersucht. Im Gegensatz zu Drosophila-Zellen zeigten sich in murinen Zellen jedoch keine Auswirkungen dieser Mutationen auf die Lokalisation von HP1a an Heterochromatin. Wieterhin konnten Interaktionen des Replikationsinhibitors Geminin mit den Replikationsproteinen ORC1, ORC2 und CDC7 sowohl im Two Hybrid-System als auch in Immunpr{\"a}zipitationen gezeigt werden, die unterschiedliche Zellzyklusabh{\"a}ngigkeiten aufwiesen. In murinen NIH3T3-Zellen zeigte eine Knock Down von Geminin jedoch im Gegensatz zu anderen Zellinien keinen Einfluß auf die Replikation. In weiteren Teilen dieser Arbeit konnten Interaktionen des Retinoblastoma Proteins mit ORC2 und MCM7 sowohl in Two Hybrid- als auch in Immunpr{\"a}zipitations-Experimenten gezeigt werden. Dar{\"u}berhinaus wies Pescadillo Interaktionen mit den Replikationsproteinen ORC2, ORC6, MCM2, MCM3, MCM6 und CDC45 im Two Hybrid-System und Interaktionen mit MCM2 und MCM3 in Biolumineszenz-Resonanzenergietransfer-Experimenten auf. Eine Kolokalisation von Pescadillo und ORC6 in den Nukleoli l{\"a}ßt auf eine Funktion beider Proteinen bei der Ribosomen Biogenese schließen. Es konnten ebenfalls Interaktionen der Untereinheit E1 des humanen Papillomavirus Subtyp 11 mit den Replikationsfaktoren ORC2,3,4,5,6, MCM2, MCM3, MCM6, CDC6, CDC7, CDT1, HP1a, Rb und Pescadillo im Two Hybrid-System beobachtet werden.}, subject = {Maus}, language = {de} } @phdthesis{Bacmeister2018, author = {Bacmeister, Lucas}, title = {Effect of Cadherin-13 inactivation on different GABAergic interneuron populations of the mouse hippocampus}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-172693}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2018}, abstract = {Cadherin-13 (CDH13) is an atypical member of the cadherin superfamily, a group of membrane proteins mediating calcium-dependent cellular adhesion. Although CDH13 shows the classical extracellular cadherin structure, the typical transmembrane and cytoplasmic domains are absent. Instead, CDH13 is attached to the cell membrane via a glycosylphosphatidylinositol (GPI) anchor. These findings and many studies from different fields suggest that CDH13 also plays a role as a cellular receptor. Interestingly, many genome-wide association studies (GWAS) have found CDH13 as a risk gene for attention-deficit/hyperactivity disorder (ADHD) and other neurodevelopmental disorders. In previous work from our research group, strong expression of Cdh13 mRNA in interneurons of the hippocampal stratum oriens (SO) was detected. Therefore, double-immunofluorescence studies were used to evaluate the degree of co-expression of CDH13 with seven markers of GABAergic interneuron subtypes. For this purpose, murine brains were double stained against CDH13 and the respective marker and the degree of colocalization in the SO of the hippocampus was assessed. Based on the result of this immunofluorescence study, quantitative differences in interneuron subtypes of the SO between Cdh13 knockout (ko), heterozygote (het) and wildtype (wt) mice were investigated in this dissertation using stereological methods. In addition, genotype- dependent differences in the expression of genes involved in GABAergic and glutamatergic neurotransmission were analyzed by quantitative real-time PCR (qRT-PCR). Primers targeting different GABA receptor subunits, vesicular GABA and glutamate transporter, GABA synthesizing enzymes and their interaction partners were used for this purpose. The results of the stereological quantification of the interneuron subtypes show no significant differences in cell number, cell density or volume of the SO between Cdh13 ko, het and wt mice. On the other hand, qRT-PCR results indicate significant differences in the expression of tropomyosin-related kinase B gene (TrkB), which encodes the receptor of brain-derived neurotrophic factor (BDNF), a regulator of GABAergic neurons. This finding supports a role for CDH13 in the regulation of BDNF signaling in the hippocampus.