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Das alpha-Toxin (Hla) von Staphylococcus aureus (S. aureus) spielt eine bedeutende Rolle bei S. aureus-induzierten Pneumonien. Hla bindet zunächst als Monomer an die Plasmamembran eukaryotischer Wirtszellen und assoziiert sich zu heptameren Transmembranporen. Die Sensitivität gegenüber dem Toxin ist bei verschiedenen Atemwegsepithelzelllinien unterschiedlich ausgeprägt. Die Gründe dafür sind bis jetzt nicht vollends verstanden. Mögliche Faktoren, die einen Einfluss auf die Hla-Sensitivität der Zellen haben, könnten die Rezeptordichte und Effizienz der Porenbildung sowie die Entsorgung von Poren aus der PM durch Internalisierung und Degradation (lysosomal, proteasomal) oder durch Ausschleusung von extrazellulären Vesikeln in den Extrazellularraum sein.
Ziel dieser Arbeit war es, die Bedeutung der Faktoren, die einen Einfluss auf die Toxin-Sensitivität von Wirtszellen haben könnten, am Beispiel der drei Atemwegs-Modellzelllinien 16HBE14o-, S9 sowie A549 genauer zu untersuchen.
Dabei konnte gezeigt werden, dass die Menge an rHla, allem voran die Abundanz der Heptamere in der Plasmamembran der Zellen, einen starken Einfluss auf die Toxinsensitivität (gemessen an der Rate parazellulärer Lückenbildung in den Zellverbänden) der Zelllinien hat. Diese Ergebnisse korrelierten am besten mit der Häufigkeit des potenziellen Hla-Rezeptors ADAM10 in der Plasmamembran der drei Zelltypen, aber auch das Phospholipid Sphingomyelin scheint ebenfalls einen Einfluss auf die Hla-Sensitivität der Zellen zu haben. Die Zellgröße, der für die Hla-Vorpore stabilisierende Faktor Caveolin-1, Integrin α5β1 als weiterer möglicher Hla-Rezeptor und die Lipide Phosphatidylcholin/-serin zeigten dagegen keine Korrelation zur Hla-Sensitivität der drei Atemwegsepithelzelllinien. Das Lipid Phosphatidylethanolamin wies zwar das gleiche Muster wie das des Sphingomyelins bei den Zelllinien auf, jedoch muss eine mögliche Bedeutung des Lipids in der Hla-Bindung und/oder -Heptamerisierung erst noch untersucht werden.
Untersuchungen der Internalisierung des Toxins zeigten, dass von den drei Atemwegsepithelzelllinien nur die S9-Zellen in der Lage waren die rHla-Heptamere effizient zu internalisieren. Dabei konnte unter Verwendung der rHla-Mutante rH35L, die keine Transmembranpore ausbilden kann, gezeigt werden, dass die Internalisierung der Toxin-Heptamere wahrscheinlich Poren-unabhängig geschieht. Durch die Überprüfung des rHla-Abbaus in S9-Zellen nach Inhibierung der lysosomalen oder proteasomalen Proteindegradation konnte ein Abbau des Toxins über das Proteasom ausgeschlossen werden. Dagegen scheint der lysosomale Weg von entscheidender Bedeutung für die Hla-Heptamer-Degradation zu sein. Eine saure Hydrolyse der Protease-resistenten Toxin-Heptamere in rHla-Monomere konnte allerdings nicht nachgewiesen werden und scheint somit bei dem lysosomalen Abbau keine Rolle zu spielen. Präparierte extrazelluläre Vesikel von rHla-behandelten S9-Zellen zeigten zudem, dass eine Entsorgung des Toxins über Exosomen und/oder Mikrovesikel ebenfalls bei diesen Zellen möglich zu sein scheint. Der primäre Weg der Hla-Prozessierung ist bei den S9-Zellen dennoch der lysosomale Abbau.
