Refine
Year of publication
Document Type
- Article (15825)
- Part of Periodical (2818)
- Working Paper (2353)
- Preprint (2085)
- Doctoral Thesis (2065)
- Book (1736)
- Part of a Book (1071)
- Conference Proceeding (753)
- Report (471)
- Review (165)
Language
- English (29537) (remove)
Keywords
- taxonomy (744)
- new species (444)
- morphology (174)
- Deutschland (142)
- Syntax (125)
- Englisch (120)
- distribution (117)
- biodiversity (101)
- Deutsch (98)
- inflammation (97)
Institute
- Medizin (5347)
- Physik (3819)
- Wirtschaftswissenschaften (1921)
- Frankfurt Institute for Advanced Studies (FIAS) (1762)
- Biowissenschaften (1550)
- Center for Financial Studies (CFS) (1494)
- Informatik (1401)
- Biochemie und Chemie (1090)
- Sustainable Architecture for Finance in Europe (SAFE) (1071)
- House of Finance (HoF) (710)
Abraham Lincoln
(1899)
Ligands of Iron-Sulphur Cluster N2: In this work the ubiquinone reducing catalytic core of NADH:ubiquinone oxidoreductase (complex I) from Y. lipolytica was studied by a series of point mutations replacing conserved histidines or arginines in the 49-kDa subunit. Although the missing 4th ligand of cluster N2 could not be found in the 49-kDa subunit of complex I, it was clearly demonstrated that iron-sulphur cluster N2 resides directly on the interface between the PSST and 49-kDa subunits. The results presented in this work show that residues in the 49-kDa subunit have strong influence on this redox centre and also on catalytic activity. The strong influence of Arg-141 and His-226 residues in 49-kDa subunit on this cluster can be deducted from complete loss of N2 signals in EPR spectra such as in case of mutants H226A and R141A. In the case of mutant H226M the EPR signal from cluster N2 was shifted and cluster N2 even lost the pH dependence of its redox midpoint potential and became more similar to the other so called 'isopotential' clusters. Specifically in the case of mutants R141M and R141K the characteristic signature of cluster N2 became undetectable in EPR spectra. However, specific dNADH:DBQ oxidoreductase activity that could be inhibited with the specific complex I inhibitors DQA and rotenone was not absolutely abolished but rather reduced. These reductions in complex I activity did not correspond to similar reductions in the specific EPR signal of cluster N2 as it was observed in the His-226 mutant series. No indications could be found that these mutations had modified the magnetic properties of cluster N2, resulting in different EPR spectra. From these observations it could be concluded that both mutants R141K and R141M virtually or entirely lack iron-sulphur cluster N2. The rates in complex I activity could be reconciled with electron transfer theory: After removal of a single redox centre in a chain, electron transfer rates are predicted to be still much faster than steady-state turnover of complex I. These results from mutants R141K, R141M and also the result from mutant H226M that protons are being pumped even if the redox midpoint potential of cluster N2 is not pH dependent questions the prominent role in the catalytic mechanism of complex I that has been ascribed to cluster N2. Histidine 91 and 95 were found to be absolutely essential for activity of complex I since in both mutants complex I was fully assembled and artificial NADH:HAR activity was parental whereas complex I specific dNADH:DBQ activity was abolished. The signal from cluster N2 in EPR spectra was parental for all His-91 and -95 mutants. Mutations at the C-terminal arginine 466 affected ubiquinone affinity and inhibitor sensitivity but also destabilised complex I. All these results provide further support for a high degree of structural conservation between the 49-kDa subunit of complex I and the large subunit of water soluble [NiFe] hydrogenases. Remodelling of Human Pathogenic 49-kDa Mutations in Y. lipolytica: Y. lipolytica has been proven a good system for studying complex I properties and thus also for studying defects that occur in humans. In this work pathogenic mutations in the 49-kDa subunit of complex I were recreated and studied. The P232Q mutant showed non-assembly of complex I and this is probably the cause why this mutation was lethal in patients. The mutants R231Q and S416P were parental for the content, artificial and also specific complex I activity, Km for DBQ and IC50 for DQA. From these results we can conclude that these two residues Arg-228 and Ser-413 in mammalian cells have specific structural importance for the 49-kDa subunit even if they are not directly involved in catalytic process.
