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Introduction: The involvement of platelets in various diseases has been increasingly recognized in the recent decades. This contribution is believed to involve platelet secretion and formation of reactive microparticles. Platelets contain two functionally important forms of vesicles, alpha and dense granules, which are secreted upon activation of platelets. Alpha granules incorporate larger molecules such as adhesive proteins, e.g. P-selectin, vWF and fibrinogen; chemokines like PF4 and RANTES and growth hormones like VEGF and PDGF are among the most important proteins attributed to the involvement of platelets in pathological conditions. In contrast, dense granules contain small molecules like ADP, ATP, serotonin and histamine, and they are more rapidly and completely secreted than alpha granules. Like in all secreting cells, regulated exocytosis in platelets is mediated by “zippering” of three different classes of SNARE proteins. The subtypes of these proteins found to be involved in platelet secretion are SNAP-23, syntaxin-2 and -4 and VAMP-3 and -8. Apart from SNARE proteins, other conserved proteins influencing exocytosis by e.g. acting on SNARE proteins have been described, one of the most important ones being Munc13. Platelets contribute to the progression of atherosclerosis by local deposition of inflammatory mediators like PF4, RANTES and CD40L, which leads to enhanced leukocyte recruitment and plaque formation. In 1865, Armand Trousseau first described the correlation between cancer and thrombotic events. Since the 1960s, an increasing number of studies have found an involvement of platelets also in the progression of cancer, especially in the formation of metastases. Platelets bind to circulating tumor cells and may shield them from NK cell attacks and shear stress. Platelets may also facilitate the interaction of tumor cells with other cell types and the vessel wall. Lastly, they may secrete molecules that influence the tumor cell phenotype and invasiveness.
Aims of this study: We sought to generate and describe genetically modified mouse lines with defective platelet secretion and to employ these mouse lines in murine models of atherosclerosis and tumor progression to study the role of platelet secretion under pathological in vivo conditions.
Results: Clostridial toxins cleave members of the SNARE protein family and can thus completely block exocytosis of neuronal and other cells. We generated three transgenic mouse lines expressing tetanus, botulinum-E or -C light chains and two transgenic mouse lines with dominant-negative mutations of SNAP-23 under the control of the platelet-specific PF4 promotor. None of these constructs was able to interfere with platelet secretion despite expression of the transgene. A functional null mutant of the only Munc13 isoform expressed in platelets, Munc13-4, showed complete lack of dense granule secretion, measured by ATP release, while alpha granule release as determined by PF4 and vWF secretion, was unaltered. Morphology, composition and adhesion of these platelets were also normal. Aggregation in response to U46619 and collagen and formation of large aggregates in flow chamber assays was attenuated. Munc13-4-deficient mice showed a severe defect in bleeding time and no formation of stable aggregates in FeCl3 thrombosis model. In response to B16 melanoma and LLC1 carcinoma cells, Munc13-4 KO platelets also showed complete abrogation of dense granule secretion, whereas alpha granule secretion and binding of platelets to tumor cells was unchanged. Interestingly, wild-type platelets, but not Munc13-4 KO platelets, enhanced transmigration of B16 and LLC1 cells through an endothelial cell layer. Exogenous ATP was able to mimic the effect of wild-type platelets and the ATP-degrading enzyme apyrase blocked platelet-mediated tumor cell transmigration. Platelets incubated with tumor cells secreted large amounts of ATP. Murine endothelial cells showed perturbed adherens junctions identified by irregular VE-cadherin staining and gap formation when incubated with supernatants from tumor cell-activated platelets as well as increased permeability under the same conditions. Addition of apyrase preserved normal endothelial morphology and function. In vivo, primary tumor growth and weight was comparable in wild-type and Munc13-4 KO mice upon B16 or LLC1 flank injection but formation of lung metastases was strongly reduced. Number, but not size of metastases was also reduced upon i.v. injection of B16 and LLC1 cells. We found P2Y2 and P2X4 receptors to be the most abundantly expressed endothelial metabotropic and ionotropic ATP receptors, respectively. Neither knock-down nor inhibition of P2X4 in endothelial cells influenced platelet-mediated transendothelial migration of B16 cells, but knock-down of P2Y2, for which no specific antagonist is available, strongly reduced plateletdependent tumor cell transmigration. When B16 melanoma cells were injected i.v. shortly after FITC-dextran (70 kDa) into wild-type mice, prominent leakage of FITC-dextran was observed three hours post-injection at extraluminal sites in the lung. In contrast, leakage into the lung parenchyma was at basal levels in Munc13-4 KO and P2Y2 KO mice after B16 cell injection. Marginal vascular leakage in Munc13-4 KO mice lacking platelet ATP secretion and in P2Y2 KO mice lacking the main endothelial ATP receptor correlated with strongly reduced extravasation of CFSE-labeled B16 melanoma cells 6 hours post-injection in these mice. Consistently, P2Y2 KO mice showed strongly reduced formation of metastases in the lung after i.v. injection of B16 or LLC1 tumor cells. Bone marrow-transplanted LDLR KO mice reconstituted with Munc13-4-deficient or wildtype bone marrow and subjected to 16 weeks of high fat diet showed no significant difference in atherosclerotic plaque formation in the aorta.
