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The goal of this thesis was to gain further insight into the binding behavior of ligands in the heptahelical domain (HD) of group I metabotropic glutamate receptors (mGluRs). This was realized by the establishment of strategies for the detection and optimization of molecules acting as non-competitive antagonists of group I mGluRs (mGluR1/5). These strategies should guarantee high diversity in the retrieved chemotypes of the detected compounds not resembling original reference molecules (“scaffold-hopping”). The detection of new scaffolds, in turn, was divided into two approaches: First the development of pharmacological assays to screen compounds at a certain target for bioactivity (here: affinity towards the allosteric recognition site of mGluR1 and mGluR5), and second the evaluation of computer assisted methods for the identification of virtual hits to be screened afterwards on the pharmacological assays established before. Promising molecules should be optimized with respect to activity/affinity and selectivity, their binding mode investigated and, finally, compared to existing lead compounds. Initially, membrane based binding assays for the HD of mGlu1 and mGlu5 receptors with enhanced throughput (shifting from 24-well plates to 96-well plates) were set up. For the mGluR1 assay the potent antagonist EMQMCM exhibited high affinity towards the binding site (Ki ~3nM), which is in accordance with published data from Mabire et al. (functional IC50 3nM). For mGluR5 the reference antagonist MPEP binds with high affinity to the receptor (binding IC50 13.8nM), which confirmed earlier findings from Anderson et al. (binding IC50 15nM). In another series of experiments the properties of rat cerebellar (mGluR1) and corticalmembranes (mGluR5) as well as of radiotracers were investigated by means of binding saturation studies and kinetic experiments. Furthermore, the influence of the solvent DMSO, necessary for compound screening of lipophilic substances, on positive and negative controls was evaluated. As the precise architecture of the HD of mGluR1 is still not known our efforts in identifying new ligands for this receptor focused on the ligand-based approach. All computer assisted methods that were applied to virtually screen large compound collections and to retrieve potential hits (“activity-enriched subsets”) acting at the heptahelical domain of mGluR1 relied on the existence of a valid dataset of reference molecules. This was realized by an initial compilation of a mGluR reference data collection comprising in total 357 entries predominantly negative but also some positive allosteric modulators for mGluR1 and mGluR5. In the next step a pharmacophore model for non-competitive mGluR1 antagonists was constructed. It was based upon six selective, potent and structurally diverse ligands. Prospective virtual screening was performed using the CATS atom-pair descriptor. The Asinex Gold-Collection was screened for each seed compound and some of the most similar compounds (according to the CATS descriptor) were ordered and tested forbinding affinity and functional activity at mGluR1. A high hit rate of approximately 26% (IC50 < 15 micro M) was yielded confirming the applicability of this method. One compound exerted functional activity below one micro molar (IC50-value of C-07:362nM ± 0.03). Moreover, non-linear principal component analysis was employed. Again the Asinex vendor database served as test database and was filtered by the pharmacophore model for mGluR1 established before. Test molecules that were adjacently located with mGluR1 antagonist references were selected. 15 compounds were tested on mGluR1 in binding and functional assays and three of them exhibited functional activity (IC50) below 15 micro M. The most potent molecule P-06 revealed an IC50-value of 1.11 micro M (± 0.41). The COBRA database comprising 5,376 structurally diverse bioactive molecules affecting various targets was encoded with the CATS descriptor and used for training two selforganizing maps (SOM). The encoded mGluR reference data collection was projected onto this map according to the SOM algorithm. This projection allowed to clearly distinguish between antagonists of mGluR1 and mGluR5 subtype. 28 compounds were ordered and tested on activity and affinity for mGluR1. They exhibited functional activity down to the sub-micro molar range (IC50-value of S-08: 744nM ± 0.29) yielding a final hit rate of 46% (<15 micro M). Then, the Asinex collection was screened using the SOM approach. For a predicted target panel including the muscarinic mACh (M1) receptor, the histamine H1-receptor and the dopamine D2/D3 receptors, the tested mGluR ligands exhibited the calculated binding pattern. This virtual screening concept might provide a basis for early recognition of potential sideeffects in lead discovery. We superimposed a set of 39 quinoline derivatives as non-competitive mGluR1 antagonists that were recently published by Mabire and co-workers. A CoMFA model (QSAR) was established and the influence of several side chains on functional activity was investigated. The coumarine derivative C-07 was obtained as a result of similarity searching. Starting from this compound a series of chemical derivatives was synthesized. This led to the discovery of potent (B-28, IC50: 58nM ± 0.008; Ki: 293nM ± 0.022) and selective (rmGluR5 IC50: 28.6 micro M) mGluR1 antagonists. From a homology model of mGluR1 we derived a potential binding mode for coumarines within the allosteric transmembrane region. Potential interacting patterns with amino acids were proposed considering the difference of the binding pockets between rat and human receptors. The proposed binding modes for quinolines (here:EMQMCM) and coumarines (here:B-04) were compared and discussed considering in particular the influence on activity of several side chains of quinolines obtained from the QSAR studies. The present studies demonstrated the applicability of ligand-based virtual screening for non-competitive antagonists of a G-protein coupled receptor, resulting in novel, potent and selective agents.
1. Halobacillus halophilus akkumuliert zum Ausgleich geringer, extrazellulärer Wasserpotentiale kompatible Solute. Bei Anzuchten in Gegenwart von 0,4 – 1,5 M NaCl wurden Glutamin und Glutamat als die dominierenden kompatiblen Solute identifiziert, während zwischen 2,0 und 3,0 M NaCl Prolin das dominierende Solut darstellt. Außerdem wurde Ectoin als zweites kompatibles Solut gefunden, das spezifisch bei hohen Salzgehalten akumuliert wird. Die Konzentrationen während der exponentiellen Wachstumsphase war jedoch um den Faktor 6 – 7 geringer im Vergleich zu Prolin. 2. Aus Wachstumsexperimenten in Gegenwart unterschiedlicher Anionen war bekannt, dass Glutamat, im Gegensatz zu Gluconat und Nitrat, in der Lage ist, das Wachstum von H. halophilus auch in Abwesenheit von Chlorid zu ermöglichen. Um der Frage nachzugehen, ob die wachstumsfördernde Wirkung von unphysiologisch hohen Glutamat-Konzentrationen im Medium auf die Verwendung von Glutamat als kompatiblem Solut in den Zellen zurückzuführen ist, wurden Gesamtsolutepools von Chlorid-, Nitrat-, Gluconat- und Glutamat-gezogenen Zellen gemessen. In NaCl-gezogenen Zellen zeigte sich Glutamat als dominantes Solut, während Prolin und Glutamin einen geringeren Teil am Gesamtpool ausmachten. In Nitrat-gezogenen Zellen betrug der Gesamtpool nur noch 83% und in Gluconat-gezogenen Zellen nur noch 27% im Vergleich zu Chlorid-gezogenen Zellen. Zellen, die mit Glutamat gezogen wurden, zeigten jedoch eine Gesamtkonzentration an Soluten, die ca. 100% über dem Vergleichswert aus Chlorid-gezogenen Zellen lag. Die Konzentration an Glutamin in den Zellen stieg dabei um 168%, die Konzentration an Glutamat sogar um 299%. Die Prolinkonzentration verringerte sich um 32%. Diese Daten belegen, dass der wachstumsstimulierende Effekt von Glutamat auf die Verwendung als kompatibles Solut zurückzuführen ist. 3. Zur Untersuchung der molekularen Grundlage der Salzadaptation sowie der Abhängigkeit von Chlorid in H. halophilus wurde in Zusammenarbeit mit der Gruppe von Prof. D. Oesterhelt (MPI für Biochemie, Martinsried) die Sequenzierung des Genoms begonnen. Das Projekt ist zur Zeit noch nicht abgeschlossen und befindet sich in der „Lückenschluß-Phase“. Die bisherigen Sequenzdaten konnten dennoch für die in dieser Arbeit beschriebenen Untersuchungen herangezogen werden. Das Genom besitzt eine Größe von ca. 4,1 Mbp mit einem ungefähren GC-Gehalt von 40%. Außerdem wurden 2 Plasmide identifiziert mit einer Größe von 16047 und 3329 bp. 4. Die Schlüsselgene bekannter Biosynthesewege für Glutamin und Glutamat konnten identifiziert werden. Darunter befinden sich zwei Isogene für eine Glutamatdehydrogenase (gdh1 und gdh2), ein Gen für die große Untereinheit einer Glutamatsynthase (gltA), zwei Gene für die kleine Untereinheit einer Glutamat-Synthase (gltB1 und gltB2) und zwei Isogene für eine Glutaminsynthetase (glnA1 und glnA2). glnA1 befindet sich in einem Cluster zusammen mit einem Gen, das für einen Regulator kodiert (glnR), wie er auch aus B. subtilis bekannt ist. Über reverse Transkription von mRNA und anschließender PCR-Analyse konnte gezeigt werden, dass sowohl gltA/gltB1 als auch glnA1/glnR in einem Operon organisiert sind. 5. Wurde die Transkriptmenge der in Punkt 4 erwähnten Biosynthesegene in Zellen quantifiziert, die in Gegenwart unterschiedlicher Salzkonzentrationen (0,4 – 3,0 M NaCl) gezogen wurden, so zeigte sich keine Abhängigkeit von der Salzkonzentration für die Gene gltA, glnA1 und gdh1. Über die Transkriptmengen von gdh2 ließ sich keine abschließende Aussage treffen, da die gefundenen Transkriptmengen sehr gering waren und daher zu sehr großen Varianzen bei der Quantifizierung führten. Eine klare Abhängigkeit der Transkriptmenge von der im Medium zugesetzten Salzkonzentration konnte für glnA2 gezeigt werden. Die glnA2 mRNA-Menge stieg dabei mit steigender Salzkonzentration an und erreichte bei 1,5 – 2.0 M NaCl ein Maximum. Bei diesen Salzkonzentrationen war die Menge an mRNA ca. 4 mal höher als der Vergleichswert bei 0,4 M NaCl. Bei höhern Salzkonzentrationen sank die Menge an Transkript wieder leicht und war dann ca. nur noch 3 mal so hoch wie bei 0,4 M NaCl. 6. Die zelluläre Konzentration der glnA2-Transkripte in Abhängigkeit unterschiedlicher Anionen im Anzuchtmedium wurde untersucht. Die Quantifizierung der glnA2–mRNA ergab eine 2 mal höhere Transkriptmenge in Gegenwart von Chlorid verglichen mit Nitrat oder Gluconat. 7. Es wurde nach Enzymaktivitäten der bekannten Schlüsselenzyme im Glutamat und Glutamin-Biosyntheseweg gesucht. Eine Glutamatdehydrogenase und eine Glutamatsynthase – Aktivität konnte nicht oder nur in vernachlässigbarem Maße nachgewiesen werden. Im Gegensatz dazu konnt eine Glutaminsynthetase – Aktivität eindeutig belegt werden. Diese Aktivität erwies sich abhängig von der Art und der Konzentration des angebotenen Anions im Medium. Maximale Aktivitäten wurden mit NaCl in einer Konzentration von 2,5 – 3,0 M erreicht. Interessanterweise erwies sich die Glutaminsynthetase – Aktivität auch abhängig von der Art des im Testpuffers verwendeten Anions. Hier zeigte sich eine deutliche Stimulierung der Aktivität durch das Anion Chlorid. [Die für diesen Punkt zugrunde liegenden Daten wurden im Rahmen einer von mir mitbetreuten Diplomarbeit von Jasmin F. Sydow erhoben und sind aus Gründen der vollständigen Darstellung des Projektverlaufes mitaufgeführt!] 8. Wie im Punkt 1 dargelegt, wird Prolin vor allem bei hohen Salzkonzentrationen in H. halophilus - Zellen akkumuliert. Neben der Abhängigkeit von der Salzkonzentration wurde außerdem die Abhängigkeit von der Wachstumsphase untersucht. Die Analyse der Prolinkonzentrationen während verschiedener Wachstumsphasen in Kulturen, die bei 1,0 bzw. 2,5 M NaCl angezogen wurden, zeigte, (i) dass die Prolinkonzentration während der frühen exponentiellen Phase ca. 2,5-fach erhöht war im Vergleich zu Niedrigsalz-Zellen, (ii) dass die Prolinkonzentration beim Übergang von der frühen in die späte exponentielle Phase dramatisch abnahm (um 64% bei 2,5 M NaCl) und dass (iii) in der stationären Phase Prolin praktisch nicht mehr nachzuweisen war. 9. Die Biosynthesegene für die Herstellung von Prolin aus Glutamat konnten im Genom von H. halophilus identifiziert werden. Es handelt sich dabei um ein Cluster von 3 Genen, die für eine putative Pyrrolin-5-carboxylatreductase (proH), eine Glutamat-5-kinase (proJ), und eine Glutamat-5-semialdehyd-dehydrogenase (proA) kodieren. Mittels reverser Transkription von mRNA und anschließenden PCR-Analysen konnte gezeigt werden, dass die drei Gene ein Operon bilden. 10. Eine Quantifizierung der Transkriptmengen der Biosynthesegene proH, proJ und proA mittels quantitativer PCR in Zellen, die bei unterschiedlichen NaCl-Konzentrationen gezogen wurden, zeigte einen deutlichen Zusammenhang zwischen der Salinität des Mediums und der Menge an Transkript. Diese war umso höher, je höher die Salinität des Mediums war. Die maximale Transkriptmenge (6-fach) wurde bei einer Salzkonzentration von 2,5 M NaCl erreicht. Bei noch höherer Salzkonzentration sank die Transkriptmenge auf die ca. 5-fache Menge des Kontrollwertes ab. 11. Um die Regulation und Dynamik der Osmoregulation unabhängig vom Wachstum untersuchen zu können, wurde ein Zellsuspensions-System für H. halophilus etabliert, bei dem eine konzentrierte Zellsuspension direkt von geringen auf hohe Salzkonzentrationen überführt wurde und bei dem die Prozesse der Transkription, Translation und Solut-Biosynthese erhalten blieben. Beispielhaft wurde dieses System an der Produktion von Prolin nach einem Salzschock von 0,8 auf 2,0 M NaCl getestet. Es zeigte sich bei der Analyse, dass sich die Transkriptmengen unmittelbar nach dem Salzschock deutlich erhöhten und bereits nach 1,5 Stunden ein Maximum erreicht wurde. Verglichen mit dem Wert zu Beginn des Versuches waren die Transkriptmengen ca. 13-fach erhöht, sanken im weiteren Verlauf jedoch wieder ab und blieben bei einer 4-fachen Transkriptmenge konstant. Mit der Erhöhung der Transkriptmenge ging auch eine Erhöhung der Prolinkonzentration einher, die ein Maximum von ca. 6 μmol/mg Protein nach 6 Stunden erreichte. Auch diese Konzentration verringerte sich im weiteren Verlauf wieder und erreichte nach 20 Stunden den Ausgangswert. 12. Um den Einfluß diverser Anionen bzw. Osmolyte im Medium auf die Produktion von Prolin zu untersuchen, wurden Zellsuspensionen von H. halophilus einer Erhöhung der Osmolarität von 0,8 M auf 2,0 M unterzogen. Es zeigte sich dabei, dass die maximale Akkumulation von Prolin in Anwesenheit von Chlorid am höchsten war. Nitrat und Glutamat führten zu ähnlichen, aber leicht geringeren maximalen Konzentrationen (92 bzw. 83% des Chloridwertes). Gluconat führte noch zu einer Akkumulation von ca. 51%, während die anderen Osmolyte zu keiner Akkumulation führten. Eine Analyse der Transkriptmengen zeigte jedoch ein völlig anderes Bild. Während Chlorid, Nitrat und Gluconat zu vergleichbaren Anstiegen der Transkripmengen führten, war die maximale Transkriptmenge der Glutamatinkubierten Zellen 3-9 mal höher als in Vergleichszellen mit Chlorid. In anschließenden Titrationsexperimenten mit verschiedenen Glutamatkonzentrationen konnte gezeigt werden, dass eine minimale Konzentration von 0,2 M Glutamat ausreichend ist, um eine 90-fache Steigerung der Transkriptmenge herbeizuführen. 13. Als Antwort auf Hochsalz-Bedingungen akkumuliert H. halophilus neben Prolin auch Ectoin. Die Ectoinkonzentration bei 2,5 M NaCl war ca. 2-3 mal höher als in Zellen, die bei 1,0 M gezogen wurden. Die Bestimmung der intrazellulären Ectoin-Konzentrationen während des Wachstums zeigte außerdem, dass die Produktion von Ectoin wachstumsphasenabhängig ist. Die Konzentration in der stationären Phase war ca. 5-fach höher als in der exponentiellen Phase. Die Entwicklung der Ectoin- Konzentration verhielt sich somit reziprok zur Entwicklung der Prolin-Konzentration während des Wachstums. 14. Es wurde ein Cluster von drei Genen im Genom von H. halophilus identifiziert, deren Genprodukte die Biosynthese von Ectoin aus Aspartatsemialdehyd katalysieren. ectA kodiert dabei für eine putative Diaminobutyrat-Acetyltransferase, ectB für eine putative Diaminobutyrat-2-oxoglutarat-Transaminase und ectC für eine putative Ectoin-Synthase. Mittels reverser Transkription von mRNA und anschließenden PCR-Analysen konnte gezeigt werden, dass die drei Gene ein Operon bilden. 15. Die Transkription der ect-Gene war abhängig von der Salinität des Mediums. Ab 2,0 M stieg die Menge an RNA um das 10-fache an und erreichte bei 3,0 M ein Maximum mit der 23,5-fachen Menge. 16. Nach einem osmotischen Schock stieg die Konzentration an ect-mRNA signifikant und erreichte ein Maximum nach 3 - 4 Stunden. Das Maximum wurde somit 1,5 – 2,5 Stunden später erreicht als bei anderen Genen der Solute-Biosynthese wie etwa gdh1, das für eine Glutamatdehydrogenase, glnA2, das für eine Glutamin-Synthetase oder proH, das für eine Pyrrolin-5-Carboxylase kodiert. Die maximal erreichten Wert lagen 13-fach (ectA), 6,5-fach (ectB) und 3-fach (ectC) über dem Wert vor dem Salzschock. Gegen EctC wurden polyklonale Antikörper generiert. Western-Blot Analysen mit diesem Antikörper zeigten, dass die EctC-Menge nach 4 Stunden um das 2,5-fache stieg, dann aber wieder abfiel auf das 1,6 – 1,7-fache des Ausgangswertes. Der Rückgang an EctC fand keine Entsprechung in der gemessenen Ectoin-Konzentration, welche über einen Zeitraum von 18 Stunden kontinuierlich anstieg. Die maximale Konzentration nach 18 Stunden betrug das ca. 6,3-fache des Ausgangswertes. 17. Wurden H. halophilus Zellen mit anderen Osmolyten außer NaCl geschockt, so ergab sich folgendes Bild der Regulation der Ectoin-Biosynthese: (i) die Transkription der ect-Gene zeigte keine Chlorid-abhängige Regulation. Die maximale Transkriptmenge wurde in Gegenwart von Nitrat erreicht, wohingegen Gluconat zu vergleichbachen mRNA-Mengen führte wie Chlorid. Glutamat führte nur zu schwacher Stimulierung der Transkription. (ii) auf Ebene der Proteinmenge war zu sehen, dass die Menge an EctC nach osmotischem Schock vergleichbar war in Zellen, die mit Chlorid oder Nitrat inkubiert wurden. Gluconat führte nur zu einer 40%-igen Zunahme während andere Osmolyte nahezu wirkungslos auf die Menge an EctC blieben. (iii) die höchste Akkumulation an Ectoin nach einer plötzlichen Erhöhung der Osmolarität wurde erreicht mit Chlorid (6-fache Zunahme) gefolgt von Nitrat (5,6-fache Zunahme). Gluconat führte lediglich zu einer 3,3-fachen und Glutamat nur noch zu einer 2-fachen Steigerung der Ectoinkonzentration. Glutamat hat somit ähnliche Effekte wie Tartrat, Saccharose oder Sulfat. Succinat führte zu keiner Akkumulation und Glycin sogar zu einer deutlichen Abnahme. Die Produktion von Ectoin ist somit hauptsächlich abhängig vom Anion/Osmolyt und nur untergeordnet von der Osmolarität.