Removal of apoptotic cells by macrophages or resident semi-professional phagocytes is a prominent principle with important implications for the pathophysiology of chronic inflammatory diseases, viral infections, or cancer. To characterize mechanisms which may determine the fate of apoptotic cells, I investigated chemokine expression in apoptotic promonocytic U-937 cells or PBMC. Exposure of U-937 cells to the anti-cancer drug etoposide (VP-16), an inducer of apoptosis in these cells, was associated with increased expression of the chemokines IL-8 and macrophage inflammatory protein 1alpha (MIP-1alpha). Upregulation of IL-8 mRNA expression by VP-16 was observed as early as 4 h after onset of treatment and was still detectable after 19h of exposure. A serine protease inhibitor prevented both VP-16-induced apoptosis and release of IL-8, whereas inhibition of p38 MAP-kinases reduced IL-8 secretion only. Moreover, I observed that incubation with 2-chlorodeoxyadenosine (CdA) upregulated release of IL-8 from adherent PBMC in parallel to induction of apoptosis. In these cells a modest but significant induction of TNF-alpha release by CdA was also detected. In addition, CdA augmented release of IL-8 from whole blood cultures. By facilitating adequate recruitment of phagocytes to sites of cell death, stress-induced upregulation of chemokines associated with apoptosis may contribute to mechanisms aiming at efficient removal of apoptotic cells.
This dissertation study argues that 'policy advice formation', as a discourse development, is a differentiated hybrid resultant from merger between comparative education and policy studies disciplines. Through discourse analysis based on John Creswell's format, this study identifies revisions, restatements and shifts in emphasis of theories, methodological models and challenge topics of comparative education and policy studies. Findings which display the development of policy advice formation' discourse. In conclusion, this study found differential patterns seemingly formed because of collaborative affects of standardization in education science knowledge expressed within discourse.
Remodeling of extracellular matrix (ECM) is an important physiologic feature of normal growth and development. In addition to this critical function in physiology many diseases have been associated with an imbalance of ECM synthesis and degradation. In the kidney, dysregulation of ECM turnover can lead to interstitial fibrosis, and glomerulosclerosis. The major physiologic regulators of ECM degradation in the glomerulus are the large family of zinc-dependent proteases, collectively refered to matrix metalloproteinases (MMPs). The tight regulation of most of these proteases is accomplished by different mechanisms, including the regulation of MMP gene expression, the processing and conversion of the inactive zymogen by other proteases such as serine proteases and finally the inhibition of active MMPs by endogenous inhibitors of MMPs, denoted as tissue inhibitors of metalloproteinases (TIMPs). Namely, the MMP-9 has been shown to be critically involved in the dysregulation of ECM turnover associated with severe pathologic conditions such as rheumatoid arthritis or fibrosis of lung, skin and kidney. In the present work I searched for a possible modulation of MMP-9 expression and/or activity in glomerular mesangial cells which are thought as key players of many inflammatory and non-inflammatory glomerular diseases. I found that various structurally different PPARalpha agonists such as WY-14,643, LY-171883 and fibrates potently suppress the cytokine-induced MMP-9 expression in renal MC. Furthermore, I demonstrate that the inhibition of MMP-9 expression by PPARalpha agonists was paralleled by a strong increase of cytokine-induced iNOS expression and subsequent NO formation, suggesting that PPARalpha-dependent effects on MMP-9 expression level primarily result from alterations in NO production which in turn reduces the MMP-9 mRNA half-life. Searching for the detailed mechanism of NO-dependent effects on MMP-9 mRNA stability, I found that NO either given from exogenous sources or endogenously produced increases the MMP-9 mRNA degradation by decreasing the expression of the mRNA stabilizing factor HuR. Furthermore, I demonstrate a reduction in the RNA-binding capacity of HuR containing complexes to MMP-9 ARE motifs in cells treated with NO. Since the reduction of HuR expression can be mimicked by the cGMP analog 8-Bromo-cGMP, I suggest that NO reduces in a cGMP-dependent manner the expression of HuR. Finally, I elucidated the modulatory effect of extracellular nucleotides, mainly ATP, on cytokine-triggered MMP-9 expression. Interestingly, I found that in contrast to NO, gamma-S-ATP the stable analog of ATP potently amplifies the IL-beta mediated MMP-9 expression. The increase in mRNA stability was paralleled by an increase in the nuclear-cytosolic shuttling of the mRNA stabilizing factor HuR. Furthermore, I demonstrate an increase in the RNA-binding capacity of HuR containing complexes to the 3'-UTR of MMP-9 by ATP. In summary, the data presented here may help to find new targets (posttranscriptional regulation) that could be used to manipulate or modulate the expression of not only MMP-9 but also other genes regulated on the level of mRNA stability.