Discussion: We hereby provide a thorough analysis of a mouse line with an exclusive defect in platelet dense granule secretion, thus representing a unique genetic tool to study the role of dense granule secretion in various contexts without interfering with other platelet functions. We also provide evidence how extravasation of circulating tumor cells is facilitated by tumor cell-induced ATP release from platelets. This ATP release destabilizes endothelial barriers and facilitates tumor cell extravasation and formation of metastases in the target organ. Since metastasis is the leading cause of cancer death, pharmacological interference with endothelial P2Y2 receptor function may represent a promising therapeutic strategy.
Untersuchungen zur Bedeutung von Superoxid-Dismutasen für die Alterung von Podospora anserina
(2012)
Im Rahmen dieser vorliegenden Doktorarbeit sollte die Bedeutung von Superoxid-Dismutasen für das Resistenzverhalten und den Alterungsprozess bei P. anserina untersucht werden. Folgende Befunde aus den Analysen konnten erhalten werden:
1. Lokalisationsstudien der drei PaSods: Aus den biochemischen und fluoreszenzmikroskopischen Untersuchungen der drei verschiedenen PaSODs geht hervor, dass PaSOD1, eine Cu/ZnSOD, überwiegend im Cytosol und zu einem geringen Anteil im mitochondrialen Intermembranraum lokalisiert ist. Eine der beiden MnSODs, PaSOD2, wird vermutlich zur Abwehr von exogenem Superoxid sekretiert. Bei PaSOD3 handelt es sich um eine mitochondriale MnSOD.
2. Generierung von verschiedenen PaSod-Mutanten: Im Rahmen dieser Arbeit wurden von jeder PaSod mindestens drei unabhängige Überexpressionsstämme, ein GFP-Stamm- und ein Deletionsstamm hergestellt. Weiterhin wurden alle möglichen Doppel-Deletionsstämme und die Dreifach-Deletionsmutante erzeugt. Alle Stämme wurden auf DNA-Ebene verifiziert, zusätzlich wurde die Proteinmenge bzw. –Aktivität überprüft.
3. Einfluss der PaSODs auf die ROS-Toleranz: Die Analysen der ROS-Resistenzen haben gezeigt, dass PaSODs eine wichtige Rolle in der Entgiftung von Superoxiden spielt. So ließ sich bei den Deletionsstämmen der PaSods eine gesteigerte Sensitivität gegenüber Paraquat feststellen. Eine Aufsummierung der Sensitivität gegenüber Paraquat ist bei der PaSod-Tripelmutante (ΔPaSod1/2/3) zu erkennen.
Überraschenderweise kann durch die gesteigerten Mengen an aktiver PaSOD in den Überexpressionsstämmen (PaSod1-3_OEx) keine verbesserte Resistenz gegenüber Paraquat erzielt werden. Darüber hinaus führt die Überexpression des Gens für die mitochondriale SOD, PaSOD3, zu massiven negativen Effekten.
4. Einfluss auf die Lebensspanne: Durch eine fehlende Entgiftung von Superoxid in den PaSod-Deletionsmutanten ist eine Verminderung der Lebensspanne nicht festzustellen. Bei PaSod-Mutantenstämme, die eine erhöhte PaSOD-Aktivität und damit eine gesteigerte Abbaurate des Superoxids aufweisen, kann bei den PaSod1- und PaSod2-Überexpressionsstämmen keine verbesserte Lebensspanne unter den gewählten Standardbedingungen erzielt werden. Vielmehr noch ist die Lebensspanne der PaSod3-Überexpressionsstämme stark reduziert.