Rhythmic changes in environmental lighting conditions have ever been the most reliable environmental cue for life on earth. Nature has therefore selected a genetically encrypted endogenous clock very early in evolution, as it provided cells and subsequently organisms with the ability to anticipate persevering periods of light and darkness. Rhythm generation within the mammalian circadian system is achieved by clock genes and their protein products. The mammalian endogenous master clock, which synchronizes the body to environmental time, is located in the suprachiasmatic nucleus (SCN) of the hypothalamus. As an integral part of the time-coding system, the pineal gland serves the need to tune the body to the temporal environment by the rhythmic nocturnal synthesis and immediate release of the hormone melatonin. In contrast to the transcriptional regulation of melatonin synthesis in rodents, a post-translational shaping is indicated in the human pineal gland. Another important mediator of circadian time and seasonality to the body is the pituitary gland. The aim of this work was to elucidate regulation of melatonin synthesis in the human pineal gland. Furthermore, presence and regulation of clock genes in the human pineal and pituitary gland, and in the SCN were analyzed. Therefore, human tissue, taken from regular autopsies, was analyzed simultaneously for different parameters involved in melatonin biosynthesis and circadian rhythm generation. Presented data demonstrate that post-mortem brain tissue can be used to detect the remnant profile of pre-mortem adaptive changes in neuronal activity. In particular, our results give strong experimental support for the idea that transcriptional mechanisms are not dominant for the generation of rhythmic melatonin synthesis in the human pineal gland. Together with data obtained for clock genes and their protein products in the pituitary, data presented here offer 1) a new working hypothesis for post-translational regulation of melatonin biosynthesis in the human pineal gland, and 2) a novel twist in the molecular competence of clock gene proteins, achieved by nucleo-cytoplasmic shuttling in neuronal and neuroendocrine human tissue. Furthermore, in this study, oscillations in abundance of clock gene proteins were demonstrated for the first time in the human SCN.
Analysis of coding principles in the olfactory system and their application in cheminformatics
(2007)
Unser Geruchssinn vermittelt uns die Wahrnehmung der chemischen Welt. Im Laufe der Evolution haben sich in unserem olfaktorischen System Mechanismen entwickelt, die wahrscheinlich optimal auf die Erfüllung dieser Aufgabe angepasst sind. Die Analyse dieser Verarbeitungsstrategien verspricht Einblicke in effiziente Algorithmen für die Kodierung und Verarbeitung chemischer Information, deren Entwicklung und Anwendung dem Kern der Chemieinformatik entspricht. In dieser Arbeit nähern wir uns der Entschlüsselung dieser Mechanismen durch die rechnerische Modellierung von funktionellen Einheiten des olfaktorischen Systems. Hierbei verfolgten wir einen interdisziplinären Ansatz, der die Gebiete der Chemie, der Neurobiologie und des maschinellen Lernens mit einbezieht.
The topic of this thesis is the functional renormalization group. We discuss some approximations schemes. Thereafter we apply these approximations to study different fields of condensed matter physics. Generally we have to evaluate an infinite set of vertex functions describing the scattering of particles. These vertex functions get renormalized away from their bare values governed by an infinite hierarchy of flow equations. We cannot expect to actually solve these equations but have to apply a couple of approximations. The aim is to somehow separate relevant contributions from irrelevant ones. One possible scheme opens up if we rescale fields and vertices. Here "relevance" is used in a quantitative way to describe the scaling behaviour of vertices close to a fixed point of the RG. One disadvantage of describing the system in terms of infinitely many vertices is that the majority of these vertices we have to evaluate are not of interest to us. In most cases we are just looking for the self-energy or the two-particle effective interaction. However there might be contributions to the flow of these vertices that are generated by irrelevant vertices. We generally assume that we can express irrelevant vertices in terms of the relevant and marginal ones. Then in turn it should be possible to write the contributions of these irrelevant vertices to the flow of relevant and marginal ones in terms of relevant and marginal vertices as well. We show how this can be achieved by what we term the adiabatic approximation. We now consider weakly interacting bosons at the critical point of Bose-Einstein condensation. As the transition takes place at a finite temperature this temperature defines an effective ultraviolet cut-off. For the investigation of physical properties that depend on momenta smaller than this cut-off it is therefore sufficient to describe the system by a classical field theory. Our central topic here is the self-energy of the bosons and we are able to evaluate it with the full momentum dependence. For small momenta it approaches a scaling form and as the momentum is gradually increased we observe a crossover to the perturbative regime. As a test for the reliability of our expression for the selfenergy we investigate the interaction induced shift of the critical. Our results compare quite satisfactory to the best available estimates for this shift. For the anomalous dimension our approach predicts the correct order of magnitude however with a considerable error. As an improvement we include more vertices into our calculations. Here we observe that our fixed point estimates indeed approach the best known results but this convergence is quite weak. We turn toward systems of interacting fermions. The formulation of the functional renormalization group implicitly requires knowledge of the true Fermi surface of the full interacting system. In general however we can just calculate it a-posteriori from the self-energy. The requirement to flow into a fixed point can be translated into a fine-tuning of the frequency/momentum independent part r_0 of the rescaled 2-point function. We show how this bare value is related to the momentum dependent effective interaction along the complete trajectory of the RG. On the other hand r_0 expresses the difference between the bare and the true Fermi surface. Putting both equations together results into an exact selfconsistency equation for the Fermi surface. We apply our self-consistency equation above to tackle the problem of finding the true Fermi surface of interacting fermions in low dimensions. The most simple non-trivial model with an inhomogeneous Fermi surface is a system of two coupled metallic chains. The process of interband backward scattering leads to a smoothing of the Fermi surface. Of special interest is if the Fermi momenta of the two bands collapse into just one value. We propose the term confinement transition for this behaviour. We bosonize the interband backward scattering by means of a Hubbard-Stratonovich transformation and treat our system as a single channel problem. This bosonization together with the adiabatic approximation allows us to investigate the system even at strong coupling. Within a simple one-loop treatment our method predicts a confinement transition at strong coupling. However taken vertex renormalizations into account we observe that this confinement is destroyed by fluctuations beyond one-loop. Actually we observe how the confined phase can be stabilized by the inclusion of interband umklapp scattering. Thereafter we consider the physically more relevant case of a two-dimensional system of infinitely many coupled metallic chains. Here the Fermi surface consists of two disconnected weakly curved sheets. We are able to repeat the calculations we have performed for our toy model. Within a self-consistent 2-loop calculation indeed signs for a confinement transition at finite coupling strength emerge.
End-stage renal disease has been denominated a vasculopathic state, owing to the accelerated arterial stiffening, which occurs in addition to and independent of atherosclerosis and bears an increased cardiovascular risk. The altered metabolic milieu in uraemia leads to an increased oxidative stress, heightened inflammatory burden, and an abnormal calcium-phosphate metabolism, which are thought to be responsible for the vascular changes. The pulse wave velocity (PWV) is a widely employed surrogate parameter of arteriosclerosis. The purpose of this study was to gain more insight into the pathogenesis of arterial stiffness, by investigating the influence of markers of oxidative stress, procoagulation, and inflammation, and of the calcium-phosphate product on the PWV. We conducted a cross-sectional study in 53 stable patients aged 59 ± 16 years, who had been on haemodialysis for at least 4 months (68 ± 48). Carotid-radial PWV was measured using a semi-automated device, Complior SP (Artech Medical, France). Advanced glycosylation end-products (AGE) and advanced oxidation protein products (AOPP), were quantified according to previously described methods. High sensitive CRP was measured using ELISA, whereas the other biochemical parameters, i.e. fibrinogen, albumin, calcium, phosphate, cholesterol, and triglycerides, were determined using routine methods. For statistical calculations we employed SPSS (Statistical Package of Social Science, 12.0, 2003). The correlations between PWV, as the dependent variable, and many dependent variables were assessed by means of multiple regression analysis, in which we controlled for the influence of the traditional cardiovascular risk factors and some of the patients’ medication (calcium-channel blockers and statins). PWV was found to be significantly correlated to serum CRP (p=0.003), LDLcholesterol (p<0.001), triglycerides (p<0.001), AGE (p=0.002), calcium (p<0.001), phosphate (p=0.001), and fibrinogen (p=0.020). Between PWV and dialysis duration (months) an interesting quadratic relationship (p=0.058) was noted. Against expectation, regression analysis showed a negative correlation between AOPP and PWV (p=0.001). We failed to confirm the correlation between PWV and age, systolic blood pressure, or heart rate. Among traditional cardiovascular risk factors only LDL-cholesterol was positively correlated to PWV. In this cross-sectional analysis we could put forward that PWV correlates positively and significantly with fibrinogen, CRP, AGEs, calcium, phosphate, and LDL-cholesterol in haemodialysis patients. It seems procoagulatory and proinflammatory pathways, oxidative stress, and the calcium-phosphate product exert a synergistic effect on disturbances of vascular architecture in ESRD patients.
Two distinct mechanisms contribute to the development of blood vessels: vasculogenesis, which is the de novo formation of vascular structures from progenitor cells, and angiogenesis, the formation of new blood vessels from pre-existing ones.
Angiogenesis is a highly ordered and carefully regulated multi-step process, during which the precise spatio-temporal interaction between endothelial and mural cells, i.e. smooth muscle cells and pericytes, is prerequisite for the formation of a functional blood vessel. The crosstalk between these two latter cell ty pes is mediated indirectly by various
secreted growth factors, and directly through cell-cell and cell-matrix interactions. The secretory epidermal growth factor-like protein 7 (EGFL7) has been implicated to
play an important role in the regulation of smooth muscle and endothelial cell recruitment and vascular tube formation. However, in-depth investigation of the underlying molecular mechanism has so far been hampered by the lack of functional recombinant EGFL7. In this study for the first time full length EGFL7 was successfully expressed as a His 6- tagged fusion protein from insect cells using the Baculovirus expression vector system. Recombinant EGFL7 was purified in a two-step protocol involving ion metal affinity chromatography and gel filtration. Furthermore, recombinant EGFL7 was
purified from human embryonic kidney EBN A 293 cells using a similar approach, allowing the production of high amounts of recombinant EGFL7 protein in its native state, with proper post-translational processing and full biological activity. Detailed analysis of the post-translational processing of recombinant EGFL7 and EGFL7-mutants revealed extensive proteolytic processing by protein convertases both at the N- and the C-terminus, the latter being prerequisite for EGFL7 secretion. Furthermore, secreted EGFL7 protein was shown to bind to the extracellular matrix and the responsible heparin-binding domain of EGFL7 was mapped to its N-terminal
portion. Purified recombinant EGFL7 protein was tested for its functionality using cell migration assays, cell proliferation studies and in vivo matrigel studies in mice. In the
modified Boyden chamber migration assay, recombinant EGFL7 proteins inhibited PDGF-BB-induced smooth muscle cell migration. Moreover, recombinant EGLF7 proteins strongly inhibited PDGF-BB-induced proliferation of smooth muscle cells, while it did not affect VEGF induced proliferation of endothelial cells. When applied in the in vivo matrigel plug assay, EGFL7 proteins induced a strong pro-angiogenic response, comparable with that of VEGF on an equimolar basis. Moreover, EGFL7 expression was strongly induced in endothelial cells in response to VEGF stimulation. These novel findings demonstrate the important function of EGFL7 in angiogenesis and are well in line with previous results. They demonstrate a cell specific action of EGFL7 on the different cell types involved in vessel formation, which is a prerequisite for a regulatory function in cell-to-cell crosstalk. Based on the results described here, the following model can be proposed: VEGF, a known strong initiator of angiogenesis, induces endothelial cell proliferation and migration, allowing the
escape from the comparatively rigid structure of a functional vessel to form an angiogenic sprout. At the same time VEGF induces the expression of EGFL7 in endothelial cells. EGFL7 is expressed, proc essed and secreted from these cells. While EGFL7 has no known effect on endothelial cells, it inhibits smooth muscle cell proliferation and migration, providing a mechanism to prevent pre-mature stabilization of the forming vessel. The availability of purified recombinant EGFL7 will be helpful in the detailed characterization of the underlying molecular mechanism of EGFL7 action, including the identification of the putative EGFL7 receptor, and will allow - together with knock-out experiments in mice - the exploration of the additional biological functions of EGFL7. Moreover, considering the strong pro-angiogenic effect of EGFL7 in vivo, it would be also of a great therapeutic interest to investigate its role in the development of tumor vasculature. The insights into these molecular mechanisms might provide a novel approach for the development of anti tumor therapies.
Aims: The purpose of this study was to evaluate the feasibility and short-term efficacy of transcatheter paravalvular leak closure using different occlusion devices. Methods and Results: Twenty one patients underwent transcatheter closure of either aortic or mitral paravalvular leak from June 2002 to February 2006 using the Amplatzer PDA, ASD or VSD occluder. All patients had symptoms and signs of haemolysis and/or cardiac decompensation with dyspnoea. Implantation of a device was technically successful in twenty patients (95 %). Immediate residual leak was found in seventeen patients (85 %). Significant shunting persisted in nine cases during follow up (45 %). Permanent leaflet obstruction was observed in one patient. Severe complications during follow up led to early death in one patient and surgical intervention in three. A successful second catheter treatment was performed in another three patients. The event-free survival from reoperation, death and stroke at the end of the observation period was 80 %. Conclusion: Transcatheter closure of paravalvular leaks is a technically feasible, but demanding procedure. Residual leaks are common and may worsen pre-existing haemolysis. Due to the significant ongoing morbidity in this group of patients and the complexity of follow up individual patient results differ considerably. Nevertheless, it is possible to achieve some symptomatic relief, thus an interventional approach should be discussed as a potential treatment option for those patients with a limited defect and who are not deemed suitable for another operation.
Koalas are popular zoo animals, but difficult in husbandry. In addition to their specialised diet of eucalyptus leaves, they are prone to “stress” and disease. Particularly in European zoos, themonitoring of theirwell-being has high priority and they are protected from possible stressors. However, stress signs in koalas are vague and monitoring techniques like weighing might result in discomfort itself. Additionally, husbandry routines are planned according to keeper’s schedule, not to the endogenous rhythms of the koalas. Therefore it is necessary to investigate activity pattern in captive koalas and the signals influencing them. These signals have to be assessed on the strength and quality of their impact. A total of 17 koalas have been observed in three zoological gardens in Australia and Europe. Koalas kept in outdoor enclosures with little human contact (Koala Walkabout, Taronga Zoo, Sydney) showed a uniform activity pattern, which was clearly entrained by light. Activity levels were higher during the night, and there was a pronounced resting period in the morning which corresponds with low body temperature measured by Degabriele and Dawson (1979). Activity peaks were related to twilight and changed during the year related to day lengths. However, there was a clear influence from the introduction of fresh browse which resulted in a distinct feeding peak in the afternoon. With short day lengths, this stimulus competed with dusk. Activity patterns from koalas in indoor enclosures (Zoo Duisburg, Vienna Zoo) varied between individuals and in some cases lacked a detectable rhythm. Though activity peaks were related to light, entrainment to sunlight was weak. In winter, koalas reacted primarily to the artificial light, but some also showed activity peaks related to sunlight. Activity patterns in these koalas were less structured and differed severely from patterns expected according to literature. Activity was often related to the keeper’s presence and food introduction. Frequency of feeding bouts was considerably higher at Vienna Zoo compared to the other zoos and the bouts were shorter in duration. Time budgets of the koalas were within the range given in free-range studies. Feeding showed seasonal changes and was increased in lactating females. Koalas at Vinna Zoo had a high level of locomotor activity compared to the size of the enclosure. Koalas at Koala Walkabout were not used to handling, so they resisted the keeper. The koalas at the two European zoos were handled regularly and settled down quickly. However, handling took place in the morning; in most koalas, there was no activity prior to it. In Vienna, resting periods were interrupted daily due to weighing. Food introduction at KoalaWalkabout took place in the afternoon. It was preceded by locomotor activity and triggered a long feeding bout in the koalas. It is not clear, whether food had true Zeitgeber properties or masked the endogenous rhythm. In the two European zoos, food was introduced in the morning. The peaks related to this were smaller than those at Koala Walkabout. Activity was rarely observed prior to food introduction. The koalas at Koala Encounter, Taronga Zoo (Sydney),were regularly confronted with visitors, though no contact was allowed. Direct observation by the keepers did rarely show any stress signs. Activity patterns at night were strikingly similar to Koala Walkabout, but differed dramatically during the day. Food was introduced three times a day, which usually resulted in activity that interrupted a resting period. Generally, the koalas at Koala Encounter were more active than those at KoalaWalkabout. They also displayed a high level of locomotor activity, especially on the ground, which is an accepted sign of discomfort in koalas (Wood 1978; Zoological Society of San Diego 2001; Yusuf& Rosenthal unpublished data). In summary, this chronoethological study of the captive koalas showed that there are several problems with koala husbandry. Artificial light regimes for koalas are not sufficient for entrainment and result in unstructured activity pattern. This is especially the case in winter, when the day in Europe is artificially extended. Due to the mainly nocturnal behaviour of koalas, such an extension might not be necessary and therefore should be avoided. Handling in Europe took place during the physiological resting time of the koalas. Interruptions of resting times are considered as stressors (Wood 1978) and should be avoided. Handling in the afternoon would be more suitable for the koalas and triggered activity in the two koalas at Vienna Zoo. It is also arguable if daily weighing is necessary to monitor health in captive koalas or if the frequent interruption of resting countervail the advantages of constant monitoring. Frequent contact with visitors, evenwithout the so-called cuddling, has a considerable impact on activity patterns and time budget of koalas, even if no immediate stress signs are displayed. Such contact should therefore be reduced to a minimum and chronoethological observations of the koalas should be used. A study on koalas with direct visitor contact is also advisable to revise the current legislation on “koala cuddling”. Koalas frequently rested in living trees if they had access to it. Since no food-poisoning has been reported from koalas using living non-food trees, the provision of living trees with an appropriate canopy should be included in the husbandry guidelines. Increased locomotor activity has been shown to be related to conditions of discomfort or stress and possibly to oestrus. This is in accordance with literature (Wood 1978; Zoological Society of San Diego 2001). Further observation, combined with hormone analysis, are advisable to establish this parameter for evaluation of well-being. Chronoethology has proven to be useful for the evaluation of husbandry conditions and group dynamics. Different to other, traditional ethologicalmethods, it indicated problems and enabled me to advise more appropriate times for handling and food introduction. It is desirable that zoos already using 24-hour video observation include chronoethological aspects into their analysis.
The rate of species extinctions due to anthropogenic activities has dramatically increased within the past few centuries (Dirzo & Raven, 2003; Novacek & Cleland, 2001). Although the mechanisms and ultimate causes leading to the extinction of species remain largely unclear (Frankham et al., 2002), five threats to global biodiversity have frequently been referred to as the most important: habitat destruction and fragmentation, global climate change, hunting and overuse of food resources, biological invasions and environmental pollution (Dudgeon et al., 2006; Lewis, 2006; Novacek & Cleland, 2001). Different research fields, as conservation biology, ecology and ecotoxicology, investigate the effects of these factors on organisms and found strong evidence for their negative impact on regional and global biodiversity.
In most cases, natural populations will be impacted not only by one threat, but rather a combination of them (Buckley & Roughgarden, 2004; Kappelle et al., 1999). Multiple environmental stress factors can have cumulative negative effects on the survival of populations (Sih et al., 2004). To understand, how natural populations respond to combinations of different stress factors is thus of crucial importance in order to understand our present and future impact on all scales of biodiversity (Warren et al., 2001).