}, subject = {Cadherine}, language = {en} } @phdthesis{Baig2019, author = {Baig, Ayesha Anjum}, title = {Studies on platelet interactions with the coagulation system and on modulators of platelet (hem)ITAM signaling in genetically modified mice}, doi = {10.25972/OPUS-16488}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-164888}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2019}, abstract = {Activated platelets and coagulation jointly contribute to physiological hemostasis. However, pathological conditions can also trigger unwanted platelet activation and initiation of coagulation resulting in thrombosis and precipitation of ischemic damage of vital organs such as the heart or brain. The specific contribution of procoagulant platelets, positioned at the interface of the processes of platelet activation and coagulation, in ischemic stroke had remained uninvestigated. The first section of the thesis addresses this aspect through experiments conducted in novel megakaryocyte- and platelet-specific TMEM16F conditional KO mice (cKO). cKO platelets phenocopied defects in platelets from Scott Syndrome patients and had severely impaired procoagulant characteristics. This led to decelerated platelet-driven thrombin generation and delayed fibrin formation. cKO mice displayed prolonged bleeding times and impaired arterial thrombosis. However, infarct volumes in cKO mice were comparable to wildtype (WT) mice in an experimental model of ischemic stroke. Therefore, while TMEM16F-regulated platelet procoagulant activity is critical for hemostasis and thrombosis, it is dispensable for cerebral thrombo-inflammation in mice. The second section describes the generation and initial characterization of a novel knockin mouse strain that expresses human coagulation factor XII (FXII) instead of endogenous murine FXII. These knockin mice had normal occlusion times in an experimental model of arterial thrombosis demonstrating that human FXII is functional in mice. Therefore, these mice constitute a valuable tool for testing novel pharmacological agents against human FXII - an attractive potential target for antithrombotic therapy. Glycoprotein (GP)VI and C-type lectin-like receptor 2 (CLEC-2)-mediated (hem)immunoreceptor tyrosine-based activation motif (ITAM) signaling represent a major pathway for platelet activation. The last section of the thesis provides experimental evidence for redundant functions between the two members of the Grb2 family of adapter proteins - Grb2 and Gads that lie downstream of GPVI and CLEC-2 stimulation. In vitro and in vivo studies in mice deficient in both Grb2 and Gads (DKO) revealed that DKO platelets had defects in (hem)ITAM-stimulation-specific activation, aggregation and signal transduction that were more severe than the defects observed in single Grb2 KO or Gads KO mice. Furthermore, the specific role of these adapters downstream of (hem)ITAM signaling was essential for maintenance of hemostasis but dispensable for the known CLEC-2 dependent regulation of blood-lymphatic vessel separation.}, subject = {Blutgerinnung}, language = {en} } @phdthesis{Bartlang2014, author = {Bartlang, Manuela Slavica}, title = {Timing is everything: The interaction of psychosocial stress and the circadian clock in male C57BL/6 mice}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-106486}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2014}, abstract = {Due to the rotation of the earth in the solar system all inhabitants of our planet are exposed to regular environmental changes since more than 3.5 billion years. In order to anticipate these predictable changes in the environment, evolutionarily conserved biological rhythms have evolved in most organisms - ranging from ancient cyanobacteria up to human beings - and also at different levels of organization - from single cells up to behavior. These rhythms are endogenously generated by so called circadian clocks in our body and entrained to the 24 h cycle by external timing cues. In multi-cellular organisms the majority of the cells in the body is equipped with such an oscillator. In mammals, the circadian system is structured in a hierarchical fashion: A central pacemaker resides in the bilateral suprachiasmatic nucleus (SCN) of the hypothalamus, while subsidiary peripheral clocks exist in nearly every tissue and organ. In contrast to the aforementioned recurrent environmental changes most organisms are also exposed to unpredictable changes in the environment. In order to adapt to these sudden alterations the acute activation of the stress response system, involving the hypothalamic-pituitary-adrenal (HPA) axis and the sympathetic nervous system, displays a fundamental survival mechanism. However, if activation of the stress system becomes chronic, devastating somatic and affective disorders might be the consequence. At first glance, the circadian and the stress system seem to represent two separate bodily control systems that are involved in adaptation to predictable and unpredictable