5. Einfluss der PaSod-Modulation auf andere Komponenten des ROS-Abbausystems: Die PaSOD-Aktivitäten scheinen miteinander co-reguliert zu werden. Des Weiteren scheint es ein Zusammenhang zwischen den beiden sekretierten Enzymen PaSOD2 und PaCATB zu geben. Deutlich wird auch, dass die Modulation der Superoxid-Dismutasen eine weitreichende Auswirkung auf andere Schutzsysteme hat. Beispielweise konnte gezeigt werden, dass Komponenten des mitochondrialen ROS-Schutzsystems und der Protein-Qualitätskontrolle in den PaSod3-Überexpressionsstämmen verändert sind.
Zusammenfassend lassen die Analysen der PaSod-modulierten Stämme den Schluss zu, dass die Superoxid-Dismutase in P. anserina ein wichtiges Enzym zum Abbau des schädlichen Superoxids darstellt, welches aber nur eine untergeordnete Rolle bei der Kontrolle der Lebensspanne unter den gewählten Wachstumsbedingungen im Labor ausübt. Des Weiteren haben die Analysen gezeigt, dass es durch die Modulation der PaSod-Gene zu weitreichenden Änderungen, die das ROS-Schutzsystem (PaSOD, PaCATB und PaPRX1) sowie die Protein-Qualitätskontrolle (PaHSP60, PaLON und PaCLPP) betreffen, kommt. Welche Auswirkung dabei diese Veränderungen in Bezug auf die Lebensspanne hat, kann nur schwer abgeschätzt werden und muss mit weiteren Untersuchungen geklärt werden.
In the first part of this work, the development of a novel two-dimensional native gel electrophoretic system (2-D BN/hrCNE) is described. This new system simplifies proteomics and biochemical analysis of mega protein complexes that are dissociated into the constituent complexes during 2-D electrophoresis, thereby reducing the complexity of the system considerably. This technique is exceptionally well suited for the in-gel detection of fluorescence-labeled proteins and the identification of individual enzymes and protein complexes by specific in-gel assays on native gels.
In the second part, a new technique for the native immunoblotting of blue native gels (NIBN) was developed. This new technique allows for the identification of conformation-specific antibodies and the discrimination of antibodies recognizing linear epitopes of denatured proteins. Identification of conformation-specific antibodies is becoming increasingly important not only for the electron microscopic identification of native proteins but also for structural investigations in general. For this purpose, a commonly used protocol for Western blotting of blue native gels was modified in such a way that the native state of proteins and protein complexes was retained throughout the complete protocol. Instead of using the denaturing methanol in Western blotting protocols, mild detergents such as Tween 20, digitonin and Brij 35 were used for the obligatory removal of protein bound Coomassie-dye.
The detection of respiratory complex I by activity staining on the blot membrane demonstrated that all three non-ionic detergents preserved the native state of complex I. The native state of the enzyme on the blot membrane was also monitored and confirmed with the help of a set of conformation-specific antibodies. NIBN can be used as a simple alternative method to the demanding native ELISA to screen for conformation-specific antibodies for structural studies. Unlike the time consuming native ELISA, NIBN does not require introduction of appropriate affinity tags and purification of the target protein by chromatography. Thus, the NIBN technique is especially useful for microscale projects and for proteins not easily accessible to genetic manipulation.
The third part aimed at identification of the immediate protein interaction partners of Cox26, a hydrophobic protein that has been identified by our group as a novel component of yeast respiratory supercomplex. Multi-dimensional electrophoretic techniques were applied to identify non-covalent and covalent protein-protein interactions of Cox26. Three-dimensional electrophoresis (BNE/BNE/SDS-PAGE) gave both qualitative and quantitative information on covalent and non-covalent interactions of Cox26 and subunits of cytochrome c oxidase (complex IV), and showed that most of the Cox26 protein was non-covalently bound to the complex IV moiety of the respirasomes. Four-dimensional electrophoresis (BNE/BNE/SDS/SDS-PAGE) applying reducing and non-reducing conditions revealed that a minor fraction of Cox26 used a single cysteine residue in the center of a predicted transmembrane helix to form a disulfide bond with the Cox2 subunit of complex IV. A structural role of Cox26 protein in the assembly/stability of respiratory strings or patches has been suggested.