The effects of anthropogenically introduced chemicals on organisms and ecosystems are investigated in the field of ecotoxicology. Research in this area has led to a large body of information concerning the impact of chemical stress on the fitness of model species in the laboratory. In contrast to this, there is an obvious lack of knowledge on the effects of contaminants on natural populations and communities (Bickham et al., 2000; Bourdeau et al., 1990). For instance, ecotoxicologists have just started to investigate the impact of environmental pollution on the genetic variability of natural populations (Bickham et al., 2000; Whitehead et al., 2003). Genetic variation provides the raw material for populations in order to adapt to changing environmental conditions and is thus the substrate for evolution and long-term survival of populations and species (Frankham, 2005). The amount of genetic variation in populations is positively correlated with the effective population size (Frankham, 1996). Habitat destruction and fragmentation has divided the ranges of many species into small and isolated refuges. Without migration from adjacent habitats, isolated populations will decrease in their level of genetic diversity through random loss of alleles (Hedrick, 2000). Frankham (1995) for instance, showed that 32 of the 37 endangered species (which occur in small populations per definition) of different animals and plant taxa display reduced levels of heterozygosity compared to closely related and more frequent species.
In strongly human impacted landscapes, both factors, environmental pollution and habitat destruction, can be expected to occur frequently together. It is thus of crucial importance to investigate the impact of reduced genetic diversity and inbreeding on the response to chemical stress. In addition, chemical exposure has frequently been discussed to have an impact on the extent of genetic variability in exposed populations (Guttman, 1994; Staton et al., 2001; van Straalen & Timmermans, 2002). However, evidence for this 'genetic erosion hypothesis' remained scarce to date, most likely because of the difficulty to single out the impact of pollution stress from a background of multiple factors which influence patterns of genetic variability in natural populations (Belfiore, 2001; Staton et al., 2001; van Straalen & Timmermans, 2002).
G protein-coupled receptors (GPCRs) constitute an important class of integral membrane proteins that are involved in several signaling pathways. About 50% of the currently available drugs are targeted against these receptors and high-resolution structures of these receptors will be of immense importance from the perspective of designing specific and potent drugs. However, structure determination of these receptors and of membrane proteins in general, has been a very challenging task till date. A major limitation in the structure determination of these proteins is that they are present in minute amounts in the native tissues and therefore, they must be produced heterologously. Additionally, crystallization of GPCRs is difficult owing to their flexible nature and limited hydrophilic surface area available for crystal contacts. The aim of my Ph.D. thesis work is two fold, first, to address the problem of GPCR crystallization by using a fusion protein complex approach and second, to tailor Rhodobacter sphaeroides as an expression system for the heterologous production of GPCRs. In the first approach, R. sphaeroides was used as an expression system to generate a fusion protein complex of the photosynthetic reaction center (RC) with a GPCR, expecting that such a complex would be easier to crystallize than the receptor alone. The notion behind this approach is that the RC will act as a scaffold in providing surface area to create crystal contacts and at the same time, it will also reduce the flexibility of the receptor, hopefully without perturbing the functionality of the receptor. Based on the computational modelling experiments, two ways to generate a fusion complex were assigned. Long linkers were inserted between the subunits of the RC and the GPCR. The linkers were designed with a possibility of straightforward alteration of their length as they contained a number of restriction enzyme sites. A series of these constructs were designed and expressed in R. sphaeroides deletion strain, which did not possess the chromosomal RC genes. Though most of these fusion constructs could be successfully expressed, as analyzed by western blot, majority of them were not functional in terms of ligand binding of the GPCR component of the fusion complex. Interestingly, one of these constructs, where the M subunit of RC was directly fused to the human angiotensin II type 1a receptor (AT1aR), exhibited significant functional expression. Based on saturation binding analysis using [125I] iodotyrosyl4Sar1Ile8-angiotensin II (an AT1aR subtype specific antagonist), an expression level of 40+5 pmol/mg of total membrane protein was calculated. This expression level corresponds to approximately 0.3 mg of functional receptor per liter culture and it is significantly higher than the AT1aR expression in native tissues. Additionally, the binding affinity of the recombinant receptor for its endogenous ligand angiotensin II was found to be 1±0.1 nM, which is similar to that observed for the AT1aR in native tissues. More interestingly, the RC part of the fusion complex was structurally assembled in other words, properly folded as judged by the presence of the characteristic peaks at 760 nm, 800 nm and 850 nm by absorption spectroscopy. However, a slight change in the intensity of the peak at 800 nm was observed while comparing the spectra of native RC with that in the fusion protein complex. This slight variation might be due to the change in the protein environment. The fusion protein complex RC-AT1aR was functionally solubilized and purified using a decahistidine tag fused at the c-terminus of the AT1aR. Subsequently, the monodispersity and integrity of the complex was confirmed by size exclusion chromatography, which revealed a homogeneous peak. Additionally, it was also possible to solubilize and purify this complex in the presence of a fluorescein tagged angiotensin II ligand which provides a nice tool to judge the functionality of the AT1aR and integrity of the complex at the same time. The purified RC-AT1aR fusion complex was then subjected to three-dimensional (3-D) crystallization trials and it was possible to obtain reproducible crystals of this complex. The crystals were fluorescent (as the complex was purified in presence of fluorescently labelled angiotensin II) and needle or tetragonal in shape, but produced a powdery diffraction pattern. Further attempts to improve the crystallization condition and to optimize the cryo-conditions are underway. In addition, attempts are also being made to obtain the crystals of this complex with the antagonist (e.g. losartan) bound to the receptor. In view of several limitations in the heterologous expression of GPCRs, as the second part of my Ph.D. thesis, I decided to explore the possibilities of developing a novel expression system based on R. sphaeroides for production of recombinant GPCRs. The notion behind using this host is that lack of inclusion bodies and high concentration of membranes in R. sphaeroides would result in efficient functional overexpression of recombinant membrane proteins. For this purpose, a R. sphaeroides strain, modified by the deletion of the genes encoding the RC and the light harvesting proteins LH1 and LH2, was used. The genes for RC and LHs constitute about 85-90% of total membrane proteins in a R. sphaeroides cell. These membranes are normally housed in special membrane vesicles called intracytoplasmic membranes (ICMs) that can fill almost the entire cell volume under certain growth conditions. Synthesis of a heterologous protein under the control of the moderately strong photosynthetic superoperonic promoter should be coordinated with the synthesis of new membranes to harbour these proteins, thus acting as a natural induction system. Moreover, as most of the native membrane proteins are absent in this deletion strain, heterologously produced protein should not experience a shortage of molecular chaperones for proper folding and insertion. Additionally, the absence of inclusion bodies in this host should enhance the functional and homogenous population of the recombinant proteins. Three human GPCRs, namely the adenosine A2a receptor (A2a), the angiotensin II type 1a receptor (AT1aR) and the bradykinin subtype 2 receptor (B2R) were tested for expression and functionality in this system. Two different constructs were used to determine the optimal position and ribosome-binding site (RBS) in the superoperon for the highest expression level. Of these three receptors, the AT1aR and B2R were successfully produced, while the A2aR failed to express, producing green carotenoid free R. sphaeroides mutants, for unknown reasons. For the recombinant B2R, [3H] bradykinin binding analysis revealed a low functional expression level of 0.7-0.8 pmol/mg of total membrane protein. This expression level corresponds to 0.01 mg functional receptor per liter of culture and is not sufficient for large-scale expression of this receptor. However, for the recombinant AT1aR, [125I] iodotyrosyl4Sar1Ile8- angiotensin II binding analysis revealed an expression level of 12±1 pmol/mg of total membrane protein. This expression level corresponds to approximately 0.1 mg functional receptor per liter culture and this is significantly higher than the AT1aR expression in native tissues. This expression system is still in the nascent stages of development and there are several parameters, which are still to be assessed for the optimal use of this system for the production of GPCRs and other membrane proteins. In conclusion, my Ph.D. work presents a novel fusion protein complex based approach for obtaining crystallizable GPCRs and a novel expression system for producing heterologous GPCRs. It was possible, for the first time, to produce a functional RC-GPCR complex that could easily be crystallized, though further finetuning of the system is required. R. sphaeroides based novel expression system was successfully used to produce functional human GPCRs under the control of a moderately strong photosynthetic superoperonic promoter. This expression system represents a naturally induced system where the expression of a heterologous protein is coordinated with the synthesis of new membranes to harbour the recombinant protein. The fusion protein complex approach and the expression system presented here can hopefully be used as a general method to facilitate the expression and crystallization of other membrane proteins.
The work presented in this thesis addresses a key issue of the CBM experiment at FAIR, which aims to study charm production in heavy ion collisions at energies ranging from 10 to 40 AGeV . For the first time in this kinematical range, open charm mesons will be used as a probe of the nuclear fireball. Despite of their short decay length, which is typically in the order of few 100 µm in the laboratory frame, those mesons will be identified by reconstructing their decay vertex.
The development of novel drugs targeting GPCRs is of particular interest since modulation of subfamilies of this receptor class highly influences neurotransmission in the central nervous system. This study has focused on the development of ligands for the dopamine D3 receptor. The receptor belongs to the dopamine D2-like family among the biogenic amine binding GPCRs. The dopamine D3 receptor is involved in neurological and neuropsychiatric disorders such as Parkinson’s disease, schizophrenia and drug addiction. Due to its close structural similarity to the dopamine D2 receptor subtype, it is still a challenge to identify and further optimize new leads. Therefore an in vitro screening assay, which also allows elucidating comprehensive structure-affinity relationships, is required. In this investigation the implementation and evaluation of radioligand binding assays for human dopamine D2S and dopamine D3 receptors and for the related aminergic human histamine H1 receptor stably expressed in Chinese hamster ovary (CHO) cells has been performed. Saturation binding experiments with [³H]spiperone at dopamine D2S and D3 receptors and with [³H]mepyramine at histamine H1 receptors were carried out. The determined equilibrium dissociation constant of radioligands (Kd) and the total number of specific binding sites (Bmax) of the receptor membrane preparations were in good agreement with reference data. Inhibition constants (Ki) of reference ligands obtained in radioligand competition binding experiments at dopamine hD2S, hD3 and histamine H1 receptors validated the reliability and reproducibility of the assay. In order to discriminate agonists from antagonists, a GTP shift assay has been investigated for dopamine D2S and D3 receptors. In competition binding studies at dopamine D2S receptors the high- and low affinity state in the absence of the GTP analogue Gpp(NH)p has been recognized for the agonists pramipexole and the seleno analogue 54. In the presence of Gpp(NH)p a decrease in affinity, referred to as “GTP shift”, has been revealed for agonists at dopamine D2S and D3 receptors. An effect of Gpp(NH)p on dopamine D2S receptor binding has not been observed for the antagonists ST 198 and BP 897, while a reverse “GTP shift” has been noticed at the dopamine D3 receptor. For the development of novel ligands with high affinity and selectivity for dopamine D3 receptors, investigation in refined structure-affinity relationships (SAR) of analogues of the lead BP 897 has been performed. Replacement of the naphthalen-2-carboxamide of BP 897 by aryl amide residues (1 - 4) had a clear influence on affinity binding and selectivity for dopamine D3 receptors. Introduction of the benzo[b]thiophen-2-carboxamide (1) has markedly improved binding with subnanomolar affinity and enhanced selectivity for dopamine D3 receptors. Exchanging the aryl substituted basic alkanamine residue of 1 by a 1,2,3,4-tetrahydroisoquinoline moiety (6) emphasized the benefit of the 4-(2-methoxyphenyl) piperazine residue of BP 897 regarding dopamine D2 and D3 receptor affinities. The change of particular elements of BP 897 and the rearrangement of the amide functionality resulted in inverse amide compounds with new chemical properties. Moderate affinity binding data, as obtained for the isoindol-1-carbonyl compound 11, suggest that inverse amides provide a worthwhile new lead structure with a novel structural scaffold. A hybrid approach combining privileged scaffolds of histamine H1 receptor antagonists and fragments of dopamine D3 receptor-preferring ligands, related to BP 897and analogues has been investigated. Various benzhydrylpiperazine derivatives and related structures have shown moderate to high affinities for dopamine D3 receptors with the impressive enhancement of the cinnamide substituted bamipine-related hybrid 39, exhibiting the highest affinity and selectivity for dopamine D3 receptors. Improved affinity profiles of structural modified histamine H1 receptor antagonists for dopamine D2 and D3 receptors and a refined SAR has been achieved. A SAR of derivatives of the dopamine agonist pramipexole and the related etrabamine has been studied. The propargyl substituted etrabamine derivative 61 demonstrated highest affinity and selectivity. The ligand attracts attention since neuroprotective properties have been reported for the propargyl functionality. Further development resulted in the most promising compound 64, a cinnamide derivative with 4-fluoro substitution on the phenyl ring. Subnanomolar affinity and remarkable selectivity for dopamine D3 receptors has aroused particular interest in this ligand due to its development potential as a radioligand for PET studies. Radioligand binding studies in combination with virtual screening and different classification techniques of chemoinformatic methods resulted in further elucidation of SAR. New leads with novel chemical scaffolds have been found in the bicycle[2.2.1]heptane derivative 95 and the benzhydrylidene substituted pyrrolidindione 112 and can be further optimized by chemical modifications. The outcome of the studies provides the development of various novel high affine and dopamine D3 receptor selective ligands. Modifications of lead structures or application of chemoinformatic tools in combination with radioligand competition binding assays have resulted in new leads with different chemical scaffolds. Furthermore, a comprehensive insight into structure-affinity relationships of ligands at dopamine D3 receptors has been revealed. This refined SAR is valuable to develop more affine and selective drug candidates with a designed pharmacological receptor profile.
Deferred imitations assess declarative memory in infants. Many cross-sectional and a few longitudinal studies revealed that, with development, infants learn faster,and retain more target actions over longer retention intervals. Longitudinal stabilities are modest and increase through the second year. To date, there are only few multivariate deferred imitation studies pointing to interactions between declarative memory, language and self-development. However, as these studies applied variable-centered data analysis approaches, the individual stance was not taken into account.Therefore, the present dissertation focuses on the explanation of inter-individual differences of deferred imitation through the second year. In the multivariate, longitudinal Frankfurt Memory Study (FRAMES), declarative memory (deferred imitation), non-declarative memory (train task), as well as cognitive, language, motor, social, emotional and body self-awareness development (Developmental Test for 6-month- to 6-year-olds, ET6-6) were assessed on three measurement occasions (12-, 18- and 24-month-olds). From a psychometric perspective, sound tests for the assessment of deferred imitation in the respective age groups were developed (Paper 1 & 2). Reliability analyses (Paper 3) indicated relatively high short-term-stability for the deferred imitation test (12-month-olds). The co-development of declarative and nondeclarative memory in 12- and 18-month-olds provided evidence for discriminative validity (Paper 4). Longitudinally, deferred imitation performance tremendously increased throughout the second year, and performance was moderately stable between 12 and 18 months and stability increased between 18 and 24 months. Using a person-centered analysis approach (relative difference scores; cluster analysis), developmental subgroups were extracted out of the total sample. These groups differed in terms of mean growth and stability. However, between the first and second measurement occasion, the groups did not differ with respect to motor, cognitive and language development (Paper 5). Using the data of three measurement occasions, subgroups were extracted showing significant differences with respect to language, motor and body self-awareness development (Paper 6). The results are discussed against the background of infancy development theories.
An application of EPR spectroscopy that is becoming increasingly important is the measurement of distances between electron spins. Several EPR methods have been developed for this purpose, all based on measuring the dipolar coupling between two spins. Due to the specific nature of the sample, we applied dipolar relaxation enhancement measurements to study the geometry of a protein-protein complex. The paramagnetic centers in question had EPR spectra that were too broad and had such short relaxation time that they could not be studied using the more straightforward PELDOR technique. EPR spectral resolution can be increased appreciably by measuring at a frequency higher than conventional X-band (9 GHz) frequency. The spectra of many paramagnetic species can only be resolved at frequencies higher than 90 GHz. For accurate measurement of the orientation of the vector between two dipolar coupled spins with respect to the g-tensors of the spins, high spectral resolution is required. We therefore performed our EPR measurements at G-band (180 GHz) frequency. Dipolar relaxation measurements were applied to study the complex that is formed by the two electron-transfer proteins cytochrome c and cytochrome c oxidase (CcO) from the soil bacterium Paracoccus denitrificans. We were able to detect dipolar relaxation enhancement due to complex formation of soluble subunit II of P.d. CcO (CcOII) with two substrate cytochromes, which was practically absent in a mixture of CcOII with the negative control protein cytochrome c1. This complex formation was characterized by a pronounced temperature dependence that could be simulated using a home-written computer program. The G-band EPR measurements could not be simulated with a single complex geometry. This provided evidence for the hypothesis that electron-transfer protein complexes are short-lived and highly dynamic; they do not seem to form one specific electron-transfer conformation, but rather move around on each other’s binding surfaces and transfer an electron as soon as the distance between donor and acceptor is short enough. As a test of our simulation program, we also applied dipolar relaxation measurements to specially synthesized organic molecules that contained a nitroxide radical and a metal center. The transverse relaxation of Cu2+-OEP-TPA was compared to the relaxation of Ni2+-OEP-TPA at temperatures between 20 and 120 K. In this temperature range, the nitroxide relaxation was enhanced due to the presence of Cu2+, but not by Ni2+. Similarly, relaxation enhancement was found in the nitroxide-Mn2+ pair in Mn2+-terpyridine-TPA with respect to the terpyridine-TPA ligand. Due to the fast T2 relaxation of the nitroxide radical at high temperatures, the measurements were all performed in the low-temperature regime where the T1 relaxation rate of the metal ion was smaller than the dipolar coupling frequency. In this region, no structural information about the molecule can be deduced, since the dipolar relaxation enhancement is only determined by the T1 of the metal ion. The dipolar relaxation measurements we performed at high field indicated a difference in relaxation times between X-band and G-band frequencies. Extensive T1 - measurements of different paramagnetic centers (CuA, Cu2+) confirmed a strong dependence of T1 on magnetic field in the temperature range where the direct process is the dominating T1 relaxation process. This dependence is very strong (factor of 103 with respect to X-band), but does not follow the B04 dependence predicted in literature. The T1 relaxation of low-spin iron in cytochrome c at high magnetic field, estimated from dipolar relaxation data, is also in agreement with a larger contribution by the direct process (factor of 104). Dipolar relaxation enhancement was found to be a technique that is useful for measuring distances between paramagnetic centers, but only for systems where several important conditions are met, such as: the system exists in one certain static geometry, and the relaxation rate of the fast-relaxing spin is faster than the dipolar coupling frequency within the accessible temperature range. Additionally, it is a great advantage for the analysis of dipolar relaxation data if the procedure of dividing the relaxation trace of the dipolar-coupled slow-relaxing spin by the relaxation trace of the slow-relaxing spin in absence of dipolar coupling can be applied. Another useful application of dipolar relaxation enhancement measurements is the measurement of T1 relaxation of extremely fast-relaxing spins, or spins that are otherwise difficult to detect.