stimuli, respectively. However, both systems are fundamental for survival, and thus, communicate with each other at various levels. Early studies already demonstrated that stressor exposure at different times of the diurnal cycle generates different stress effects, whereupon the type of stressor plays a pivotal role. Moreover, alterations in the SCN and peripheral circadian clocks could be shown following stressor exposure. In cooperation with various co-workers, I investigated whether the stress responsiveness is modulated by the endogenous clock in a diurnal fashion and whether repeated psychosocial stress impacts the circadian clock depending on the time of day of stressor exposure. Therefore, male C57BL/6 mice were repeatedly exposed to a psychosocial stressor, either at the beginning of the inactive/light phase (SDL mice) or active/dark phase (SDD mice). Subsequently, different behavioral, physiological/endocrine and immunological/ inflammatory consequences were assessed. It could be shown that the effects of repeated psychosocial stressor exposure strongly depend on the time of day of stressor exposure. The present results demonstrate that repeated daily stressor exposure has a more negative outcome when applied during the active/dark phase compared to the inactive/light phase. Stressor exposure during the active phase resulted in a loss of general activity, decreased interest in an unfamiliar conspecific, a shift towards a more pro-inflammatory body milieu, and rhythm disturbances in plasma hormones, all representing well-accepted hallmarks of depression. In contrast, C57BL/6 mice exposed to the stressor in their inactive phase exhibited minor physiological alterations that might prevent the formation of the maladaptive consequences mentioned above, thus representing beneficial adaptations. The second focus of this thesis was put on the investigation of the effects of repeated psychosocial stressor exposure at different times of the light-dark cycle on various levels of the circadian system. An increased expression of the PERIOD2 (PER2) protein, which represents an essential core clock component, could be found in the SCN of mice repeatedly exposed to the stressor during their active phase. In consistence with the alterations in the central circadian pacemaker, the daily rhythm of different hormones and the activity rhythm were considerably affected by SDD. Mice exposed to the psychosocial stressor in their active phase showed a shifted, or absent, rhythm of the hormones corticosterone and leptin. Moreover, their activity was found to be phase-delayed, which seems to be attributable to the Period (Per) gene since Per1/Per2 double-mutants still exhibited their normal activity rhythm following 19 days of stressor exposure during the active phase. In contrast, a phase-advance in the peripheral adrenal gland clock could be seen in C57BL/6 mice subjected to the stressor during their inactive phase. This phase-shift might be required for maintaining the normal rhythmicity in hormonal release and activity. It has previously been suggested that activation of the HPA axis upon stressor exposure at different times of the light-dark cycle is depending on whether the stressor is of physical or psychological nature. Data from the HPA axis analysis now refine previous findings, indicating that psychosocial stressors also modulate HPA axis responses based on the time of day of stressor presentation. The present results demonstrate that HPA axis activity was reduced following repeated stressor exposure during the active phase. It is reasonable to speculate that this reduced basal activity of the stress system represents a failure in HPA axis adjustment, which could contribute to the negative consequences of repeated psychosocial stressor exposure during the dark phase. Taken together, it can be concluded that the endogenous clock in mice modulates the stress responsiveness in a circadian fashion and that repeated psychosocial stressor exposure affects the biological clock depending on the time of day of stressor presentation. Thereby, stressor exposure during the active phase results in a more negative outcome as compared to stressor experience during the inactive phase. It is assumed that the interaction between the circadian clock and the stress system is a complex issue that might ensure that the endogenous clock does not get out of synchrony in any order.