The last part of this work focused on the isolation and characterization of native and morphologically intact nucleoids from bovine heart mitochondria, since only a few studies on nucleoid organization and composition have been carried out on mammalian tissues. The nucleoids appeared as distinct bands (apparent mass around 30-36 MDa) in blue native-PAGE on large pore gels. The moderate variation in particle size seems to reflect variations in the binding of loosely nucleoid-associated components like respiratory chain complexes. The estimated 30-36 MDa mass of nucleoids on native gels suggested that each nucleoid contains one mtDNA molecule provided that nucleoids contains equal amounts of DNA, protein and RNA (Miyakawa et al., 1987).
Electron microscopic analysis of native nucleoids, which was performed by Dr. Karen Davies from the Max-Planck-Institute of Biophysics, Department of Structural Biology, Frankfurt, showed homogenous pool of particles with dimensions in 85x100 nm (in negative stain) and 100x150 nm (in cryo-tomography). Some of the nucleoids showed dumbbell-shape indicating dimerization of nucleoids. Recent EM and high-resolution light microscopy analysis of mammalian nucleoids have reported that nucleoids have a size of 70 nm in average. We also observed the same size of 70 nm in cryo-tomogramms when we applied harsher treatment of the native nucleoid particles with dimensions 100x150 nm. This observation is in agreement with published nucleoid sizes from both EM and high-resolution light microscopy, if we assume that native nucleoids have been dissociated under harsher treatment.
The protein composition of bovine heart mt-nucleoids was analyzed by a number of complementary approaches to identify low and highly abundant, easily dissociating and tightly bound proteins, and to rank the 90 most abundant mt-nucleoid proteins. Native and denaturing gel electrophoresis techniques were coupled to LC-MS/MS to achieve a comprehensive protein component analysis. Qualitative MS analysis of highly purified nucleoids identified more than 400 proteins, including well known nucleoid proteins such as mitochondrial transcription factor and mtDNA-binding protein (TFAM), mitochondrial single-stranded DNA-binding protein (mtSSB), mitochondrial DNA polymerase subunit gamma-2 (POLG2) and mitochondrial helicase C26H10ORF2 protein (Twinkle). These proteins were ranked according to Mascot scores, and sorted according to presumed functional properties. A large group of proteins involved in protein synthesis comprised an almost complete set of subunits of mitochondrial ribosomes suggesting that the nucleoids contained significant amounts of mitochondrial ribosomes. Identification of sixty six proteins from the oxidative phosphorylation (OXPHOS) system comprising around 100 proteins in total suggested that OXPHOS proteins are also associated with mt-nucleoids.
Interestingly, TFAM, described as a main mtDNA packaging factor in human and other mammalian cells, was not confirmed here as a major nucleoid component from bovine heart mitochondria. Fluorescence staining of protein spots on 2-D IEF/SDS gels clearly identified TFAM, but according to the stain intensity, this protein did not rank in the list of the 90 most abundant nucleoid proteins. Western blot analysis of sucrose gradient fractions revealed an enrichment of putative TFAM isoform in nucleoid fractions. Unexpectedly, the uncharacterized mitochondrial protein Es1 was identified as the most abundant nucleoid protein in bovine heart nucleoids instead. This implicates that nucleoid organization may differ between species and tissues. A functional characterization of Es1 is required to clarify its role in mammalian nucleoids.
Pulsed electron–electron double resonance (PELDOR) spectroscopy is a powerful tool for measuring nanometer distances in spin-labeled systems and recently is increasingly applied to membrane proteins. However, after reconstitution of labeled proteins into liposomes, spin labels often exhibit a much faster transversal relaxation (Tm) than in detergent micelles, thus limiting application of the method in lipid bilayers. In the first part of the thesis, optimization of transversal relaxation in phospholipid membranes was systematically investigated by use of spin-labeled derivatives of stearic acid and phosphatidylcholine as well as spin-labeled derivatives of the channel-forming peptide gramicidin A under the conditions typically employed for PELDOR distance measurements. Our results clearly show that dephasing due to instantaneous diffusion that depends on dipolar interaction among electron spins is an important contributor to the fast echo decay in cases of high local concentrations of spin labels in membranes. The main difference between spin labels in detergent micelles and membranes is their local concentration. Consequently, avoiding spin aggregation and suppressing instantaneous diffusion is the key step for maximizing PELDOR sensitivity in lipid membranes. Even though proton spin diffusion is an important relaxation mechanism, only in samples with low local concentrations does deuteration of acyl chains and buffer significantly prolong Tm. In these cases, values of up to 7 μs have been achieved. Furthermore, our study revealed that membrane composition and labeling position in the membrane can also affect Tm, either by promoting the segregation of spin-labeled species or by altering their exposure to matrix protons. Effects of other experimental parameters including temperature (<50 K), presence of oxygen, and cryoprotectant type are negligible under our experimental conditions.