Colorectal cancer is one of the most cause of cancer and death in Western societies. Recently, histone deacetylase inhibitors (HDIs), which regulate transcription through modification of chromatin structure, received considerable interest on the ground of they ability to stop the growth and induce cell death in colon cancer tumours, representing a promising transcriptional cancer therapy. This kind of cancer initiates with an activating mutation in the Wnt cascade, allowing the nuclear import of ß-catenin binding to LEF/TCF. This induces the overexpression of growthpromoting oncogenes affecting the cell cycle arrest, lineage-specific cell differentiation and apoptosis processes. In addition, ß-catenin also participates in cell-cell adhesion via interactions with E-cadherin, which can be repressed by families of transcription factors Snail and ZEB. This, and gain of vimentin has been closely correlated with local invasion and metastasis since they avoid the induction of apoptosis through the loss of cell anchorage, a phenomenon called anoikis. In this process the inactivation of the kinases Src an FAK provoking disruption of focal adhesion complexes through is involved. LAQ824 is a HDAC inhibitor derivative of hydroxamic acid, which present antitumor effect in colon and other cancer cells. The aim of this study is to analyse the effect of LAQ824 in cell proliferation, apoptosis, motility and tumour invasion in a colon carcinoma model based on the adenoma-carcinoma sequence descrying trough which pathways LAQ824 is able to cause these effects. Here I demonstrate for the first time that a HDAC inhibitor, LAQ824, induces detachmentinduced cell death of colon cancer cell lines HCT116 and HT-29, a phenomenon called anoikis, in a caspase-dependent and p53-independent manner. In this process the component of the Wnt signalling pathway ß-catenin is involved. Furthermore LAQ824 upregulates the adhesion molecule E-cadherin expression in these cell lines independently of its repressor Snail, but probably mediated by the repressor ZEB. In addition LAQ824-induced anoikis is caused by disruption of focal adhesion complexes through inhibition of the activity of the kinases FAK and Src inhibiting cell motility indicating a strong antimetastatic potential for LAQ824.
Transcranial magnetic stimulation (TMS) is a non-invasive technique which can be used to study different intracortical excitatory and inhibitory neuronal circuits in the intact human being. In the primary motor cortex, there are essentially three different TMS measures of inhibitory neuronal circuits as determined by paired-pulse TMS: short-interval intracortical inhibition (SICI), long-interval intracortical inhibition (LICI) and interhemispheric inhibition (IHI). It was hypothesized that SICI is a GABAA receptor mediated inhibition (Ilic et al., 2002) whereas LICI and IHI are mediated by GABAB receptors (Daskalakis et al., 2002; McDonnell et al., 2006). Additionally, it was shown that these inhibitory circuits interact negatively, possible due to presynaptic GABAB receptor mediated inhibition (Sanger et al., 2001; Daskalakis et al., 2002). Which neuronal populations exactly underlie SICI, LICI and IHI, is not completely clear and by which mechanism these inhibitory circuits interact has never been tested pharmacologically so far. Thus, the effects of a single oral dose of Diazepam (DZP), a specific positive allosteric modulator at the GABAA receptor, and of Baclofen (BAC), a specific GABAB receptor agonist, on SICI, LICI and IHI as well as their interactions were tested here in a randomized, placebo controlled, double-blinded crossover study. SICI significantly increased after intake of DZP whereas BAC did not change SICI. Conversely, LICI significantly increased after intake of BAC but did not change after intake of DZP. IHI showed only a trend towards a decrease after intake of DZP but no change after intake of BAC. The interactions IHI-SICI, LICI-IHI and LICI-SICI were all negative at baseline. SICI and IHI were partially suppressed in the presence of IHI and LICI, respectively, and SICI in the presence of LICI was almost completely blocked. BAC did not change any of these interactions, whereas DZP significantly increased SICI in the presence of LICI. This study is the first to examine by means of pharmacological testing the complex interactions between different inhibitory circuits in the human motor cortex. The effects of DZP and BAC on SICI and LICI confirmed the notion that SICI is a GABAA receptor mediated intracortical inhibition whereas LICI depends on GABAB receptor mediated neurotransmission. The pharmacology of IHI at short interstimulus intervals of < 20 ms (12 ms in this study) remains still inconclusive and warrants further investigation. Findings further suggest that SICI, LICI and IHI represent three different inhibitory neuronal circuits which can be tested non-invasively by means of paired-pulse TMS. Furthermore, the data support the idea that the negative interactions IHI-SICI, LICI-IHI and LICI-SICI are most likely due to presynaptic GABAB receptor mediated autoinhibition.
Many environmental chemicals are suspected of disturbing the human and animal endocrine system. These so-called endocrine disruptors can operate in many ways. The interaction of endocrine disruptive effects that eventually endanger human health is still unclear. However, one of the basic mecha-nisms of endocrine disruption is the inhibition of key enzymes in the hormone metabolism. In this study, we focused on the inhibitory potency of suspected endocrine disrupting compounds on aromatase (P450arom) and 5alpha-reductase (5alpha-Re) activities in human tissue and human cancer cells. Both enzymes are essential for the human sex steroid hormone metabolism. We were able to demonstrate that the organotin compounds tributyltin (TBT) and triphenyltin (TPT) are potent unspecific inhibitors of P450arom and 5alpha-Re activity. Prochloraz and fenarimol inhibited P450arom activity at low concentrations (IC50<2 µM), while 5alpha-Re activity was only impaired at higher concentrations (IC50>10 µM). While the human tissue assay proved to be more practical and sensitive as a screening tool for putative endocrine disruptors, the cell assay reflected partly the situation in vivo. In another experimental series, we investigated the inhibitory effect of TPT on P450arom, 5alpha-Re, 3beta-HSD type 2, 17beta-HSD type 1 and type 3 alone and in combination with the strong antioxidant dithioerythrithol (DTE). TPT inhibited unspecifically all enzymes that were tested. The experiments also showed that DTE is able to compensate the adverse effects of TPT, and that the effectiveness of the compensatory activity of DTE differs among the enzymes investigated. The suppressed 5alpha-Re activity could not be reactivated with DTE. Conceivably, cysteine residues that are responsible for the tertiary and quarternary structure of the enzyme are critical targets for TPT. A human sampling study was undertaken with the COMPRENDO partner in Gdansk. 60 Polish and 15 German blood samples were investigated for chemical residues and sex hormone concentrations. In addition, 15 placenta samples from Poland and Germany, respectively, were tested for chemical residues, P450arom activities and CYP19 mRNA contents. The chemical analysis was performed by the COMPRENDO partners in Milan (p,p´DDE), Orleans (TBT and TPT) and Ioannina (diuron, fenarimol, linuron und vinclozolin). The results showed that individual sex hormone concentrations in blood were not correlated with chemical body burden. The detected differences in sex hormone concentrations, specific aromatase activity and relative CYP19 mRNA content of Polish and German donors were presumably the result of other factors than the ones determined in this study. Another task of the EU-project was the investigation of the effects of chemical exposure of the aquatic model organisms Pimephales promelas, Rutilus rutilus and Xenopus laevis. We investigated the specific P450arom and 5alpha-Re activities in brain and gonads of the animals. During the qualitative investigation of the androgen metabolism in Xenopus laevis brain, 5alpha-reductase activity was discovered for the first time. In contrast to the inhibitory potency of TPT discovered in our enzyme assays, TPT exposure of aquatic model organisms had no observed effect on enzyme activity in the organs investigated, except for P450arom activities in female gonads of Pimephales promelas at 320 ng TPT/L. In this group, mean P450arom activities were elevated, possibly as a result of an overshooting upregulation due to the inhibition of P450arom by TPT. The exposure of Rutilus rutilus and Xenopus laevis to the effector substances methyltestosterone and letrozole resulted in slightly different mean enzyme activities compared to the control group. In conclusion, many of the tested pesticides are able to inhibit P450arom and 5alpha-Re, and thus might be of clinical relevance. However, results are not always coherent, and possible risks for human and wildlife health are therefore difficult to predict. Risk assessment will require large studies with an additional number of short and long term in vitro and in vivo assays. Any extrapolation to humans should be very meticulously performed.
The strong nuclear force is described by Quantum Chromodynamics (QCD), the parallel field theory to Quantum Electrodynamics (QED) that describes the electromagnetic force. It is propagated by gluons analogously to photons in the electromagnetic force, but unlike photons, which do not carry electric charge, gluons carry color, and they can self-interact. However, as individual quarks have never been observed in nature, it is postulated that the color charge itself is confined, and hence all baryons and mesons must be colorless objects. To study nuclear matter under extreme conditions, it is necessary to create hot and dense nuclear matter in the laboratory. In such conditions the confinement between quarks and gluons is cancelled (deconfinement). This state is characterized with a qusi-free behavior of quarks and gluons. The strange (s) and anti-strange (anti-s) quarks are not contained in the colliding nuclei, but are newly produced and show up in the strange hadrons in the final state. It was suggested that strange particle production is enhanced in the QGP with respect to that in a hadron gas. This enhancement is relative to a collision where a transition to a QGP phase does not take place, such as p+p collisions where the system size is very small. Therefore the energy- and system size dependence is studied to receive a picture about the initial state. In this thesis experimental results on the energy- and system size dependence of Xi hyperon production at the CERN SPS is shown. All measurements were performed with the NA49 detector at the CERN SPS. NA49 took central lead-lead collisions from 20 - 158 AGeV, minimus bias lead-lead collisions at 40 and 158 AGeV, and semi-central silicon-silicon colisions at 158 AGeV. The NA49 experiment features a large acceptance in the forward hemisphere allowing for measurements of Xi rapidity spectra. At the SPS accelerator at CERN Pb+Pb collisions are performed with beam energies to 158 AGeV. The analyzed data sets were taken in the period from 1999 to 2002. The NA49 experiment is a large acceptance hadron spectrometer, which measures charged hadrons in a wide acceptance. The main components are the four TPCs (Time Projection Chamber). The centrality of nucleon-nucleon collisions was done by measuring the not in the collision participating (spectator-) nucleons in the VETO-calorimeter. The study of strangeness is motivated by its role as a signature for the Quark Gluon Plasma. Any enhancement in the yield must be with respect to a ’normal’ yield, where a QGP is not formed. This is usually taken to mean suitably scaled p+p collisions, where the volume of the system created is too small for a QGP to occur. The results at SPS and RHIC energies show an enhancement, with the doubly strange Xi? being enhanced more than the Lambda, in accordance with the original prediction. However, the enhancement at SPS energies is higher than at RHIC energies.
Membrane proteins play vital role in a variety of cellular processes, such as signal transduction, transport and recognition. In turn they are involved in numerous human diseases and currently represent one of the most prevalent drug targets. A comprehensive understanding of the mechanisms mediated by membrane proteins requires information about their structures at near-atomic resolution, although structural studies of membrane proteins remain behind those of soluble proteins. A bottleneck in the study of membrane proteins resides in the difficulties that are encountered during their high-level production in cell based systems. However, many toxic effects attributed to the over production of membrane proteins are eliminated by cell-free expression, as viable host cells are no longer required. Therefore, the objective of this study was to obtain adequate amounts of selected membrane transport proteins for their structural studies using a cell-free expression system. For the establishment of the cell-free system for membrane proteins, the transporters YbgR and YiiP from Salmonella typhimurium LT2, PF0558 and PF1373 from Pyrococcus furiosus, from the cation diffusion family (CDF), BetP from Corynebacterium glutamicum from the betaine/carnitine/choline transporter (BCCT) family and Aq-2030 from Aquifex aeolicus VF5 from the monovalent cation/proton antiporter-2 (CPA2) family were selected. An Escherichia coli S-30 extract based cellfree system was established by generating the best expression constructs of the target proteins, preparing T7 RNA polymerase and an S-30 extract with high translation efficiency. The functionality of the S-30 extract was shown by the cell-free expression of correctly folded Green Fluorescent Protein (GFP). Essential factors of the cell-free system such as the Mg2+ concentration, the bacterial S-30 extract proportion in the reaction mixture and the time-course of cell-free reactions have been optimized. For the cell-free production of membrane proteins in soluble form, the possibility to supplement cell-free reactions with detergents was explored. A wide range of non-ionic or zwitterionic detergents, were found to be compatible with cell-free synthesis, while ionic detergents and non-ionic detergents at high concentrations had an inhibitory effect. Moreover, high concentrations of polyoxyethylene-alkyl-ethers (Brij) detergents were found to have enhancing effect on the production levels as well as on the solubility of cell-free produced proteins. As membrane proteins tend to misfold and aggregate in a membrane-free translation system, the possibility to supplement the cell-free reactions with inner membrane vesicles (IMVs) to obtain correctly folded target transport proteins was explored. All the target proteins were successfully produced in the batch cell-free reactions and were found to be incorporated in the IMVs. A continuous exchange cell-free (CECF) system was established, where consumable substrates (amino acids, nucleotides and energy regenerating compounds) were supplied to the cell-free reaction mixture through a dialysis membrane, which in consequence resulted in high-level production of target proteins compared to the batch system. The osmosensing and osmoregulated sodium-coupled symporter BetP from C. glutamicum was chosen for the large scale production in CECF set-up. The protein is easily produced in E. coli and is functional as assayed by its transport activity, after purification and reconstitution in liposomes. It is therefore possible to compare in-vivo and cell-free production. High-level cell-free production of BetP was achieved in CECF mode in different forms: (i) as precipitate, (ii) as soluble form in detergent, and (iii) incorporated in IMVs. Cell-free production of BetP resulted in the yield of about 0.5 mg of purified BetP from 1 ml of CECF reaction. The yield of purified BetP was increased to 1.6 fold by addition of 1% polyoxyethylene-(20)-cetyl-ether (Brij58) detergent in the reaction mixture. Moreover, the high level cell-free production of BetP (0.5 mg purified BetP/ml reaction mixture) incorporated in IMVs was shown for the first time in this work.However, it was observed that oligomerization of BetP was not efficient in the cell-free system. Factors that can promote the folding of membrane proteins such as lipids and chaperones were investigated. Addition of lipids and molecular chaperone GroE facilitated correct folding of BetP resulting in increased yield and stability of cell-free produced BetP. The results obtained indicate that most of the cell-free produced BetP exists in functional oligomeric form. The possibility of obtaining milligram amounts of BetP, a 12 trans-membrane protein from the cell-free reactions holds promise for structural and functional studies of other membrane proteins. In any case, the strategies adapted in this study should prove extremely valuable for the production of membrane proteins in the E. coli cell-free expression system.
This thesis is concerned with various aspects of estimating trend output and growth and discusses and evaluates methods to prepare medium-term GDP growth projections. Furthermore, econometric techniques suited for cross-correlated macroeconomic panel data with a focus on factor models are applied for unit root and cointegration testing as well as panel error correction estimation. Applications involve the identification of growth determinants as well as the modelling of aggregate labor supply in a multi-country framework. The first chapter evaluates a very popular method for potential output estimation and medium-term forecasting---the production function approach---in terms of predictive performance. For this purpose, a particular forecast evaluation framework is developed and an evaluation of the predictions of GDP growth for the three to five years ahead for each individual G7 country is carried out. In chapter two, a new approach for estimating trend growth of advanced economies is proposed. The suggestion combines econometric methods that have been used to test and estimate the implications of the extended Solow growth model in a cross sectional time series setting with an application of multivariate time series filter techniques. The last chapter discusses several panel unit root tests designed to accommodate cross-sectional dependence. These methods are then applied to an OECD country sample of the aggregate labor supply measure "hours worked".
The thesis is devoted to the study of the Antarctic polar vortex, mainly by analyzing data collected during APE-GAIA (1999) and ASHOE (1994) campaigns and recorded by the ADEOS satellite (1996-1997), and to improvement of the chromato-graphic processing schemes. A general introduction and overview of the campaigns and instruments relevant to the present work are given in Chapters 1 and 2. A relatively large part of the thesis (Chapters 3-5) is on improvement of the analysis of raw chromatographic data recorded during in-flight measurements of the trace gases. A Gaussian non-straight-base-line method, i.e. the Gaussian processing scheme (Chapter 3), is developed for better evaluation of the chromatographic peak size. Furthermore, a statistical cross-correlation method (Chapter 5) based on statistical behaviour of the whole chromatogram series fNchrg recorded, e.g., during a research flight or laboratory calibration, is developed and applied to measure the low-concentration trace gases. As demonstrated for HAGAR's chromatograms (HAGAR - High Altitude Gas Analyzer), the combination of the Gaussian fitting scheme for individual chromatograms and the statistical cross-correlation method for a series of subsequent chromatograms considerably improves and stabilizes quantitative analysis of in-flight chromatographic data. In this case, the detection accuracy of weak and noisy chromatographic signals can be improved by up to 40 %. A particular attention is paid to the in-flight two-standard calibration method. For this method, a special procedure, that allows to evaluate and effectively remove a weak background chromatographic signal associated with residual molecules in the carrier gas N2, is proposed and coded (Chapter 4). The developed approaches and methods are completely automized and, therefore, can be used for processing of in-flight chromatograms of recent and future field campaigns. The main part of the thesis (Chapters 6-8) deals with a two-dimensional quasi-Lagrangian coordinate system ... , based on a long-lived stratospheric trace gas i, and its systematic use for i = N2O in order to describe the structure of a well-developed Antarctic polar vortex, linearization and compactization of the tracer-tracer correlations in the polar vortex core (i.e. the stratospheric dynamics in this area), and the differential ozone losses in the Antarctic polar vortex area. In the coordinate system ... (...-method, Chapter 6), which refers to a well-developed polar vortex, the mixing ratio Âi is the vertical coordinate and ... = .... i is the reference profile in the vortex core) is the meridional coordinate. The quasi-Lagrangian coordinates ... are much more long-lived comparing with the standard quasi-isentropic coordinates, potential temperature ... and equivalent latitude ..e, do not require explicit reference to geographic space, and therefore well-suited for studying the dynamics of the Antarctic polar vortex and the relevant ozone loss processes. By using the introduced coordinate system ... to analyze the well-developed Antarctic vortex investigated in the APE-GAIA campaign, it is shown, in concurrence with the conclusion of A. M. Lee et al. (2001), that the Antarctic vortex area can be described in terms of the well-mixed and well-isolated vortex core, relatively wide vortex boundary region and adjoining surf zone. In this case, the reference profile ... i , which is compact in a well-developed and isolated polar vortex core [J. B. Greenblatt et al. (2002)], can be found by combining airborne (and/or balloon) data with high-altitude satellite measurements. A criterion, which uses the local in-situ measurements of Âi = Âi(£) and attributes the inner vortex edge to a rapid change (±-step) in the meridional pro¯le of the mixing ratio..., is developed in Chapter 6 to determine the (Antarctic) inner vortex edge. In turn, the outer vortex edge of a well-developed Antarctic vortex is proposed to attribute to the position of a local maximum of ...H2O in the polar vortex area. For a well-developed Antarctic vortex, the ...-parametrization of tracer-tracer correlations allows to distinguish the tracer-tracer inter-relationships in the vortex core, vortex boundary region and surf zone (Chapter 7). This is clearly illustrated by analyzing the tracer-tracer relationships Âi ¡ ÂN2O obtained from the in-situ data of the APE-GAIA campaign for i = CFCl3 (CFC-11), CF2Cl2 (CFC-12), CBrClF2 (H-1211) and SF6. The solitary anomalous points in the ...CFC11 ¡ ÂN2O correlation, observed in the Antarctic vortex core during the APE-GAIA and ASHOE campaigns, are interpreted in terms of small-scale localized differential descent. As detailed in Chapter 8, the quasi-Lagrangian coordinate system fÂN2O; ¢ÂN2Og is an effective tool for evaluation of the differential ozone losses in the polar vortex area. With this purpose, a two-parametric reference function ...O3 = F(...), which characterizes the unperturbed O3 distribution in the early winter polar vortex area, is introduced to separate and quantify in terms of the meridional coordinate ...2O the differential ozone losses in the vortex core and vortex boundary region. The method is applied to analyze the ozone depletion in the Antarctic stratosphere during the austral spring 1999 (APE-GAIA campaign). In Chapter 9, the main results of the thesis are summarized.