}, subject = {Maus}, language = {en} } @phdthesis{Bergert2011, author = {Bergert, Maria Pamela}, title = {Zellul{\"a}re und quantitative Verteilung von Glutamattransportern im Kleinhirn der Maus w{\"a}hrend der postnatalen Ontogenese}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-76689}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2011}, abstract = {Zellul{\"a}re und quantitative Verteilung von Glutamattransportern im Kleinhirn der Maus w{\"a}hrend der postnatalen Ontogenese}, subject = {Glutamattransporter}, language = {de} } @phdthesis{Bettaga2014, author = {Bettaga, Noomen}, title = {Bedeutung der NO-sensitiven Guanylyl Cyclase bei der Angiogenese und der Arteriogenese in der Maus}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-111284}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2014}, abstract = {Stickstoffmonoxid (NO) spielt eine wichtige Rolle bei Gef{\"a}ßremodelling-Prozessen wie Angiogenese und Arteriogenese. Die NO-Synthese im Gef{\"a}ßsystem wird haupts{\"a}chlich durch die endotheliale NO-Synthase (eNOS) gew{\"a}hrleistet. Sie kann durch verschiedene Faktoren wie Scherkr{\"a}fte und Zytokine wie der vaskul{\"a}re endotheliale Wachstumsfaktor (VEGF) reguliert werden. VEGF ist ein wichtiger Stimulator der Angiogenese und wird w{\"a}hrend dieses Prozesses hochreguliert. Die meisten physiologischen Effekte von NO werden durch die NO-sensitive Guanylyl-Cyclase (NO-GC) vermittelt. Als Hauptrezeptor f{\"u}r NO produziert die NO-GC den sekund{\"a}ren Botenstoff cyklisches Guanosinmonophosphat (cGMP) und f{\"u}hrt dadurch zur Stimulation der verschiedenen Effektoren wie z.B. der PKG. Ob die Wirkung von NO in Angiogenese und Arteriogenese ebenfalls durch NO-GC vermittelt wird, war bis zum Beginn dieser Arbeit noch unklar. Die NO-GC besteht aus zwei Untereinheiten (α und ß). Die Deletion der ß1-Untereinheit in M{\"a}usen resultiert in einer vollst{\"a}ndigen Knockout Maus (GCKO). Mithilfe des Cre-LoxP-Systems wurden zus{\"a}tzlich zellspezifische Knockout-M{\"a}use f{\"u}r glatte Muskelzellen (SMC-GCKO) und Endothelzellen (EC-GCKO) generiert. Um die Rolle der NO-GC in der Angiogenese und Arteriogenese zu untersuchen, wurden drei gut etablierte Methoden benutzt. Im ersten Teil des Projekts sollte die Expression der NO-GC in Endothelzellen untersucht werden. Zu diesem Zweck wurde die reverse Transkriptase-Polymerase-Kettenreaktion (RT-PCR) benutzt. Die Ergebnisse zeigen, dass die NO-GC in Endothelzellen der Lunge nur {\"a}ußerst gering wenig exprimiert ist. Durch den Aortenring-Assay wurde eine Rolle der NO-GC bei der VEGF-vermittelten Angiogenese festgestellt. Dabei zeigte sich eine st{\"a}rkere Angiogeneserate bei globaler Abwesenheit der NO-GC. Bei Fehlen der NO-GC ausschließlich in Endothelzellen zeigte sich kein Unterschied in den aussprossenden Aorten im Vergleich zu den Kontroll-Tieren. Dies zeigt, dass die NO-GC in Endothelzellen sehr wahrscheinlich keine Rolle bei der VEGF-vermittelten Angiogenese spielt. Im zweiten Teil wurde die Rolle der NO-GC bei der Angiogenese in einem in vivo-Modell untersucht. In dem Modell der Sauerstoff-induzierten-Retinopathie zeigten die GCKO-M{\"a}use eine verringerte Vaso-Obliteration, eine verlangsamte Angiogenese und eine erh{\"o}hte Tuft-Bildung. {\"A}hnliche Ergebnisse wurden bei den SMC-GCKO-Tieren beobachtet. EC-GCKO-M{\"a}use zeigten eine gegen{\"u}ber den Kontroll-Tieren unver{\"a}nderte Vaso-Obliteration, Angiogeneserate und Tuft-Bildung. Diese Ergebnisse lassen darauf schließen, dass die NO-GC in Endothelzellen keine Rolle spielt. Immunfluoreszenz-Aufnahmen zeigten die Expression von NO-GC in Perizyten der Gef{\"a}ßkapillaren der Mausretina. Daher k{\"o}nnte die NO-GC in diesem Zelltyp letztendlich f{\"u}r die Effekte bei den GCKO- und SMC-GCKO-Tieren verantwortlich sein. Im letzten Teil dieser Arbeit wurde eine Versuchsreihe unter Anwendung des Hinterlauf-Isch{\"a}mie-Modells durchgef{\"u}hrt. Hierbei entwickelten die Pfoten aller GCKO- und teilweise der SMC-GCKO-Tiere nach der Ligation der Femoralarterie eine Nekrose. Die Regeneration der Hinterl{\"a}ufe der EC-GCKO-Tiere nach der Operation verlief normal. Diese Ergebnisse schließen eine bedeutende Rolle der NO-GC in Endothelzellen aus, zeigen allerdings, dass die NO-GC in den glatten Muskelzellen essentiell f{\"u}r den Arteriogenese-Prozess ist. Zusammengefasst f{\"u}hrt die Deletion der NO-GC in glatten Muskelzellen und wahrscheinlich auch in Perizyten zur einer verlangsamten Angiogenese und Inhibierung der Arteriogenese.}, subject = {Guanylylcyclase}, language = {de} }