In the second part of the thesis, inhomogeneous distribution of spin-labels in detergent micelles has been studied. A common approach in PELDOR is measuring the distance between two covalently attached spin labels in a macromolecule or singly-labeled components of an oligomer. This situation has been described as a spin-cluster. The PELDOR signal, however, does not only contain the desired dipolar coupling between the spin-labels of the molecule or cluster under study. In samples of finite concentration the dipolar coupling between the spin-labels of the randomly distributed molecules or spin-clusters also contributes significantly. In homogeneous frozen solutions or lipid vesicle membranes this second contribution can be considered to be an exponential or stretched exponential decay, respectively. In this study, it is shown that this assumption is not valid in detergent micelles. Spin-labeled fatty acids that are randomly partitioned into different detergent micelles give rise to PELDOR time traces which clearly deviate from stretched exponential decays. As a main conclusion a PELDOR signal deviating from a stretched exponential decay does not necessarily prove the observation of specific distance information on the molecule or cluster. These results are important for the interpretation of PELDOR experiments on membrane proteins or lipophilic peptides solubilized in detergent micelles or small vesicles, which often do not show pronounced dipolar oscillations in their time traces.
In the third part, PELDOR has been utilized to study the structural flexibility of the Toc34 GTPase homodimer, a preprotein receptor of the translocon of the outer envelope of chloroplasts (TOC). Toc34 belongs to GAD subfamily of G-proteins that are regulated and activated by nucleotide-dependent dimerization. However, the function of Toc34 dimerization is not yet fully understood. Previous structural investigations of the Toc34 dimer yielded only marginal structural changes in response to different nucleotide loads. PELDOR revealed a nucleotide-dependent transition of the dimer flexibility from a tight GDP to a flexible GTP-loaded state. Substrate-binding stabilizes the dimer in the transition state mimicked by GDP-AlFx, but induces an opening in the GDP or GTP-loaded state. Thus, the structural dynamics of bona fide GTPases induced by GTP hydrolysis is replaced by substrate-dependent dimer flexibility, which represents the regulatory mode for dimerizing GTPases.
In the fourth part of the thesis, conformational flexibility and relative orientation of the N-terminal POTRA domains of a cyanobacterial Omp85 from Anabaena sp. PCC 7120, a key component of the outer membrane protein assembly machinery, were investigated by PELDOR spectroscopy. Membrane proteins of the Omp85-TpsB superfamily are composed of a C-terminal β-barrel and a different number of N-terminal POTRA domains, three in the case of cyanobacterial Omp85. It has been suggested that the N-terminal POTRA domains (P1 and P2) might have functions in substrate recognition. Molecular dynamics (MD) simulations predicted a fixed orientation for P2 and P3 and a flexible hinge between P1 and P2. The PELDOR distances measured between the P2 and P3 POTRA domains are in good agreement with the structure determined by X-ray, and compatible with the MD simulations suggesting a fixed orientation between these domains. PELDOR constraints between the P1 and P2 POTRA domains imply a rather rigid structure with a slightly different relative orientation of these domains compared with the X-ray structure. Moreover, the large mobility predicted from MD is not observed in the frozen solution. The PELDOR results further highlight the restricted relative orientation of the POTRA domains of the Omp85-TpsB proteins as a conserved characteristic feature that might be important for the processive sliding of the unfolded substrate towards the membrane.
Ziel dieser Arbeit war es erstmals durch eine Kombination aus chemischer Mutagenese und gezielter genetischer Modifikation (hier: „metabolic engineering“) einen Phaffia-Stamm herzustellen, welcher über die Mutagenese hinaus über eine weiter verstärkte Astaxanthin-Synthese verfügt.