Two types of proteins transport ions across the membrane – ion channels and ion pumps. Ion pumps transport ions against their electrochemical gradient by co-transporting another ion or a substrate molecule through a concentration gradient or by coupling this process to an energy source like ATP. Those that couple ATP hydrolysis to ion transport are called ion motive ATPases and can be classified as ‘V’, ‘F’ and ‘P’ types. In this thesis, two sub-classes of P-type ATPases, PIIIA and PIB were studied. Attempts were made to over-express and crystallize the plant proton pump AHA2 (a PIIIA-ATPase). Also, the two putative copper transporting ATPases, CtrA3 (CopB-like) and CtrA2 (CopA-like) from Aquifex aeolicus (both PIB pumps) were over-expressed in E. coli and characterized. PIIIA-type pumps transport protons across the membrane and are found exclusively in plants and fungi, and probably some archaea. One of the most characterized proton pump biochemically is the A. thaliana proton pump AHA2. An 8Å projection map of this enzyme is already available (Jahn 2001). PIBATPases, also called CPX type pumps transport heavy metal ions such as Cu+, Cu2+, Zn2+, Pb2+, Cd2+, Co2+ across biological membranes and play an important role in homeostasis and biotolerance of these metals. CopA and CopB are two such proteins that transport copper across cell membrane found in many prokaryotes. CopB-like proteins are found almost exclusively in bacteria, with CPH sequence motif, while CopA-like proteins have CPC sequence motif, also found in eukaryotic copper transporters including human ATP7A and ATP7B. CopB extrudes Cu2+ across the membrane. CopA is activated by and transports Cu+ but the direction of transport is debated. Attempts were made to over-express the plant proton pump AHA2 in yeast Pichia pastoris. However, the yeast expressed only a truncated protein, which could not be used for further studies. It can be concluded that P. pastoris strain SMD1163 is not a good host for expression of AHA2. Focus was then shifted to AHA2 that has been over-expressed and purified from S. cerevisiae strain RS72. Growth and purification protocols had to be changed from published methods because of laboratory constraints and this probably had an effect on the protein produced. The protein purified from S. cerevisiae could not be crystallized reproducibly for structural studies by electron microscopy. CtrA3 was expressed in E. coli and purified using Ni2+-NTA matrix. Like CopB of A. fulgidus (Mana Capelli 2003), it was active only in the presence of Cu2+ and to some extent in Ag+. The protein was maximally active at 75°C, at pH 7 and in presence of cysteine. Lipids were essential for the activity of CtrA3. However, when the protein was purified in Cymal-6, CtrA3 could not hydrolyze ATP, even when lipids were added to the reaction mixture. For reconstitution of CtrA3 into liposomes for 2D crystallization, several lipids were tested. To screen the lipids compatible for protein incorporation, CtrA3 was dialyzed with different lipids at a high lipid-to-protein ratio of 10:1 and centrifuged by sucrose density gradient. Protein incorporated in lipids localized with liposome fraction in the gradient. Most of the CtrA3 was incorporated into DPPC with no aggregation. This lipid was used for reconstitution of CtrA3 at low LPRs, and at an LPR of 0.3-0.5, the protein formed 2D crystals. A NaCl concentration of 50mM was necessary for the formation of crystals. However, salt removal by dialysis prior to harvesting was essential for obtaining wellordered lattices of CtrA3. Addition of preservatives like trehalose and tannin or direct plunging in liquid ethane for cryo-microscopy destroyed the crystal lattice. Similar to CtrA3, the gene responsible for expression of CtrA2 was amplified from genomic DNA of A. aeolicus and expressed in E. coli and purified by Ni2+-NTA. Functional characterization of CtrA2 was done by analyzing ATP hydrolysis activity of the enzyme. Similar to CopA of A. fulgidus (Mandal 2002), CtrA2 was activated in the presence of Ag+ and to some extent, Cu+. It is possible that both the copper ATPases of A. aeolicus have different ion selectivity- CtrA3, specific for Cu2+ and CtrA2, specific for Cu+. Maximal activity of CtrA2 was also at 75°C. Cysteine was essential for activity of CtrA2, but the protein was not dependent on addition of lipids for activation. Reconstitution of CtrA2 was done similar to CtrA3 for screening of lipids for 2D crystallization. Of the lipids tested, DOPC reconstituted the protein best. However, screening at low LPRs did not yield any crystals. Even though both CtrA3 and CtrA2 are similar heavy metal transporting Ptype ATPases from the same organism and have 36% identity, they behaved completely different in their expression levels in E. coli, purification profiles, activity and reconstitution in lipids.
Quantum chromodynamics predicts the existence of a phase transition from hadronic to quark-gluon matter when temperature and pressure are sufficiently high. Colliding heavy nuclei at ultra-relativistic speeds allows to deposit large amounts of energy in a small volume of space, and is the only available experimental mean to produce the extreme conditions necessary to obtain the deconfined state. Numerous models and ideas were developed in the last decades to study heavy ion physics and understand the properties of extremely heated and compressed nuclear matter. With the ever increasing energy available in the center of mass frame (and thus number of particles produced) and the development of large acceptance detectors, it has become possible to study the fluctuations of physical quantities on an event-by-event basis, and access thermodynamical properties not present in particle spectra. The characteristics of the highly excited matter produced, e.g. thermalization, effect of resonance decay. . . can be investigated by fluctuation analyses. In fact, fluctuations are good indicators for a phase transition and a plethora of fluctuation probes have been proposed to pin down the existence and the properties of the QGP. We study various fluctuation quantities within the Ultra-relativistic Quantum Molecular Dynamics UrQMD and the quantum Molecular Dynamics qMD models. UrQMD is based on hadron and string degrees of freedom and allows to disentangle purely hadronic effects. In contrast, the qMD model includes an explicit transition from quark to hadronic matter and can serve to test adequate probes of the initial QGP state. We show that the qMD model can reasonably reproduce various experimental particles rapidity distributions and transverse mass spectra in wide energy range. Within the frame of the dynamical recombination procedure used in qMD, we study the enhancement of protons over pions (p/π) ratio in the intermediate pt range (1.5 < pt < 2.5). We show that qMD can reproduce the large p/π ≈ 1 observed experimentally at RHIC energies at hadronization. However, the subsequent decay of resonances makes the ratio fall to values incompatible with experimental data. We thus conclude that resonance decay might have a drastic influence on this observable in the quark recombination picture. Charged particles multiplicity fluctuations measured at SPS by the NA49 collaboration are enhanced in midperipheral events for Pb+Pb collisions at Elab = 160 AGeV. This feature is not reproduce by hadron-string transport approaches, which show a flat centrality dependence, within the proper experimental acceptance and with the proper centrality selection procedure. However, we show that the behavior of multiplicity fluctuations in transport codes is similar to the experimental result in full 4π acceptance. We identify the centrality selection procedure as the reason for the enhanced particle multiplicity fluctuations in midperipheral reactions and argue that it can be used to distinguish between different scenarios of particle productions. We show that experimental data might indicate a strong mixing of projectile and target related production sources. Strangeness over entropy K/π and baryon number over entropy p/π ratio fluctuations have been measured by the NA49 experiment in the SPS energy range, from Elab = 20 AGeV up to Elab = 160 AGeV. We investigate the sensitivity of this observable to kinematical cuts and discuss the influence of resonance decay. We find the dynamical p/π ratio fluctuations to increase with beam energy, in agreement with the measured data points. On the contrary, the dynamical K/π ratio fluctuations are essential flat as a function of centrality and depend only weakly on the kinematical cuts applied. Our results are in line with the simulations performed earlier by the NA49 collaboration in their detector acceptance filter. Finally, we focus on the correlations and fluctuations of conserved charges. It was proposed that these fluctuations are sensitive to the fractional charge carried by the quarks in the initial QGP stage and survive the whole course of heavy ion reactions. A crucial point is the influence of hadronization that may relax the initial QGP fluctuation/correlation signals to their hadronic values. We use the quark Molecular Dynamics qMD model to disentangle the effect of recombination-hadronization on charged particles ratio fluctuations, charge transfer fluctuations, baryon number-strangeness correlation coefficient and various ratios of susceptibilities (i.e. correlations over fluctuations). We find that the dynamical recombination procedure implemented in the qMD model destroys all studied initial QGP fluctuations and correlations and might ex- plain why no signal of a phase transition based on event-by-event fluctuations was found in the experimental data until now.
The ABC protein ABCE1, also called HP68 or RNase L inhibitor (RLI), is one of the most conserved proteins in evolution. It is universally expressed in eukaryotes and archaea, where ABCE1 is essential for life. ABCE1 plays a crucial role in translation initiation and ribosome biogenesis, however, the molecular mechanism of ABCE1 remains unclear. In addition to two ABC ATPase domains, ABCE1 contains a unique N-terminal region with eight conserved cysteines predicted to coordinate iron-sulfur (Fe-S) clusters. To analyze the function of ABCE1, the hyperthermophilic crenarchaeote Sulfolobus solfataricus was chosen as a model system. S. solfataricus ABCE1 was overexpressed homologously in S. solfataricus and heterologously in E. coli. Noteworthy, for tagged-protein production in S. solfataricus a novel expression system based on a virus shuttle vector was established. This is the first example for a successful overexpression and purification of isolated full-length ABCE1. For the first time it was shown that ABCE1 indeed bears biochemical properties of an ABC protein even though it has unique features. Remarkably, the nucleotide binding domains (NBDs) of ABCE1 bound ATP and AMP, but were functionally non-equivalent in ATP hydrolysis. Mutations of conserved residues in the second NBD led to a hyperactive ATPase, which implies an intramolecular mechanism of dimer formation. Truncation of the Fe-S cluster domains did not influence ATPase activity. The Fe-S clusters of ABCE1 were analyzed by biophysical and biochemical methods. As presented in this study, ABCE1 harbors two essential diamagnetic [4Fe-4S]2+ clusters, one ferredoxin-like cluster formed by cysteines at position 4/5/6/7 and one unique ABCE1 cluster formed by cysteines at position 1/2/3/8. ABCE1 was found to be associated with RNA after purification from S. solfataricus and bound ribosomal RNA in vitro. In addition, ABCE1 showed homo-oligomerization and appeared to form a hexameric complex of ~440 kDa, which was RNase sensitive. Archaeal ABCE1 associated with ribosomes, however, the unique Fe-S clusters of ABCE1 were not required for this interaction. Although archaeal ABCE1 assembled with ribosomes and ribosomal RNA, ABCE1 proved not to be essential for translation in S. solfataricus and did not interact with archaeal initiation factors. Nevertheless, the ABCE1 gene is one of the few genes conserved between archaea and eukaryotes and fulfills a universal task, which needs further characterization.
21 Hsfs belonging to classes A, B and C were identified in Arabidopsis following the sequencing of its genome. 1.) Cloning of full length and CTD chimeric constructs followed by transient reporter assays in tobacco protoplast using GUS fusion constructs of the promoters of Hsp17.4-CI, synthetic (HSE9) and APX2 showed Hsfs A1a, A1b, A1d, A1e, A2, A3 and A9 to be active. CTDs of Hsfs A7a, A7b and HsfC1 had activity but they showed poor DNA binding in reporter assays. Hsfs A1a, A1b, A1d, A1e, A2 and A3 were able to induce the expression of endogenous Hsps in tomato protoplasts. Interesting differences in promoter selectivity were observed for several Hsfs. 2.) RT-PCR and microarray analysis showed the Hsfs to be differentially expressed depending on tissue, abiotic and biotic stress, hormone and developmental s ge. Interesting patterns of coexpressed Hsfs were observed under different stresses and developmental stages. 3.) HsfA1b was found to be active on the plasmid borne PHsf:GUS reporters of Hsfs A1d, A2, A4a, A7b and B4 when tested in tobacco mesophyll protoplasts. Hsfs A1d, A2, A4a, A7b and B4 when tested in tobacco mesophyll protplasts. HsfA2 was inactive on PHsfA:GUS. HsfB1 showed repression of endogenous activity on several PHsf:GUS reporter constructs. 4.) The transcriptional regulation under heat stress and promoter organization of HsfA2 and FtSH4 (a metalloprotease gene oriented in a head to head fashion with HsfA2 in the Arabidopsis genome, sharing a common promoter region) was studied. The transcripts of FtSH4 and HsfA2 coaccumulated under heat stress. HsfA1b was active on PHsfA2:GUS and PFtSH4:GUS. Hsf binding sites on the intergenic region were determined using promoter deletion constructs in tobacco and Arabidopsis protoplasts. A bidirectional regulation of HsfA2 and FtSH4 by HsfA1b was observed in tobacco protoplast. 5.) Microarray analysis of a HsfA2 T-DNA insertion line vs. wild type Col-0 under heat stress conditions led to identification of a subset of target genes to be severely affected in the absence of HsfA2. Apart from several Hsps (heat stressproteins) and APX2 (Ascorbate peroxidase 2, oxidative stress scavenger), several other unknown genes are affected. APX2 was the most severely affected among them. HsfA2 was able to induce the transcription from its target gene promoters in fusion to GUS in transient reporter assays in tobacco protoplast. The HSE cluster to which HsfA2 binds on the APX2 promoter was also mapped by the same technique. The direct binding of HsfA2 to the promoter of selected target genes in the Arabidopsis genome was also demonstrated by chromatin immunoprecipitation studies.
The removal of apoptotic cells (AC) can be regarded as an integral component of the program to terminate inflammation. Clearance of AC by professional phagocytes such as macrophages induces an anti-inflammatory phenotype in the latter ones. Anti-inflammatory or M2 polarization is also observed in macrophages infiltrating certain human tumors. These tumor-associated macrophages (TAM) contribute actively to tumor progression by promoting immune evasion, angiogenesis and tumor cell survival. The aim of my Ph.D. thesis was to approach the mechanisms as well as the characteristics of macrophage phenotype alterations induced by AC, and to elucidate a possible connection between tumor cell apoptosis and TAM generation. In the first part of my studies, I investigated the impact of AC on macrophage viability. I could show that macrophage survival against pro-apoptotic agents increased after the interaction with AC. Protection of macrophages against cell death required activation of phosphatidylinositol-3 kinase (PI3K), extracellular signal-regulated kinase 1/2 (ERK1/2) and Ca2+ signaling, and correlated with Bcl-XL and Bcl-2 up-regulation as well as Ser136-Bad phosphorylation. Unexpectedly, neither phagocytosis nor binding of apoptotic debris to the phagocyte was necessary to induce protection. AC released the bioactive lipid sphingosine-1-phosphate (S1P), dependent on sphingosine kinase (SphK) 2, as a survival messenger. These data indicated an active role of AC in preventing cell destruction in their neighborhood. My next aim was to elucidate the mechanism of S1P production by AC. During cell death, SphK 2 was cleaved at its N-terminus by caspase-1. Thereupon, the truncated but enzymatically active fragment of SphK 2 was released from cells. This release was coupled to phosphatidylserine exposure, a hallmark of apoptosis and a crucial signal for the phagocyte/apoptotic cell interaction. Thus, I observed a link between common signaling events during apoptosis and the extracellular production of S1P, which is known to affect immune cell attraction and polarization as well as angiogenesis in cancer. In the next part of my studies, I asked for a correlation between tumor cell apoptosis and TAM polarization. During co-culture of human macrophages with human breast cancer carcinoma cells (MCF-7), the latter ones were killed, while macrophages acquired an alternatively activated phenotype. This was characterized by decreased tumor necrosis factor (TNF)-α; and interleukin (IL)-12-p70 production, but increased formation of IL-8 and IL-10. Alternative macrophage activation required tumor cell death, because a co-culture with apoptosis-resistant colon carcinoma cells (RKO) or Bcl-2-overexpressing MCF-7 cells failed to induce phenotype alterations. These phenotype alterations were also achieved with conditioned media from apoptotic tumor cells, which again argued for a soluble factor being involved. Knock-down of SphK2, but not SphK1, to attenuate S1P formation in MCF-7 cells, repressed the otherwise observed alternative macrophage polarization during co-culture. Furthermore, macrophage polarization achieved by tumor cell apoptosis or substitution of authentic S1P was characterized by suppression of pro-inflammatory nuclear factor (NF)-κB DNA binding. These findings suggested that tumor cell apoptosis-derived S1P contributes to the macrophage polarization present in human tumors. To validate these in vitro data, I used an in vivo tumor model to clarify the relevance of SphK2 and S1P in tumor development. The growth of, as well as blood vessel infiltration into SphK2 knock-down MCF-7 (MCF-7-siSphK2) xenografts in nude mice was markedly decreased in comparison to control MCF-7 xenografts. In contrast, macrophage infiltration was similar or even more pronounced. These data provided a first hint for an in vivo role of SphK2-derived S1P in macrophage polarization associated with tumor promotion. In summary, these data indicate a new mechanism how AC themselves shape macrophage polarization, which results in the termination of inflammatory responses and macrophage survival. Furthermore, my studies present evidence that human tumors may utilize this mechanism to foster growth via increased angiogenesis.
This work analyses several granitic bodies of the Variscan Orogen of Central and Western Europe in order to improve our knowledge about different aspects of their evolution, regarding their ascent and emplacement mechanisms, as well as their deformation history. In the Iberian Massif two granitoid bodies, namely the La Bazana pluton and the Nisa-Alburquerque batholith, were studied in order to decipher their ascent and emplacement history. The La Bazana pluton is a small, sub-circular body in map view that intruded into rocks of the Ossa-Morena Zone in the core of a late upright antiform. Its three-dimensional drop-pipe shape, its internal dome foliation pattern and the structure of the host rock suggest that the magma ascended and emplaced diapirically. The Nisa-Alburquerque batholith is a large body that intruded into rocks of the Central Iberian Zone, the Central Unit, and the Ossa-Morena Zone. Its cartographic shape is elongate and parallel to the NW—SE to WNW—ESE Variscan structures. In the light of the available structural data and the gravimetric models, the intrusion is viewed as a continuous lateral magma flow from the eastern root guided towards the west through the southern limb of a kilometre-scale antiform. As mass-transfer mechanisms, a combination of rigid translation of the country rocks, stoping, and possibly ballooning is proposed. In the Bohemian Massif several small granitoid bodies showing a strong solid-state deformation were studied in order to integrate their tectonometamorphic history in the geotectonic framework of the south-western Bohemian Massif, focusing principally on the deformation phase referred to as D3. Four ductile deformation phases are proposed for the study area. D1 produced high-temperature fabrics under upper amphibolite to granulite facies conditions. Its kinematics is unknown. D2 occurred under amphibolite to upper greenschist facies conditions under N—S to NNW—SSE compression. It is responsible for a subvertical NW—SE striking foliation in migmatites developed under dextral simple shear and for the deformation at the Bayerischer Pfahl shear-zone system at its earlier stages. Many granitoid dykes and stocks were found to be affected by sinistral shear along subvertical planes trending ENE to ESE. Since this deformation, which is called D3 in the present work, is not compatible with a N—S to NNW—SSE compression, it is proposed that these sinistral shear zones in granites do not belong to the Bayerischer Pfahl shear-zone system and constitute themselves a separated one, which is called “D3 shear-zone system”. D3 took place under upper greenschist to lower amphibolite facies conditions (~480-550°C). Both the intrusion and the deformation of the granites affected by D3 occurred at deep to intermediate levels of the crust, whereas the deformation took place under NE—SW compression. Datings on two of the deformed granites yielded 324.4 ± 0.8 Ma and 315.0 ± 1.0 Ma: Thus, the age of D3 is most probably ~315 Ma. The intrusion of most of the sheared granitoids was pre-kinematic with respect to D3. After D3 the N—S to NNW—SSE compression which governed D2 was restored, giving way to the next deformation phase D4, which was linked to further deformation at and next to the principal shears of the Bayerischer Pfahl shear-zone system under greenschist facies conditions. The causes for the change of the stress field leading to a NE—SW compression during D3 might be related to (1) global changes in the dynamics of the tectonic plates in late Variscan times, (2) orogenic collapse leading to the sinking of the Teplá-Barrandian and lateral extrusion of the surrounding Moldanubian rocks, (3) distortion of the regional stress field by local intrusion of large stocks, such as the Saldenburg granite of the Fürstenstein Massif, or (4) distortion of the regional stress field due to the existence of ephemeral releasing bends in the Bayerischer Pfahl shear zone during its early evolution.