Unstable environments and habitats changing due to climate change force individuals to either respond by genetic adaptation, phenotypic plasticity or by dispersal to suitable environments. Theodoxus fluviatilis (Linneaus, 1758) is a good study organisms when researching phenotypic plasticity and genetic adaptation as it naturally appears in freshwater (FW) as well as brackish water (BW) and thus inhabits a wide range of environmental salinities (0-18‰). It is a euryhaline snail that can be found in shallow waters with stony ground or on Fucus spp. and has formed regional subgroups. The brackish water and the freshwater subgroups are spatially separated and the species cannot be found in areas inbetween, e.g. estuaries.
The species shows great variability in shell patterning and shell size and there is still debate whether the subgroups are distinguishable by these traits or not. The mitochdrial RNA marker cytochrome c subunit I did not show differences between the subgroups indicating that they must be closely related, but salinity tolerance has been observed to be higher in BW snails. This might be caused by the different protein expression patterns and osmolyte accumulation (measured as ninhydrin-positive substances) observed in this species in previous studies. The exact mechanisms regulating protein expression and osmolyte accumulation, however, are not fully understood yet.
Data collected for this thesis shows differences in shell size and suggests a less strict grouping of FW and BW individuals as shell sizes of one FW site are more similar to BW individuals than the other FW ones. A better salinity tolerance towards high salinities and a higher physiological salinity limit of BW snails was confirmed and extended by demonstrating an expanded tolerance range through slow acclimation to challenging salinities in snails from both subgroups. This was achieved by a shift in the slope of their reaction norms that was much more pronounced in BW snails than FW ones. S3 individuals showed a shift similar to that of BW individuals. The data for the salinity tolerance indicates that the underlying mechanism for these tolerances are a combination of phenotypic plasticity and genetic adaptation. Despite an acclimation and shift in the slope of the reaction norms and therefore an increased tolerance towards high salinities (plasticity) FW individuals from two collection sites were not able to cope with salinities as high as BW individuals (local adaptation). The general ability to mobilise free amino acids (FAA) as organic osmolytes was not the reason for this tolerance difference. Individuals from BW and FW sites were capable of accumulating quantities of FAAs equally well. Proline, alanine and urea were the most important components of the accumulated cocktail of organic osmolytes. Even though the total amount of FAAs accumulated under hyperosmotic conditions was the same in both subgroups, there were differences in the metabolic pathways involved in osmolyte accumulation in the foot muscle. The data indicates that the hydrolysis of storage proteins and the synthesis of proline and alanine are the main processes to avoid detrimental body volume shrinkage in T. fluviatilis. While FW individuals seemed to rely on the degradation of proteins and synthesis of alanine, BW individuals depended on newly synthesising proline and alanine and accumulating urea as a side product of transamination. The accumulation of urea is a new finding in aquatic living snails and has not been reported as a mechanism to avoid cell volume shrinkage in these animals.
Differing protein expression patterns were observed under control conditions across all collection sites. 9 spots showed volume changes in BW snails opposite to those of FW snails from collection sites S1 and S2. For 6 of those spots, S3 individuals showed patterns similar to those of BW individuals and for the remaining 3 they showed patterns similar to those of FW animals. The patterns observed when exposing snails to hypo- or hyperosmotic stress were not conclusive in relation to pinpointing individual spots that show the same pattern in all collection sites, but revealed the heterogeneity of protein expression in snails from the different collection sites and in the process of osmoregulation. It also showed the general tendency of protein reduction when snails where under osmotic stress of either kind (hypo- or hyperosmotic), which supports the hypothesis of storage protein degradation.
The investigation of an ANP-receptor showed two variations of the encoding sequence expressed in T. fluviatilis. S3 individuals as well as BW individuals were found to express one type, while FW individuals, with the exception of one sample expressed the other type. This showed that the FW subgroup of T. fluviatilis seems to be more heterogeneous than the BW subgroup, but also raises the question of the dispersal history of this species. The collected data indicates that T. fluviatilis individuals are firstly capable of surviving the acidity of a duck's gizzard and secondly can tolerate acute salinity changes to 16‰ when introduced into a new environment. Hence, if snails from the FW were to be transported to waters with a salinity of up to 16‰ by man, bird, drifting plants or some other means of transport, they would most likely survive and possibly be able to thrive and spread.