Die von „DSM Nutritional Products“ bereitgestellten chemischen Mutanten wurden analysiert und über einen Selektionsprozess auf Pigmentstabilität und Wachstum hin optimiert, da die Stämme aus cryogenisierter Dauerkultur starke Pigmentinstabilitäten und ein verzögertes Wachstum aufwiesen.
Über eine exploratorische Phase wurde die Carotinoidsynthese analysiert und festgestellt, dass in den Mutanten keine Einzelreaktionen betroffen sind, welche für die Heraufregulierung der Carotinoidsynthese in den Mutanten verantwortlich sind. Hierbei wurden Limitierungen identifiziert und diese durch Transformation von Expressionsplasmiden mit geeigneten Genen aufgehoben, um damit eine noch effizientere Metabolisierung von Astaxanthin-Vorstufen hin zu Astaxanthin zu erreichen. Eine Überexpression der Phytoensynthase/Lycopinzyklase crtYB resultierte in einem gesteigerten Carotinoidgehalt bei gleichbleibendem Astaxanthin- Anteil. Durch eine zweite Transformation mit einer Expressionskassette für die Astaxanthin-Synthase asy konnte der Carotinoidgehalt weiter gesteigert und zusätzlich eine Limitierung der Metabolisierung von Astaxanthin-Vorstufen behoben werden, sodass die Transformante nahezu alle Intermediate der Astaxanthinsynthese zu Astaxanthin metabolisieren konnte (Gassel et al. 2013). Es konnte gezeigt werden, dass auch in den Mutanten, aus Experimenten mit dem Wildtyp bekannte, Limitierungen identifiziert und ausgeglichen werden konnten.
Savanna regions in West Africa are valuable cultural landscapes and provide a wide range of ecosystem services for human well-being and are frequently affected by human-induced disturbances. Aside from agricultural activities (crop production and animal husbandry), the harvesting of timber and non-timber forest products is crucial for household income, alimentation and medicinal purposes. Most indigenous woody species have undergone increasing anthropogenic pressure as social and economic conditions have changed dramatically during recent decades, resulting in further habitat fragmentation and increased disturbance severity. Human land use activities influence growth conditions for plants by altering various abiotic factors, such as light, nutrient availability and water supply. They are found to alter demographic parameters (e.g., germination, seedling and sapling growth, survival and mortality rates) of woody plant individuals and alter the structure and stability of populations. The degree of anthropogenic disturbance varies between land-cover types, distance to settlements, and protection status. In the context of land-use change, there is an urgent need to better understand and evaluate the impact of land-use on savanna vegetation, particularly on the population biology of common savanna woody species. A major conclusion to be drawn from this thesis is that land use influences savanna vegetation in a complex way and does not necessarily lead to a decline or loss of tree populations and species. It is rather that in a constantly changing landscape, as a result of human-induced disturbances, populations of ubiquitous and some common species can be stable over time. The abundance of some species tends to decline consistently, whereas others benefit from human disturbance. Moreover, the study provides an insight into the structure and dynamics of common, dominant and less dominant savanna woody plants in a communal and a protected area. There is a need for further basic studies to assess the impact of land use and ecological preferences of all species, including repeated density studies that look at survivorship and transition probabilities over a number of seasons as well as longterm in-situ experiments in settlement areas in order to better understand woody plant populations in settlement areas as the few remaining semi-natural sites are likely to decrease in the future. A challenge will be the development of strategies to protect species within a landscape under cultivation.
Die vorliegende, publikationsbasierte Dissertation, bestehend aus den drei Einzelpublikationen Bayer (2011, 2012) und Bayer und Schönhofer (2012), verfolgte das Ziel, die Spinnenfamilie Psechridae zu revidieren. Weiterhin sollten die phylogenetische Position dieser Familie im System der höheren Webspinnen (Araneomorphae) sowie die phylogenetischen Beziehungen der einzelnen Arten innerhalb der beiden Gattungen der Psechridae untersucht werden. In Form von morphologisch-taxonomischen Bearbeitungen wurden die beiden die Psechridae bildenden Gattungen Psechrus und Fecenia revidiert, wobei sämtliches Typus-Material sowie reichhaltiges, weiteres Material eingehend beschrieben, illustriert und diagnostiziert wurde. Hierbei wurden auch intraspezifische Variabilität sowie die Prä-Epigynen subadulter Weibchen, die in taxonomischen Arbeiten bislang nur eine unwesentliche Rolle gespielt haben, beschrieben, illustriert und taxonomisch ausgewertet. Zudem wurden im Rahmen dieser Untersuchungen bereits Überlegungen über mögliche Verwandtschaftsbeziehungen innerhalb der beiden Gattungen angestellt. ...