We consider the theory of high temperature superconductivity from the viewpoint of a strongly correlated electron system. In particular, we discuss Gutzwiller projected wave functions, which incorporate strong correlations by prohibiting double occupancy in orbitals with strong on-site repulsion. After a general overview on high temperature superconductivity, we discuss Anderson’s resonating valence bond (RVB) picture and its implementation by renormalized mean field theory (RMFT) and variational Monte Carlo (VMC) techniques. In the following, we present a detailed review on RMFT and VMC results with emphasis on our recent contributions. Especially, we are interested in spectral features of Gutzwiller-Bogoliubov quasiparticles obtained by extending VMC and RMFT techniques to excited states. We explicitly illustrate this method to determine the quasiparticle weight and provide a comparison with angle resolved photoemission spectroscopy (ARPES) and scanning tunneling microscopy (STM). We conclude by summarizing recent successes and by discussing open questions, which must be solved for a thorough understanding of high temperature superconductivity by Gutzwiller projected wave functions.
Compared to all other organisms with 1 to 3 heat stress transcription factors (Hsfs) or Hsf-related factors, plants have extraordinarily large Hsf families with more than 20 Hsfs. Plant Hsfs are classified into three classes according to their oligomerization domains which is built of hydrophobic heptad repeats (HR) in two parts, HR-A and HR-B. Both parts may be immediately adjacent (class B), or they are separated by insertion of 21 (class A) and 7 amino acid residues (class C). In plant Hsf family, detailed investigations are so far limited to Hsfs A1a, A2, A3, A4d, A9, and B1. They strongly indicate functional diversification to be the main reason for the coexistence of multiple Hsfs. As an example the functional triad of HsfA1a, HsfA2, and HsfB1 is essential for all three phases of the hs response, (i) the triggering of the response by HsfA1a as master regulator, (ii) the maintenance and high efficiency of hs gene transcription by cooperation of HsfA1a with Hsfs A2 and B1, and finally, (iii) the restoration of house-keeping gene transcription during the recovery phase mediated by HsfB1 in cooperation with house-keeping transcription factors. The results presented in this thesis for Hsfs A4 and A5 open completely different aspects of functional diversification and cooperation of Hsfs. HsfA4 and HsfA5 homooligomerize and bind to corresponding HSE motifs. But in contrast to the highly active HsfA4, HsfA5 is completely inactive as transcriptional activator. Yeast two hybrid and GST pull-down techniques showed that both Hsfs have strong tendency for heterooligomerization. Using fluorescence microscopy the HsfA4/A5 heterooligomers were found to localize in the nucleus. These complexes are transcriptionally inactive due to the impairment of DNA binding. The repressor function of HsfA5 requires only its OD and no additional factors, e.g. a putative co-repressor recruited by the C-terminal domain, are involved. Evidently, the repressor effect mainly results from the interference with the oligomeric state of HsfA4b, which is essential for efficient DNA binding and activator functions. EST database search revealed that plants have a single HsfA5 and usually two A4-type Hsfs. Using bioinformatics tools, Hsfs A4 and A5 were found to be phylogenetically closely related and clearly distinct from the other members of the Hsf family. On the basis of RT-PCR and Microarray data the representatives of the A4/A5 group are well expressed in different plant tissues albeit at very different levels which change with the developmental stages and stress conditions In rice and Arabidopsis, HsfA4 functions as an anti-apoptotic factor for stress induced oxidative damages. Based on my results, I hypothesize that HsfA5 functions as a novel type of selective repressor, regulating the function of A4-type Hsfs in plants. Considering the high sequence conservation with in plant Hsf family, it is tempting to speculate that this role of Hsf4/A5 pair is a fundamental feature of the Hsf system in plants.
The high energy loss of heavy ions in matter as well as the small angular scattering makes heavy ion beams an excellent tool to produce almost cylindrical and homogeneously excited volumes in matter. This aspect can be used to pump short wavelength lasers. In an experiment performed at the GSI (Gesellschaft für Schwerionenforschung, Darmstadt, Germany) ion accelerator facility in December 2005 the well-known KrF* excimer laser was pumped with an intense high energy uranium beam. Pulses of an uranium beam with initial particle energy of 250 MeV per nucleon, provided by heavy-ion-synchrotron SIS-18, were delivered to the HHT-target station and then stopped inside a gas laser cell. The maximum beam intensity reached in the experiment was 2,5·109 particles per pulse, which resulted in 34 J/g specific energy deposited in the laser gas. By applying electron cooling and a bunch compression technique at SIS-18, the beam pulses were compressed down to 110 ns (FWHM). A mixture of an excimer laser premix gas (95,5% Kr + 0,5% F2) and a buffer gas (Ar 4.8) was used as the laser gas in proportions of 35/65 and 60/40, respectively. The gas pressure inside the laser cell was varied in the range of 1,2÷2 bar in continues flow mode. The experimental setup consisted of a 1 m long stainless steel tube with a number of diagnostic viewports and two mirror adjustment units. The optical cavity was formed by a flat, Alcoated mirror at the beam entrance and a second dielectrically coated, highly reflective mirror with 3 m radius of curvature at a distance of 1,3 m. A beam of heavy ions has been used to pump a short wavelength gas laser for the first time. Laser effect on the KrF* laser transition (λ = 248 nm) has been successfully demonstrated. Laser threshold for this specific setup was reached with a beam intensity of 1,2·109 particles per pulse. Laser action has been clearly proofed by the following methods: appearance of the laser line, spectral narrowing of the laser line, temporal narrowing of the laser signal, non-linear response of the laser output intensity on the pumping power, and cavity disalignment effect. An energy of the laser pulse of about 2 mJ was measured for an ion beam intensity of 2·109 particles per pulse. The time delay of the onset of the laser emission with respect to the pumping pulse was measured as a function of ion beam intensity. The dependence of spontaneous emission spectra on the gas pressure in a range of 1,3÷2 bar was observed and the optimal gas pressure for laser experiments in the sense of laser efficiency was concluded. As a next step in studying short wavelength lasers pumped with heavy ion beams it is planned to reduce the laser wavelength down to the VUV region of the spectrum, and to proceed to the excimer lasers of the pure rare gases: Xe2 * (λ = 172 nm), Kr2 * (λ = 146 nm), Ar2 * (λ = 126 nm), Ne2 * (λ = 83 nm) and He2 * (λ = 80 nm). We believe that the use of heavy ion beams as a pumping source may lead to new pumping schemes on the higher lying level transitions and considerably shorter wavelengths (XUV and X-ray spectral region), which rely on the high cross sections for multiple ionization of the target species.
Cytochrome b561 (cyt b561) proteins are members of the recently identified eukaryotic ascorbate reducible protein family named CYBASC (CYtochrome B, ASCorbate reducible). CYBASC proteins are di-heme-b-containing membrane proteins that catalyze the transmembrane electron transfer from ascorbate. The function of the CYBASC proteins has been correlated with ascorbate recycling and/or iron facilitation uptake. Therefore, investigations on this family are of great interest as ascorbate is one of the most powerful antioxidants and iron is essential for cell survival both in animals and plants. As the amino acid sequence conservation of animal and plant CYBASC proteins is relatively high, all CYBASC members are proposed to share the same structural motifs. However, no three-dimensional structure of any representative member of the CYBASC family has been determined to date. In the Arabidopsis thaliana (A. thaliana) genome, two complete putative CYBASC open reading frames (ORFs), artb561-a and artb561-b were identified. In this thesis, these two A. thaliana CYBASC ORFs, encoding for Acytb561-A and Acytb561-B proteins respectively, were investigated and obtained main results are listed. 1. A. thaliana CYBASC proteins were heterologously produced in Pichia pastoris and Escherichia coli and purified by a single-step immobilized metal affinity chromatography (IMAC). To facilitate detection and purification, the recombinant A. thaliana CYBASC proteins were produced in both expression systems with the histidine affinity tag. Pure and stable preparations of the cytochromes were obtained via a single-step IMAC in sufficient amounts to perform biochemical characterizations. 2. Detergent solubilized recombinant Acytb561-A and Acytb561-B are dimers. As previously suggested for other CYBASC proteins, analytical gel filtration experiment suggested that both detergent solubilized cytochromes are dimers. 3. Spectroscopic features of Acytb561-B differed from those of previously described bovine chromaffin granule cyt b561. A distinctive feature of the first identified CYBASC protein, the cyt b561 from bovine chromaffin vesicles of adrenal medulla (Bcytb561-CG), is that its differential visible absorbance spectra (visible-spectra) revealed an asymmetric α-band with a maximum at 562 nm and a clear shoulder at 557 nm. This feature was recently used to discriminate CYBASC proteins from not-CYBASC proteins. However, in this thesis, it is shown for the first time that not all CYBASC proteins display in their reduced-minus-oxidized visible-spectra an asymmetric α- band and therefore, this feature can not be used as a discriminating CYBASC characteristic. 4. Ascorbate dependent reduction of the A. thaliana CYBASC proteins is inhibited by diethylpyrocarbonate (DEPC). As previously reported for the Bcytb561-CG, the ascorbatedependent reduction of the A. thaliana CYBASC proteins was inhibited by DEPC treatment. In addition, the ‘ascorbate protectant’ effect against DEPC that was observed on the Bcytb561-CG was also observed on the Acytb561-A and Acytb561-B proteins. Furthermore, as the physiological electron donor of all CYBASC proteins is supposed to be ascorbate, ascorbate-affinity of Acytb561- A and Acytb561-B was monitored and was found to be in the same range of the one of the Bcytb561- CG. 5. A. thaliana CYBASC proteins are Fe3+-chelate reductases. Recently, the Fe3+-chelate reductase activity of various CYBASC proteins was presented. In this thesis, it is shown that also both A. thaliana CYBASC proteins reduced Fe3+-chelates such as Fe3+-EDTA and Fe3+-citrate. Consistently, heme potentiometric reductive-oxidative titration of purified Acytb561-A and Acytb561-B indicated that the midpoint potential of the two heme centres of both cytochromes was lower than the one of those Fe3+-chelates. The values of both heme centre potentials of Acytb561-A and Acytb561-B are also consistent with the observation that both cytochromes were only partially reducible by ascorbate and were fully reduced with the non-physiological reductant Na-dithionite. In summary, this work describes the heterologous production, purification and initial characterizations of two distinct CYBASC proteins from A. thaliana: Acytb561-A and Acytb561-B. Biochemical characterization of these cytochromes showed that the shape of the α-band in the differential spectra is not a discriminating factor for CYBASC proteins but it is likely the DEPC sensitivity and the Fe3+-chelate reductase activity. Establishment of a purification strategy to obtain sufficient amounts of monodispersed and stable A. thaliana CYBASC proteins has also enabled initial screening of three dimensional crystallization conditions which are a prerequisite for a deeper understanding of this new eukaryotic redox enzyme family.
All living organisms exhibit daily fluctuations in biochemical, physiological and behavioural parameters driven by endogenous oscillators, residing in the organism itself. In mammals, the core circadian oscillator is located in the paired suprachiasmatic nuclei (SCN) of the hypothalamus. Circadian rhythm generation in the SCN depends upon the expression of clock genes interacting in positive and negative transcriptional/translational feedback loops. The SCN governs the timing of peripheral circadian oscillators by neuronal pathways and by neuroendocrine mechanisms. An important neuroendocrine hand of the core circadian oscillator is melatonin, which is produced in and secreted from the pineal gland night by night. The adenohypophysis represents a peripheral circadian oscillator and the secretion of one of its hormones, prolactin, is known to be regulated by melatonin. The aim of the present study was to analyze a putative influence of melatonin on the activity state and diurnal variations of identified cell types in the hypophysis. Particular attention was paid to lactotroph, gonadotroph and pars intermedia cells. Experiments were performed with young male mice of different strains: melatonin-proficient C3H, melatonin-deficient C57BL, melatonin-proficient C3H with targeted deletions of the Mel1a receptor (MelaaBB), Mel1b receptor (MelAAbb) or both receptors (Melaabb). Cells producing prolactin (PRL), follicle stimulating hormone (FSH) were immunocytochemically identified and the presence of phosphorylated CREB protein (pCREB) and clock gene protein PER1 was demonstrated by double immunolabeling at different time points during the light/dark cycle in melatonin deficient, melatonin proficient and melatonin receptor knockout mice. Melatonin influence on Prl mRNA levels was investigated by means of in situ hybridization. At night the percentage of lactotroph cells showing a positive nuclear pCREB- and PER1-immunoreaction is significantly smaller in C57BL than in C3H mice. In both mouse strains, the percentage of pCREB –immunoreactive cells is minimal in the early morning and gradually increases to reach a maximum in the late night. PER1 levels show a parallel temporal variation in C3H, but in C57BL, they are drastically reduced in the early afternoon. The percentage of FSH-immunoreactive cells showing pCREB immunoreaction was significantly lower in the melatonin-deficient C57Bl mice than in the melatonin-proficient C3H mice during the second part of the day and during the night. In each strain, the percentage of FSH-immunoreactive cells was lowest at the early morning and gradually increases until the maximum at late night. In wild type (MelAABB) and MelAAbb mice the percentage of lactotroph cells with nuclear pCREB immunoreactions varied significantly over 24 h period, whereas in MelaaBB and Melaabb mice no significant differences were found between the five time points analyzed. The number of Prl mRNA expressing cells was significantly higher in MelaaBB and MelAAbb than in their wild type (MelAABB) littermates. pCREB levels in the pars intermedia did not show rhythmic variation in wild type or Melaabb animals, but wild type mice had higher pCREB levels than Melaabb. The observation that, during darkness, the percentage of lactotroph cells with nuclear pCREB immunoreaction is significantly higher in C3H than in C57BL mice suggests the existence of a distinct cell population that is under the control of melatonin-dependent intrapituitary signaling. Results with melatonin receptor knockout mice indicate that Mel1a and Mel1b melatonin receptors are involved in the control of the activity state of lactotroph cells, but to a differing degree. Analysis of cells expressing Prl mRNA showed that inhibitory action on the Prl expression is mostly mediated through the Mel1a receptor. The significant difference between pCREB immunoreaction in gonadotroph cells of C3H and C57BL mice might suggest that, like lactotrophes, FSH cells represent a heterogeneous population and only a subpopulation is under control of melatonin signaling. The present study is first to show that melatonin signaling also affects pCREB levels in pars intermedia of mice.
To determine the effects of inhaled IL-10 at different doses and different time points on the pulmonary and systemic inflammatory response during endotoxemia, 48 ventilated, anaesthetized rats (mean body weight ± standard deviation, 500 ± 33g) were randomly assigned to six groups (n = 8, each). Interleukin-10 was nebulised either prior to or following the intravenous injection of LPS (5mg/kg) at two doses (5.0 mycro-g or 0.5 mycro-g) in our groups. Eight rats received the same insult with no further treatment (LPS-only group). Another eight rats served as controls without endotoxemia but with aerosolized phosphate-buffered saline, the solvent of IL-10 (Sham group). Concentrations of TNF-alpha, IL-1beta, IL-6, and IFN-gamma were analyzed in plasma and bronchoalveolar lavage fluid (BALF). In addition, the nitrite release from ex-vivo cultured alveolar macrophages was determined. As compared to the LPS-only group, the concentrations of the proinflammatory cytokines TNF-alpha, IL-1beta, IL-6, and IFN-gamma in plasma were significantly reduced in the group, which inhaled 5 mycro-g IL-10 before LPS injection (p< 0.0125). Spontaneous nitrite release from exvivo cultured alveolar macrophages was suppressed in this group (p< 0.0125). Inhalation of 0.5 mycro-g IL-10 before LPS injection and both dosages of IL-10 inhalation (5 mycro-g or 0.5 mycro-g) after LPS injection did not significantly influence either inflammatory cytokine concentrations in BALF, in plasma or the nitrite release from ex-vivo cultured alveolar macrophages. In this study, inhaled IL-10 only demonstrated anti-inflammatory effects when it was administered at 5 mycro-g prior to the induction of experimental endotoxemia. Interleukin-10 aerosol had no effect when it was given either following induction of endotoxemia or given at a lower dosage (which here was 0.5 mycro-g) either before or following injection of lipopolysaccharide.
Intrinsic response properties of auditory thalamic neurons in the Gerbil (Meriones unguiculatus)
(2007)
Neurons in the medial geniculate body (MGB) have the complex task of processing the auditory ascending information from the periphery and a more extensive descending input from the cortex. Differences in the pattern of afferent and efferent neuronal connections suggest that neurons in the ventral and dorsal divisions of the MGB take different roles in this complex task. The ventral MGB (vMGB) is the primary, tonotopic, division and the dorsal MGB (dMGB) is one of the higher order, nontonotopic divisions. The vMGB neurons are arranged tonotopically, have sharp tuning properties, and a short response delay to acoustic stimuli. The dMGB neurons are not tonotopically arranged, have broad tuning properties, and a long response delay to acoustical stimuli. These two populations of neurons, with inherently different tasks, may display differences in intrinsic physiological properties, e.g. the capacity to integrate information on a single cell level. Neurons of the ventral and dorsal divisions of the MGB offer an ideal system to explore and compare the intrinsic neuronal properties related to auditory processing. Coronal slices of 200 μm thicknesses were prepared from the thalamus of 4 - 5 week old gerbils. The current-clamp configuration of the patch-clamp technique was used to do experiments on the dorsal and ventral divisions of the medial geniculate body. Slices were subsequently Nissl stained to verify the location of recording. Recordings from the dorsal and ventral divisions exhibited differences in response to depolarizing current injections. The ventral division responded with significantly shorter first spike latency (vMGB = 41.50 ± 7.7, dMGB = 128.43 ± 16.28; (p < 0.01)) and rise time constant (vMGB = 6.95 ± 0.90, dMGB = 116.67 ± 0.13; (p < 0.01)) than the dMGB. Neurons in the dorsal division possessed a larger proportion of slowly accommodating neurons (rapidly accommodating: vMGB: 89%, dMGB: 64%), including a subpopulation of neurons that fired at resting membrane potential. Neurons in the vMGB are primarily responsible for relaying primary auditory input. Dorsal MGB neurons relay converging multimodal input. A comparative analysis with the primary auditory neurons, the Type I and Type II spiral ganglion neurons, reveals a similar pattern. Type I neurons relay primary auditory input and exhibit short first spike latencies and rise time constants. The Type II neurons relay converging input from many sources, while possessing significantly slower response properties and a greater subpopulation of slowly accommodating neurons. Hence, accommodation, first spike latency, and rise time constant are suggested to be a reflection of the amount of input that must be integrated before an action potential can be fired. More converging input correlates to slower accommodation, a longer first spike latency and rise time. Conversely, a greater capacity to derive discrete input is associated with rapid accommodation, along with a short first spike latency and rise time.