Paradoxer Schlaf als Parameter zur Messung der Stressbelastung bei Giraffen (Giraffa camelopardalis)
(2012)
Das Wohlbefinden von Tieren zu schützen ist im Grundgesetz der Bundesrepublik Deutschland festgeschrieben. Das Wohlbefinden eines Tieres wissenschaftlich zu bewerten ist jedoch eine bislang ungelöste Herausforderung. Die Biologie nähert sich dem Problem, subjektive Empfindungen eines Tieres objektiv darzustellen, vorrangig über die Messung der Stressbelastung.
Die Stressantwort eines Organismus setzt sich allgemein aus einer Kombination von vier Systemen zusammen: einer Verhaltensreaktion, einer Antwort des vegetativen Nervensystems, einer neuroendokrinen Antwort und einer Immunantwort. Der in Zoos am häufigsten untersuchte Parameter zur Messung der Stressbelastung ist die Analyse der Cortisolmetaboliten-Konzentration im Kot der Tiere. Da jedoch nicht in jeder Stresssituation das „Stresshormon“ Cortisol ausgeschüttet wird, ist es für eine exakte Bewertung der Stressbelastung notwendig, weitere Systeme der Stressantwort wie beispielsweise das Verhalten zu erfassen. Die Chronoethologie verfolgt diesen Ansatz, indem sie Änderungen des Zeitmusters im Verhalten eines Tieres als Antwort auf Veränderungen in der Umwelt oder eines endogenen Faktors erfasst und diese nach Kriterien der Befindlichkeit bewertet. Hier könnte zukünftig das Schlafverhalten eine herausragende Stellung einnehmen, da es von allen vier Stressantwortsystemen beeinflusst wird. Zudem wird aus der medizinischen Schlafforschung berichtet, dass sich insbesondere die Dauer, die ein Organismus im Paradoxen Schlaf (PS) verbringt, durch Stress verändert. Dennoch fand das Schlafverhalten zur Messung der Stressbelastung bei Zoo- und Wildtieren bislang kaum Beachtung. Ziel dieser Arbeit war es daher, die Anwendbarkeit des PS als Parameter zur Messung der Stressbelastung bei Zoo- und Wildtieren zu erforschen, um letztlich die Beurteilung des Wohlbefindens von Tieren weiter zu objektivieren. Aufgrund ihrer einzigartigen Schlafstellung während des PS sowie ihrer hohen Sensibilität gegenüber Umweltveränderungen wurde die Giraffe (Giraffa camelopardalis) als Modelltier für diesen non-invasiven Forschungsansatz gewählt.
Im Rahmen der Arbeit wurde in 645 Nächten das Schlafverhalten von 17 Giraffen unterschiedlichen Alters und Geschlechts beobachtet und analysiert. Um stressbedingte Veränderungen im PS-Muster erkennen zu können, wurden die Giraffen zunächst unter „Normalbedingungen“ beobachtet, um hieraus Referenzwerte zu generieren. Anschließend wurden unterschiedliche als stressintensiv einzustufende Situationen wie Nahrungsmangel, Transport, Veränderungen in der Herdenstruktur, Auswirkungen einer Geburt auf das Muttertier sowie verschiedene singuläre Ereignisse hinsichtlich ihrer Auswirkungen auf das PS-Muster der Giraffen untersucht und den Referenzwerten gegenübergestellt. Um die Methode der Schlafbeobachtung als Parameter der Stressbelastung zu validieren, wurde zusätzlich ein bei Wiederkäuern etablierter, bereits genannter Stress-Parameter eingesetzt: die Messung der Cortisolmetaboliten-Konzentration im Kot mit Hilfe eines Enzymimmunoassays. Diese Methode wurde hier erstmalig an Giraffen angewendet.