The main subject of the thesis is the investigation of low-temperature-grown (LTG) GaAs-based photoconductive switches used in the generation of continuous-wave (CW) and pulsed terahertz (THz) radiation. The use of photoconductive switches based on low-temperature-grown GaAs proved to be a viable option in generating electromagnetic transients on a subpicosecond time-scale, corresponding to frequencies of ~1012 Hz (between microwave and far-infrared). The most appealing property of LTG-GaAs is the ultra-short carrier lifetime obtained by incorporation of a large number of As defects when GaAs is grown at low temperatures. However, the reason for poor THz emission efficiency (low CW-THz power lrvrls) is still up to this date not fully understood. The various reasons are to be found in both, optoelectronic properties of the active layer (photoconducting material) as well as in the device characteristics. The thesis focuses primarily on the limitation imposed to the performance of the THz emitters by the material of choice for the active layer (LTG-GaAs) and secondarily, on the impact of a particular emitter design on the THz radiation efficiency. In the beginning of the thesis one finds an ample overview on the electrical and optical properties of the LTG-GaAs material. A special chapter deals with the main features of current-voltage and CW-THz emission characteristics measured from a photoconductive antenna employed as photomixer. We observed deviations from the theoretical predictions of photomixing theory which were explained by considering the high-field electrons effects (velocity overshoot and elongation of the carrier trapping time). With the scope to provide a better understanding of the correlation between device and material properties when the LTG-GaAs material is integrated with a planar antenna (photoswitch), a special THz double-pulse technique (THz-pump and -probe) was implemented. The experimental results assisted by modeling of the double-pulse THz data provide a gainful insight into the ultrafast dynamics of the electrical field and photogenerated carriers. The outcome of the double-pulse experiments is the evidence for long-living carriers in the LTG-GaAs-based photoconductive antenna under applied bias, with a deleterious impact upon the emitter performance (especially for the CW case). Additionally, by measuring the THz transients generated by a constant laser pulse with and without a CW laser background illumination, we obtained further evidence of strong field-screening effects. This phenomenon was also attributed to the existence of long-living space-charge effects. For both cases (pulsed as well as CW) we derived the de-screening time constant. The principal conclusion of the present study is that, besides shortcomings imposed by the THz-circuitry, photomixers based on materials with traps (defects) exhibit great “affinity” for space-charge screening effects with cumulative and therefore long-lived deleterious impact upon device’s performance. An alternative would be the usage of a transient-time limited device where the response time is given by the carrier collection time, possibly with only one type of carrier responsible for THz signal generation.
Das genetische Material der Zellen besteht aus Molekülketten der Desoxyribonukleinsäure (DNA), die ein Träger der Erbinformation ist. In normalen Körperzellen wird die Erbinformation der DNA in eine andere Molekülkette, die sogenannte Ribonukleinsäure (RNA), übersetzt. Die RNA reguliert die Bildung von neuem Protein in der Zelle. Dass die RNA nicht bloß ein „Stempel“ ist, der die Informationen der DNA weitervermittelt, darin sind sich die Experten heute einig. RNA-Moleküle können Informationen speichern, katalytische Aktivitäten entfalten, sich perfekt tarnen, und sie regulieren auch als Produkt ihre eigene Synthese. Manche Viren enthalten ebenfalls RNA (oder DNA) und können so den Produktionsapparat der Zelle täuschen. Erkenntnisse über die Wechselwirkung dieser RNA mit natürlichen und synthetischen Liganden können zur Suche nach potentiellen Wirkstoffen beitragen. Nukleinsäuren sind lineare Biopolymere von grundlegenden Untereinheiten, die Nukleotide genannt werden und aus Adenin (A), Cytosin (C), Guanin (G), Urazil (U), und Thymin (T) zusammengesetzt sind. Sie sind jedoch in der Lage sich zu falten und so eine Doppel-Helixstruktur auszubilden. Diese besteht größtenteils aus den bekannten "Watson-Crick-Basenpaaren" (G-C und A-U oder A-T), die zur Stabilität der Struktur beitragen, sowie aus den weniger stabilen G-U-Paaren. Durch die Wechselwirkung zwischen verschiedenen Sekundärstrukturelementen entstehen Tertiärstrukturelemente, deren Struktur und Dynamik oft nur schwer experimentell zu bestimmen sind. Fortschritte in der RNA-Strukturanalyse wurden durch Röntgenkristallographie und Kernresonanzspektroskopie (NMR) möglich. Durch die Röntgenkristallographie wurden viele RNA-Eigenschaften festgestellt. Allerdings besteht keine Kristallstruktur für alle mögliche Einzelnfaser-RNA-Haarnadeln, weil diese immer dazu neigen, in eine linearen doppelte Faserform zu kristallisieren, die geringe biologische Bedeutung hat. Außerdem wurde mit Hilfe der NMR-Spektroskopie das dynamische Verhalten von RNA, z.B. Entfaltungsprozesse bei ansteigender Temperatur, beobachtet. Jedoch erlauben diese experimentellen Daten oft keine direkte mikroskopische Beschreibung der molekularen Prozesse. Molekulardynamik (MD)-Simulationen von biologischen Systemen ermöglichen es hingegen, diese Prozesse in atomischem Detail zu untersuchen. Die MD-Simulation beschreibt ein molekulares System auf atomarer Ebene mit Hilfe der klassischen Mechanik. Kräfte werden von empirischen Potentialen abgeleitet. Sie liefern zeitabhängige Trajektorien, die sich aus den Newton'schen Bewegungsgleichungen ergeben. Durch verbesserte Computerleistung, bessere Kraftfelder, und neu entwickelte genauere Methoden stimmen heutzutage MD-Simulationen von RNA mit experimentellen Daten immer besser überein. In meiner Doktorarbeit wurden MD-Simulationen durchgeführt um die Dynamik, die Struktur und insbesondere die Stabilität von RNA-Hairpins theoretisch zu beschreiben, um so ein erweitertes Verständnis für die dynamischen Vorgänge zu erhalten. Auch der SFB 579 der Universität Frankfurt beschäftigt sich mit RNA-Systemen. Erforscht wird unter anderem der D-Loop des Coxsackievirus B3 (CVB3), der Virenmyocarditis verursacht. Die Interpretation dieser experimentellen Daten wird durch MD-Simulation möglich. In dieser Arbeit wurden das GROMACS Software-Paket und das AMBER Kraftfeld verwendet, um das strukturelle, dynamische und thermische Verhalten der RNA-Hairpins mit Hilfe von MD-Simulationen auf atomarer Ebene zu untersuchen. Betrachtet wurden die 14-mer RNA-Hairpins, uCACGg und cUUCGg. Die verfügbaren NMR-Strukturen zeigen, dass das uCACGg-Tetraloop auffallend ähnlich in der gesamten Geometrie und den Wasserstoffbindungen zu der experimentellen Struktur des cUUCGg-Tetraloop ist, obwohl die schließende Basenpaarsequenz der beiden Tetraloops unterschiedlich sind. Trotz beachtlicher struktureller Ähnlichkeit unterscheiden sich allerdings die uCACGg und cUUCGg Tetraloops in Funktionalität und Thermostabilität. Zunächst orientiert sich unser erstes Bemühen an der Frage nach einem guten Modell für RNA-Hairpins und Simulationsbedingungen, um die zu untersuchenden RNA-Hairpins in Wasser möglichst realitätsnah zu simulieren. Erstens werden drei Versionen des biomolekularen AMBER-Kraftfelds geprüft, indem man die 60 ns Simulationen des 14-mer uCACGg-Hairpins durchführt. Die simulierten strukturellen Eigenschaften und Atomfluktuationen zeigen hohe Ähnlichkeiten in den drei Kraftfeldern. Darüber hinaus stimmen die von MD-Simulationen berechneten Atomkernabstände mit den experimentellen NMR-Daten gut überein. Die gute Übereinstimmung zwischen den Simulationen und den strukturellen NMR Daten belegt die Fähigkeit des AMBER-Kraftfelds zur Beschreibung der strukturellen Eigenschaft von kleinen RNA-Hairpins. Anschließend werden die Einflüsse der Methoden, welche die langreichweitigen, elektrostatischen Wechselwirkungen beschreiben, auf die strukturellen Eigenschaften untersucht. Insbesondere werden die Ergebnisse der Reaktionfeld-Methode mit denen der Particle Mesh Ewald (PME)-Methode verglichen. Es zeigt sich, dass die PME-Methode die elektrostatischen Wechselwirkungen am besten beschreibt, auch wenn die Simulationen der beiden Methoden Ähnlichkeit in der Struktur-Stabilität und der Atomfluktuation bei niedriger Natriumkonzentration aufweisen. Drittens wird der Kationseffekt auf die RNA-Stabilität untersucht. Betrachtet wurden zwei unterschiedliche Kationen (ein- und zweiwertig) und verschiedene Konzentrationen. Die Simulationen weisen darauf hin, dass sich die Metallionen in der Affinität zum RNA-Hairpin unterscheiden, wenn Na+ und/oder Mg2+ als Gegenionen verwendet werden. Weiterhin wird gezeigt, dass sich die bevorzugten Positionen der Na+-Ionen in der großen Furche (major groove) des RNA-Hairpins befinden. Insbesondere die Anlagerungsort der Na+-Ionen liegen in der Nähe des schließenden Basenpaar U5-G10. Im Vergleich zu Na+-Ionen lagern sich Mg2+-Ionen sowohl an die RNA-Basen U3, A4-U11, und die Phosphat-Gruppe, als auch an das schließenden Basenpaar U5-G10 an. Bestätigt werden die Modelle und Simulationsbedingungen durch den Vergleich von Parametern, die sowohl experimentell als auch durch Simulationen ermittelt werden können. Ferner erlauben MD-Simulationen Einblick in das System, indem sie detallierte Konformations- und andere Verteilungen liefern. In der vorliegenden Arbeit wurden die Einflüsse der Loopsequenz und des schließenden Basenpaares auf die Verteilung der Konformationen, der internen Bewegungen, und auf die Thermostabilität von zwei RNA-Hairpins mit Hilfe dieser Modelle untersucht. Zunächst wurden die strukturellen Eigenschaften bei Raumtemperatur ausgewertet. Die starken strukturellen Ähnlichkeiten und die gute Übereinstimmung mit NMR-Daten bestätigen die Hypothese, dass die zwei Tetraloops zur gleichen “erweiterten” RNA-Familie gehören. Diese zwei Hairpins haben ähnliche Lösemittelzugängliche Oberflächen (solvent accessible surface), wobei deren Lösemittel zugänglichen funktionellen Gruppen unterschiedlich sind. Weiterhin weist das uCACGg-Hairpin eine stärkere Tendenz auf Wasserstoffe abzugeben als das cUUCGg-Hairpin, was in den unterschiedlichen Bindungsaffinitäten zwischen diesen Hairpins und der viralen Protease begründet liegt. Darüber hinaus wurde der Faltungs- und Entfaltungsprozess mit Hilfe der Replica-Exchange-Molekulardynamik-Simulationen untersucht. Diese Untersuchung zielt auf das bessere Verständnis der unterschiedlichen Thermostabilität der Hairpins, indem sie die möglichen Zwischenprodukte im atomaren Detail liefern. Sowohl experimentell als auch von den MD-Simulationen ergibt sich eine Differenz in den Schmelztemperaturen der beiden Hairpins von ungefähr 20 K. Allerdings sind die von MD beobachteten Schmelztemperaturen 20 % höher als die von Experiment zu ansehende Wert. Die Ergebnisse machen deutlich, dass die Schmelztemperaturdifferenz nicht auf die Unterschiede in der Sequenz, in der Struktur, oder in der Dynamik der Loops zurückführen sind, sondern auf die Unterschiede der Basenpaaren in den Stämmen. Weiterhin wird gezeigt, dass sich das uCACGg-Hairpin einerseits kooperativ entfaltet, und die Entfaltung des cCACGg-Hairpins anderseits weniger kooperativ stattfindet. Um die schnelle interne Dynamik der uCACGg- und cUUCGg-Hairpins zu untersuchen, erlauben die Simulationen von 50 ns eine akurate Beschreibung der schnellen internen Bewegung der RNA-Hairpin, obwohl der den Hairpins zugängliche Konformationsraum nicht vollständig abgedeckt wird. Die NMR-Relaxationsparameter, die mit Hilfe der MD-Simulationen zurückgerechnet wurden, bestätigen das Modell und die Simulationsbedingungen der MD-Simulationen. Im Hinblick auf die Übereinstimmung kann man den besten Ansatz zur Berechnung der NMR-Ordnungsparameter bestimmen. In dieser Arbeit wurden drei verschiedene Ansätze angewandt, nämlich das Fitting von 100 ps auf modellfreiem Ansatz nach Lipari-Szabo, equilibrium average, und das Gaussian Axial Fluctuation (GAF)-Modell. Die zwei letzteren können nur qualitativ mit den experimentellen Daten übereinstimmen. Die NMR-Ordnungsparameter können mit Hilfe des Modells von Lipari-Szabo richtig ermittelt werden, wenn sich die interne Bewegung in kleineren Zeitskalen als zur Gesamtbewegung vollzieht. Vorausetzung für die Berechnung dieses Modells ist aber, dass das Fitting der internen Korrelationsfunktionen nur auf den ersten Teil von 100 ps der Korrelationsfunktionen eingesetzt wird. Die berechneten Ordnungsparameter deuten auf ein unterschiedliches Verhalten der beiden Hairpins besonders im Loop-Bereich hin. Die konformationelle Umordnung, die beim UUCG-Loop beobachtet wurde, tritt beim CACG-Loop nicht ein. Zusammenfassend lässt sich sagen, dass es durch den Einsatz von MD Simulationen ermöglicht wird, die strukturellen und dynamischen Eigenschaften der RNA-Systeme auf atomarer Ebene zu untersuchen. Als Schlussfolgerung zeigt diese Doktorarbeit, dass sich die Studie der konformationell Dynamik der RNA-Systeme durch die Kombination aus MD-Simulation und NMR-Spektroskopie sowie der Leistungsfähigkeit der MD-Simulationen, die die interne Bewegungen deutlich beschreiben können, untersuchen lässt.
A detailed understanding of how potassium channels function is crucial e. g. for the development of drugs, which could lead to novel therapeutic concepts for diseases ranging from diabetes to cardiac abnormalities. An improved understanding of channel structure may allow researchers to design medication that can restore proper function of these channels. This is particularly important for KCNQ channels, since four out of five family members are involved in human inherited disease. In addition to structure and function relationships the determinants which govern assembly of KCNQ subunits are decisive to understand the physiological role of the KCNQ channel family members. Many details of KCNQ channel assembly remain incompletely understood. Previous work has shown that the subunit-specific heteromerisation between KCNQ subunits is determined by a ~115 amino acid-long subunit interaction domain (si) within the C-terminus (Schwake et al., 2003). Recently, Jenke et al. (2003) proposed that the C-terminal domains in eag and erg K+ channels act as sites which drive tetramerization. From their ability to form coiled coils, these domains were referred to as tetramerizing coiled-coil (TCC) sequences. Jenke et al. also pointed out that KCNQ channels contain bipartite TCC motifs within their C-termini, exactly within the si domain, which is responsible for the subunit-specific interaction pattern. The first part of this thesis was dedicated to determine the individual role of these TCC domains on homomeric and heteromeric channel formation in order to further characterize the molecular determinants of KCNQ channel assembly. In the second part of this thesis cystein-scanning mutagenesis was employed, followed by thiol-specific modification using MTS reagents to screen more than 20 residues in the S3-S4 linker region and in the S4 transmembrane domain of the KCNQ1 channel to gain information about residue accessibility, the functional effects of thiol-modifying reagents (MTSES), and effects of crosslinking selected pairs of Cys residues by Cd+ ions, which could be used for testing model predictions based upon known Kv channel structures from the literature. According to homology modelling based on the Kv1.2 structure it was attempted to determine the proximity of individual residues from different transmembrane segments using the metal bridge approach (crosslinking by Cd+ ions). This led us to derive structural constraints for interactions between the S4 voltage sensor and adjacent transmembrane segments of KCNQ1. Similar studies have previously been performed on the Shaker K+ channel, which has served as a paradigm for structure-function research of voltage-gated K+ channels for a long time, but little is known for KCNQ channels concerning their similarity to published K+ channel structures.
NE Mount Kenya is characterised by dense population and small scale farming is the main form of land use. In the region, continual pressure on the forest resources as result of land use is a continuing problem. The NE Mount Kenya Forest Reserves (Imenti Forest Reserve, Mount Kenya Forest Reserve) play an important role in the livelihood of the neighbouring communities. However population pressure, reserve management policies, economic changes, an ineffective land tenure system and poverty are socio-economic factors contributing to land use changes and an intensification of agriculture. Illegal factors like clearing forest vegetation for firewood and grazing areas, at the expense of the protected forest areas, are present. This study focuses on an interdisplinary approach to analyse socio-economic and ecological factors in NE Mount Kenya relevant to land degradation. This includes remote sensing data (interpretation of satellite images Landsat TM 1987 and ETM 2000) combined with interviews from the land user’s perspective. Ethnographic research of this type on this topic has not been done in the region before. This entailed applying both a qualitative (giving farmers the opportunity to identify factors they perceived as important in regard to land use) and a quantitative method of data analysis. The Mount Kenya Forest region is distinguished by high elevation and a humid to sub-humid climate, while the Imenti Forest region lies lower and is characterised by semi-humid and transitional zones. Land use in the Mount Kenya Forest region is mainly perennial thus eliminating seasonal land use changes. In the Imenti Forest region, 30% of the farmers said they had gone through major land use changes within the last 20 years. The major land use change consisted of a shift from residential farming in the protected areas which offered more farming and grazing areas, to being restricted to individual farm plots which consequently led to the intensification of cultivation thus contributing to land degradation. The satellite images in the same region show a clear decrease in coverage of forest vegetation and an increase in open areas in the Imenti Forest region which the farmers explain influences the tentative land use changes in the region. On the other hand, in the Mount Kenya forest region, there has been an increase in forest vegetation cover which is also evident in the satellite images. Areas that were plantation and cultivated regions in 1987 have forest cover in 2000, which the farmers stated was as a result of their afforestation initiatives. Nevertheless, indicators of degradation e.g. rill and gully erosion are evident and correlated to the intensified land use in both forest regions. The population impact in the region apparently intensifies land use therefore the identified socio-economic factors in the region should be given priority in integrating development projects that are directly beneficial to park-adjacent communities according to the needs of the particular agro-ecological zone (AEZ). Location specific research can better enhance the understanding of the socio-economic factors influencing land use change. Furthermore, promoting alternative income generating activities, besides the present livestock and crop farming, can help reduce the risks of land degradation.
Leukemia inhibitory factor enhances neurogenin's pro-neural effect during mouse cortical development
(2007)
Die Entwicklung von unterschiedlichen Zelltypen waehrend der embryonalen ZNS-Entwicklung ist abhaengig von zellintrinsischen und positionsabhaengigen, aeusseren Einfluessen. Dabei bilden sich die verschiedenen Zellen in nacheinander ablaufenden bzw. sich teilweise ueberlappenden Zeitraeumen. Zuerst entstehen Radiaglia und Neuronen, nachfolgend Astrozyten und zuletzt Oligodendrozyten. Werden neurale Stammzellen/Vorlaeuferzellen (NPCs – neural precursor cells) zu unterschiedlichen Zeitpunkten entnommen und ohne den Einfluss von Wachstumsfaktoren kultiviert, so entwickeln sich diese Zellarten in der gleichen Reihenfolge. Die Neurogenese, die bei Mausembryos am Tag E11-12, nach dem Etablieren der Radialglia, beginnt, findet an E14 ihren Hoehepunkt. Zu diesem Zeitpunt werden die Gene Neurogenin1 (Ngn1) und Ngn2 in den neuralen Vorlaeuferzellen der Ventrikularzone des dorsalen Cortexes in hohem Masse exprimiert. Wie aus Untersuchungen von unserm Labor gezeigt wurde, beguenstigt es die Entstehung von Neuronen und blockiert gleichzeitig Pro-Astrozyten-Einfluesse. Zum einen inhibiert Ngn den JAK/STAT Signalweg, dessen Aktivierung fuer die Gliogenese noetig ist, indem es die Phosphoylierung von STAT1/3 auf bisher noch unbekannte Weise blockiert. Ausserdem bindet der Transkriptions-Coaktivator cAMP-response element binding protein (CBP), welches auch von den STATs fuer die Transkription benoetigt wird, bevorzugt an Ngn sobald dieses von den Vorlaeuferzellen exprimiert wird. Mit dem Tag E16 nimmt die Neurogenese in vivo wieder stark ab und es setzt die Gliogenese ein, bei der zunaechst ueberwiegend Astrozyten gebildet werden. Faktoren wie leukemia inhibitory factor (LIF) sowie ciliary neurotrophic factor (CNTF) beguenstigen dabei die Astrozytogenese indem sie den JAK/STAT Signalweg aktivieren. Die Bindung von LIF/CNTF fuehrt zur Phosphorylierung von STAT-Transkriptionsfaktoren, die ihrerseits dann an den CBP/p300 Komplex binden und schliesslich die Expression von Astrozyten-spezifischen Genen aktivieren. Die STAT-Faktoren koennen aber erst nach Abfall des Ngn-Spiegels an den Transkriptions-Coaktivator binden, da sich die Bindungsstellen dieser beiden ueberlappen. Um die Hypothese zu ueberpruefen, dass LIF auch die Neurogenese, oder spezifischer, die Wirkung von Ngn positiv beeinflusst, wurden cortikale NPCs von murinen Embryos entnommen und der Wirkung von LIF via Luciferase Assay untersucht. Dabei wurden die Vorlaeuferzellen mit Ngn und einem Reporter transfiziert, welcher den NeuroD-Promoter beinhaltete. NeuroD-Expression findet in der Regel gegen Mitte/Ende der Neurogenese statt und ist wichtig fuer die Reifung von Neuronen. Der Promoter von NeuroD beinhaltet ein E-box Element, an welches Ngn bindet und die Transkription einleitet. Wie unsere ersten Versuche zeigten, verstaerkt LIF die Transkriptionsaktivitaet von Ngn und somit die Transkription von NeuroD. Wenn aber im selben Versuch ein NeuroD-Reporter transfiziert wurde, dessen E-box mutiert war, wurde keine Transkriptionsaktivitaet gemessen, was wiederum bestaetigte, dass der pro-neurale LIF-Effekt ueber Ngn lief und E-box-Bindung noetig war. Um den Einfluss des pro-neuralen Effekts von LIF auf Proteinebene zu testen, wurden NPCs mit Ngn-Adenovirus infiziert und mit LIF stimuliert. Dabei wurden die Zellen auf die Expression von Neuron-spezifischem class III β-tubulin (TuJ1) untersucht. Die Ergebnisse zeigten, dass LIF bei Zellen, die Ngn exprimierten, die Rate der Neuronen von etwa 5% auf etwa 50% anstiegen liess, waehrend LIF bezueglich der Gliogenese (gezeigt durch die Expression von GFAP) in Ngn-exprimierenden Vorlaeuferzellen kaum Wirkung zeigte. Als naechstes sollte untersucht werden ueber welchen Signalweg LIF Ngn aktivierte. LIF bindet zunaechst an LIF receptor β (LIFRβ), der dann an glycoprotein 130 (gp130) bindet. Diese Bindung fuehrt dann zur Aktivierung mehrerer Signalkaskaden: dem JAK/STAT, dem MAPK, dem Akt/PI3K und dem PLCγ/PKC Signalweg. Da der JAK/STAT Signalweg fuer die Gliogenese wichtig ist, lag unser Fokus auf den anderen Signalwegen. Deren Aktivierung wurde dann mit spezifischen Inhibitoren blockiert und, wie auch in den Vorversuchen, die Wirkung von LIF auf Transkriptionsebene (NeuroD) in neuralen Vorlaeuferzellen bestimmt. Dabei zeigte sich, dass die Blockierung des PLCγ/PKC Signalweges die NeuroD-Promoteraktivitaet am starksten inhibierte, waehrend auch LIF´s pro-neurale Wirkung verloren ging. Dementsprechend zeigte die Western Blot Analyse, dass die Expression von class III β-tubulin (TuJ1) durch die Anwendung der PKC Inhibitoren am staerksten inhibiert wurde, wobei auch hier die Stimulation durch LIF keine erhoehte Neurogenese mit sich zog. In weiteren Versuchen konnten wir dann mit Hilfe von Immunoprezipitation demonstrieren, dass LIF die Bindung von Ngn an CBP verstaerkte (eine Bindung, welche durch PKC Inhibitoren aufgehoben wurde), was wiederum zu einer erhoehten Bindung dieses Transkriptionskomplexes an den NeuroD Promoter fuehrte, wie unsere Chromatin Immunoprezipitation (ChIP) Daten beweisen. Dies wiederum laesst darauf schliessen, dass womoeglich diese erhoehte Ngn-CBP/NeuroD-Promoter Bindung der Grund fuer die erhoehte NeuroD-Transkriptionsaktivitaet ist daher auch fuer die erhoehte neuronale Differenzierung. Interessanterweise konnten wir auch zeigen, dass Brahma-related gene 1 (Brg1), eine katalytische Untereinheit des SWI/SWF Komplexes, an den Ngn/CBP cotranscriptionalen Komplex bindet und dass diese Bindung durch LIF-Stimulation verstaerkt wurde. Dies suggeriert wiederum, dass auch Brg1 eine wichtige Rolle waehrend der murinen, cortikalen Neurogenese spielt. Dennoch, in folgenden Experimenten verblieb der Fokus auf Ngn und CBP. Um unsere Hypothese zu bestaetigen, dass PKCδ ein moeglicher Mediator des LIF-Effekts sein koennte, zeigten wir zunaechst, dass die PKCδ-Expression in cortikalen NPCs waehrend der Neurogenese erhoeht ist. Desweiteren demonstrierten wir, dass die Inhibition von PKCδ einen aehnliche Wirkung zeigte wie die Inhibition von PKC mit einem generellen PKC Inhibitor: weder war nach PKCδ-Inhibition eine LIF-induzierte NeuroD-Transkription erzielbar, noch wurde nach LIF-Stimulation der pro-neurale Marker class III β-tubulin/TuJ1 in Ngn1-infizierten NPCs exprimiert. Um aber mehr spezifisch die PKC- und PKCδ-Aktivitaet/Expression zu blockieren transfizierten wir NPCs mit PLCγ oder PKCδ siRNA. Unsere Daten zeigten hierbei, dass siRNA-transfizierte Zellen kein class III β-tubulin mehr aufweisen, was darauf hindeuted, dass PKCδ der potentielle Mediator des pro-neuralen LIF-Effekts ist. Durch unsere in vivo Daten demonstrierten wir schliesslich, dass LIF auch hierbei fuer die Neurogenese von Bedeutung ist. Verglichen wurden die Cortices von E13 LIF Het (heterozygote) und KO (knock out) Maeusen mit denen von WT (wild type) Maeusen. Durch Immunohistologie von Hirnschnitten konnten dabei keine groesseren Unterschiede bezueglich der Expression neuraler Marker beobachtet werden, waehrend aber mit Hilfe der Western Blot Analyse, eine quantitativere Methode, gezeigt wurde, dass LIF Het und KO Maeuse weniger pro-neurale Marker im Cortex exprimieren wie WT Mause. Um auch zu beweisen, dass dies auf eine verringerte Transkription von NeuroD zurueckzufuehren ist, demonstrierten wir mit Hilfe des ChIP Assay, dass LIF Het und KO Maeuse weniger Ngn1-CBP Bindung an den NeuroD-Promoter aufweisen wie WT Maeuse. Diese Experimente veranschaulichen einen eleganten Regulationsmechanismus, durch welchen ein einzelner, extrazellulaerer Faktor die unterschiedliche Differenzierung einer Zelle verstaerkt, abhaengig von der Anwesenheit oder Abwesenheit eines einzelnenn intrazellulaeren Faktors. Auch koennen durch die erlangten Resultate Strategien entworfen werden, durch die in Zukunft die Produktion bestimmter Neurone zur Heilung von verschiedenen, neurodegenerativen Krankheiten erhoeht wird.
The search for a modification of hadron properties inside nuclear matter at normal and/or high temperature and density is one of the more interesting issues of modern nuclear physics. Dilepton experiments, by providing interesting results, give insight into the properties of strong interaction and the nature of hadron mass generation. One of these research tools is the HADES spectrometer. HADES is a high acceptance dilepton spectrometer installed at the heavy-ion synchrotron (SIS) at GSI, Darmstadt. The main physics motivation of HADES is the measurement of e+e- pairs in the invariant-mass range up to 1 GeV/c2 in pion- and proton-induced reactions, as well as in heavy-ion collisions. The goal is to investigate the properties of the vector mesons rho, omega and of other hadrons reconstructed from e+e- decay pairs. Dileptons are penetrating probes allowing to study the in-medium properties of hadrons. However, the measurement of such dilepton pairs is difficult because of a very large background from other processes in which leptons are created. This thesis presents the analysis of the data provided by the first physic run done with the HADES spectrometer. For the first time e+e- pairs produced in C+C collisions at an incident energy of 2 GeV per nucleon have been collected with sufficient statistics. This experiment is of particular importance since it allows to address the puzzling pair excess measured by the former DLS experiment at 1.04 AGeV. The thesis consists of five chapters. The first chapter presents the physics case which is addressed in the work. In the second chapter the HADES spectrometer is introduced with the characteristic of specific detectors which are part of the spectrometer. Chapter three focusses on the issue of charged-particle identification. The fourth chapter discusses the reconstruction of the di-electron spectra in C+C collisions. In this part of the thesis a comparison with theoretical models is included as well. The conclusion and final remarks are given in chapter five.
Die vorliegende Arbeit behandelt die Entwicklung und Überprüfung von Modellen zur Berechnung von Schwingungspektren von Peptiden und Proteinen. Solche Modelle verbinden die Konformationsstruktur eines Moleküls mit seinen Schwingungseigenschaften und sind demzufolge wichtig für die Interpretation der Schwingungspektren. Die im Rahmen dieser Arbeit durchgeführte theoretische Erforschung dieses Gebietes beschränkt sich auf die Betrachtung der Amide-I-Moden, welche aufgrund ihrer physikalischen Eigenschaften sich zur Untersuchung der Peptidkonformationen eignen. Die Arbeit kann prinzipiell in zwei Teile separiert werden. In dem ersten Teil werden Fragen betrachtet, die mit der Entwicklung des Schwingungshamiltonian verbunden sind. Im zweiten Teil wurden die erhaltenen Hamiltonian für die Berechnung der Schwingungspektren verwendet. Bei der Berechnung der Schwingungspektren wurden verschiedene spektroskopische Näherungen verwendet und erforscht. Die Entwicklung des Schwingungshamiltonian beinhaltet zwei Aufgaben. Die ab initio Parametrisierung des Schwingungshamiltonian von Dipeptiden, sowie die Analyse der Entwicklungsmethoden für Schwingungshamiltonian von Polypeptiden. Die Entwicklungsmethoden stützen sich auf ab initio berecheten Schwingungseigenschaften von Dipeptiden und/oder elektrostatische Modelle. Die ab initio Parametrisierung basiert auf einer Geometrieoptimierung und anschließender Berechnung von Normalmoden. Hierbei wurde die Abhängigkeit der Ergebnisse vom theoretischen Niveau und dem verwendeten Basissatz untersucht. Die Transformation der errechneten Normalmoden lieferte die Schwingungseigenschaften der lokale Amide-I-Mode. Die Lokalisierung der Normalmode folgt diversen Kriterien. Sie ist von der Wahl der Lokalmoden und somit implizit auch von der Art der Geometrieoptimierung abhängig. Mit dieser Arbeit konnte die Abhängigkeit der Ergebnisse von der Parameterwahl weitgehend aufgeklärt und eine für das Amide-I-System geeignet Parametrisierung gefunden werden. Im nächsten Arbeitsschritt wurde die Abhängigkeit der Amide-I-Schwingungseigenschaften von den Peptidseitenketten und terminalen Gruppen untersucht. Desweiteren wurden Methoden zur Formulierung der Hamiltonian für Polypeptide konzeptionell entwickelt. Diese Untersuchung ist außerordentlich wichtig, da direkte quantenmechanische Berechnungen von Polypeptiden zu zeitaufwendig sind. Solche Methoden beruhen auf dem sogenannten “Building-Block”-Ansatz und verschiedenen elektrostatischen Modellen. In dieser Arbeit wurden sowohl die einzelnen Methoden als auch ihre Kombination für die Entwicklung des Hamiltonians verwendet. Zur Abschätzung der Genauigkeit der verwendeten Methoden wurden Vergleichsrechnungen durchgeführt. Im zweiten Teil dieser Arbeit wurden die erhaltenen Schwingungshamiltonian zur Berechnung von Schwingungsspektren diverser gelöster Peptide angewandt. In diesem Zusammenhang konnte die Genauigkeit unterschiedlicher spektroskopischer Approximationen überprüft werden. Auf Grundlage der erhaltenen Ergebnisse können wir sagen, dass eine angemessene Beschreibung der konformationellen Verteilung und eine korrekte Berechnung des dynamischen Absorptionsspektrum gewährleistet ist. Was noch fehlt, ist ein hinreichend genaues quantenchemisches Modell für die Schwingungsfrequenzen eines gelösten Peptids. Diese Aufgabe stellt zur Zeit ein aktives Forschungsgebiet dar. Zuletzt wurde das Schwingungsspektrum eines sogenanten “Photoschaltbaren”-Peptids simuliert. Mit Hilfe des dafür aufgestellten Hamiltonians ist man in der Lage spektroskopische Beobachtungen auf Konformationsänderungen direkt zu übertragen.
Molecular mechanism of intracellular signal transduction by the angiotensin-converting enzyme
(2007)
The angiotensin converting enzyme (ACE) is an important component of the renin-angiotensin system (RAS) and is crucially involved in the homeostasis of fluid and electrolyte balance and thus in the regulation of blood pressure. The zinc metallopeptidase is involved in the generation of angiotensin II, a potent vasoconstrictor and in the degradation of bradykinin, a potent vasodilator. It is worth noting that ACE more readily hydrolyzes bradykinin than it does angiotensin I thus culminating in the net physiological effect of the production of a vasoconstrictor and the decrease in the availability of a vasodilator. ACE inhibitors have become one of the most successful therapeutic approaches as a first line of therapy in hypertension, and are also widely used in treating heart failure, myocardial infarction, stroke, coronary artery disease and impaired left ventricular function. However, one unexpected clinically relevant finding related to ACE inhibitors is their ability to delay the onset of type II diabetes that was revealed by various large clinical trials. However, the mechanisms underlying these beneficial effects of ACE inhibitor therapy are currently unclear and cannot be explained by the prevention of angiotensin II formation or the attenuated degradation of bradykinin. Thus the potential beneficial effects attributed to ACE inhibitors may occur independent of reductions in blood pressure paving way for new and/or unknown mechanism. Our group has recently redefined ACE as a signal transduction molecule which upon binding to ACE inhibitor turns on a signalling cascade leading to phosphorylation of Ser1270 by CK2, activation of JNK and changes in gene expression in endothelial cells. However the mechanism by which ACE inhibitor initiates the signalling cascade was not clear. It was hypothesized that ACE, which is anchored to the membrane with a single transmembrane domain should dimerize prior to initiating further downstream signalling events in endothelial cells. Therefore, we sought to explore whether or not ACE forms dimers in endothelial cells and whether ACE dimerization is essential for the initiation of ACE signalling in endothelial cells. Using native gel electrophoresis, we found that ACE forms dimers in endothelial cells and that there is an increase in the dimer formation upon treatment of endothelial cells with ACE inhibitors. ACE homodimerization was also demonstrated using the split-ubiquitin system and chemical cross-linking experiments. ACE dimers are also formed in endothelial cells overexpressing the non-phosphorylatable ACE, wherein ACE signalling was abolished indicating that dimerization process is not influenced by the phosphorylation of the serine residue residing in the cytoplasmic tail. Monosaccharides like glucose, galactose and mannitol did not have any influence on ACE-inhibitor induced dimerization. Making use of different monoclonal antibodies directed to the epitopes of N-domain which harbours carbohydrate recognizing domain, also did not affect dimerization. However, inactivation of the C-domain active site by introducing mutation of the key histidine residues in HEMGH consensus sequences, which complexes the zinc ions, abolished enzyme dimerization both in the basal state and in response to ramiprilat. Mutation of the C-domain also resulted in the loss of ACE inhibitor-induced ACE signalling, that is we failed to observe ramiprilat-induced increase in the phosphorylation of the Ser1270 and the subsequent JNK activation. ACE-inhibitor induced dimerization precedes the phosphorylation of Ser1270 and activation of JNK. Thus the ACE-inhibitor induced dimerization via the C-domain of ACE represents the initial step in the ACE signalling pathway which involves the activation of JNK/c-Jun pathway and leading to the changes in the gene expression in endothelial cells. Our group previously identified ACE itself as well as cyclooxygenase-2 (COX-2) as two “ACE signalling-regulated” genes. To screen for additional genes regulated in a similar manner we used DNA microarray technology, to assess ramiprilat-induced changes in the endothelial cell gene expression. 21 genes were identified to be differentially regulated of which, 7 were upregulated and 14 were downregulated by ramiprilat. However, when screened at the protein level, we found no significant differences between the untreated control cells and those treated with ramiprilat. As several other cells and tissues possess a fully functional RAS we screened plasma samples from healthy volunteers as well as from patients with coronary artery disease for the proteins identified in the microarray. We observed that the cellular retinal binding protein-1 (CRBP-1) was detectable at low levels in plasma from patients and that ramipril markedly increased serum levels of this protein. Endothelial cells overexpressing CRBP-1 demonstrated increased RXRE and PPRE activity when stimulated with 9-cis retinoic acid and rosiglitazone respectively suggesting that CRBP-1 might affect gene expression via heterodimerization of PPAR elements with RXR elements by virtue of its function as a transport protein of retinoic acid. Studies aimed at determining the consequences of elevated CRBP-1 expression on endothelial cell homeostasis are ongoing. Although the RAS has been described in many other tissues apart from endothelial cells, ACE signalling has not yet been addressed in tissues such as monocytes/macrophages, which have an increased ACE expression in an atherosclerotic setting. We observed that upon stimulation of cultured ACE expressing monocytes with ramiprilat, JNK is activated suggesting the occurrence of ACE signalling in human monocytes. It is worth noting that ACE inhibitors delay the onset of type II diabetes in spite of moderate decrease in blood pressure. To further elucidate the mechanism underlying this effect, we found that ACE inhibitors increase the PPARgamma levels in the nuclear extracts of ACE expressing monocytes which were also reproduced in human endothelial cells overexpressing human somatic ACE. However, ramiprilat did not have any direct effect on the activity of a luciferase-coupled promoter containing several copies of the PPRE in human endothelial cells. These results contrasted with the actions of the PPARgamma agonist suggesting that ramiprilat enhances PPARgamma levels through an indirect mechanism. We next hypothesized that ramiprilat might increase the levels of 15-deoxy-D12,14-prostaglandin J2 (15dPGJ2) which is a natural ligand for PPARgamma via COX enzymes in monocytes. We observed that ramiprilat was able to decrease the diminution of COX-2 levels upto 48 hours of treatment but the levels of 15dPGJ2 were too low to be detected by ELISA. However ramiprilat enhanced the plasma levels of adiponectin, a downstream target of PPARgamma, which is a anti-atherogenic and anti-inflammatory adipokine, in patients with coronary artery disease. Though adiponectin is a PPARgamma-regulated gene, the observed increase in adiponectin might be attributed to the increase in RXR rather than via PPARgamma. Taken together, the results of this investigation have revealed that ACE inhibitors initiate ACE signalling by eliciting the dimerization of the enzyme, more specifically via its C-domain active centers. The ACE signalling cascade when activated leads to the enhanced expression of ACE, COX-2 and CRBP-1 which in turn favours the heterodimerization of PPARgamma with RXR and thus results in the increased expression of “PPARgamma regulated” genes such as adiponectin. The latter results provide a molecular basis for the observation that ACE inhibitors can delay the onset of type 2 diabetes in as much as it was possible to link ramipril with CRBP-1, RXR activity and the expression of adiponectin, an adipokine associated with improved insulin sensitivity. Further work is however required to elucidate the consequences of ACE inhibitors in monocytes and adipocytes as well as in intact animals.