Durchschnittlich hielt eine Giraffe unter Normalbedingungen 27 Minuten pro Nacht paradoxen Schlaf. Dabei war die nächtliche PS-Dauer in hohem Maße vom Alter abhängig. Während juvenile Giraffen im Mittel 63 Minuten PS pro Nacht aufwiesen, verbrachten gealterte Giraffen nur 4,5 Minuten pro Nacht in der PS-Stellung. Infolge eines Stressors veränderte sich die PS-Dauer der Tiere: So zeigten alle vier transportierten Giraffen in den ersten Nächten nach ihrem Transport keinen PS oder stark reduzierte PS-Zeiten. Parallel erhöhte sich nach dem Transport die Cortisolmetaboliten-Konzentration im Kot aller Giraffen für mehrere Tage. Auch die untersuchten Veränderungen in der Herdenstruktur hatten in den meisten Fällen signifikante Veränderungen der PS-Dauer zur Folge. Die stärkste im Rahmen dieser Arbeit beobachtete Veränderung des Schlafverhaltens bewirkte der Tod eines Giraffenbullen: Die adulte Giraffenkuh hielt in der Folge für eine Dauer von 21 Tagen keinen paradoxen Schlaf mehr. Ihre Cortisolmetaboliten-Konzentration im Kot stieg nach dem Tod des Bullen hingegen nicht an. Die beobachteten Giraffenmütter zeigten nach der Geburt ihrer jeweiligen Jungtiere ebenfalls eine reduzierte PS-Dauer. Hingegen hatten neugeborene Giraffen, die an Nahrungsmangel litten und innerhalb weniger Tage verstarben, eine höchst signifikant längere PS-Dauer als gleichalte Jungtiere, die überlebten.
Während bei Nahrungsknappheit eine erhöhte PS-Dauer helfen kann Energie zu sparen, ist eine Reduktion der PS-Dauer als Resultat erhöhter Aufmerksamkeit zu interpretieren, wie sie im Zuge der Feindvermeidung in Stress-Situationen sinnvoll ist.
Zusammenfassend lässt sich feststellen, dass die PS-Dauer im Gegensatz zur Cortisolmetaboliten-Konzentration von allen beobachteten Stressoren beeinflusst wurde. Dabei veränderte sich die PS-Dauer in Abhängigkeit des jeweiligen Stressors graduell unterschiedlich, was Rückschlüsse auf die Intensität des Stressors ermöglicht.
Der PS ist infolge dieser Ergebnisse hervorragend als Parameter zur Messung der Stressbelastung bei Giraffen geeignet. Die Analyse des PS kann dabei helfen, die Auswirkungen von subjektiv als stressintensiv oder stressarm eingestuften Situationen auf das Wohlbefinden eines Tieres objektiv zu bewerten. Darüber hinaus ermöglicht die kontinuierliche Überwachung des PS-Musters, z.B. mit Hilfe moderner Videosoftware, Beeinträchtigungen des Wohlbefindens, wie sie beispielsweise durch Unterernährung, Verletzung oder Krankheit hervorgerufen werden, frühzeitig zu erkennen, was ein zeitnahes Eingreifen zum Wohle des Tieres möglich macht.
The ongoing debate on deforestation in the tropics usually points out agriculture and logging as the main causes. The two activities are often linked and the trails created by logging com-panies with their heavy machines are afterwards used by farmers to penetrate deep into the forest and cultivate. Shifting cultivation is a widespread agricultural practice in the tropics and its sustainability is often a matter of controversy. It is necessary to investigate forest recovery after shifting cultivation, analyze its succession stages for comparison with regeneration after natural disturbance, and evaluate its role for discussing the hazards of deforestation.
Background: In sequencing the genomes of two Xenorhabdus species, we encountered a large number of sequence repeats and assembly anomalies that stalled finishing efforts. This included a stretch of about 12 Kb that is over 99.9% identical between the plasmid and chromosome of X. nematophila.
Results: Whole genome restriction maps of the sequenced strains were produced through optical mapping technology. These maps allowed rapid resolution of sequence assembly problems, permitted closing of the genome, and allowed correction of a large inversion in a genome assembly that we had considered finished.
Conclusion: Our experience suggests that routine use of optical mapping in bacterial genome sequence finishing is warranted. When combined with data produced through 454 sequencing, an optical map can rapidly and inexpensively generate an ordered and oriented set of contigs to produce a nearly complete genome sequence assembly.