In this thesis the anti-proton to proton ratio in 197Au + 197Au collisions, measured at mid-rapidity, at a center of mass energy of psNN = 200GeV is reported. The value was measured to be ¹p/p = 0.81+-0.002stat +- 0.05syst: in the 5% most central collisions. The ratio shows no dependence on rapidity in the range jyj < 0:5. Furthermore, a dependence on transverse momentum within 0:4< p? < 1:0 GeV/c is not observed. At higher p?, a slight drop in the ratio is observed. In the present analysis, the highest momentum considered is p? = 4:5 GeV/c yielding ¹p=p = 0:645§0:005stat: §0:10syst:. However, the systematic error is higher in this momentum range. A slight centrality dependence was observed, where a decrease from ¹p=p = 0:83§0:002stat:§0:05syst: for most peripheral collisions (less than 80% central) to ¹p=p = 0:78§0:002stat:§0:05syst: for the 5% most central collisions was measured. An estimate of the feed-down contributions fromthe decay of heavier strange baryons results in ¹p=p = 0:77 § 0:05syst:. The measured ratio indicates a » 12:5 times higher value compared to the highest SPS energy of psNN = 17:3 and an \almost net-baryon free" region, at mid- rapidity. The asymmetry of protons and anti-protons may be explained by the contribution ofvalence quarks in a nucleus break-up picture. In such a scenario, the absolute value of the ratio and the fact that the ratio does not depend on rapidity (at mid-rapidity) is well reproduced. Fragmentation of quarks and anti- quarks into protons and anti-protons is assumed. An estimate of the ratio, when feed-down correction is taken into consideration, agrees well with the prediction of a statistical model analysis at a temperature of T = 177 § 7 MeV and a baryon chemical potential of ¹B = 29 § 8 MeV. The temperature achieved is only slightly higher when compared to the top SPS energy, while the baryochemical potential is factor »10 lower. As in the case of the SPS results, these parameters are close to the phase boundary of Figure 1.6. The measurement of the ratio at high transverse momentum was of special in- terest in this analysis, since at RHIC energies, the cross section for hadrons at high transverse momentum is increased with respect to SPS energies. The weak dependence of the ratio on the transverse momentum is well described by the non- perturbative quenched and baryon junction scenario (i.e. Soft+Quench model), where baryon creation is enhanced by baryon junctions. In comparison the ratio does not decrease within the considered momentum range as predicted by pQCD.
Der Produktion von Interleukin-8 (IL-8), Hämoxygenase-1 (HO-1), und dem vaskulären endothelialen Wachstumsfaktor (VEGF) wird zunehmend größere Bedeutung im Rahmen der Regulation der Immunantwort bei Entzündung, Infektion und Tumorwachstum zugemessen. Ziel dieser Arbeit war die Untersuchung der Regulation dieser Botenstoffe in vitro durch Verwendung der humanen Dickdarmkarzinomzellinie DLD-1. Die Substanz Pyrrolidinedithiocarbamate (PDTC) verstärkt nicht nur die durch Tumornekrosefaktor-a (TNF-a) vermittelte Ausschüttung von IL-8, sondern induziert auch als alleiniger Stimulus die IL-8-Sekretion. Mutationsanalysen des IL-8-Promotors und "Electrophoretic Mobility Shift" Untersuchungen (EMSA) zeigten, daß die Aktivierung des Transkriptionsfaktors AP-1 (Aktivator Protein-1) und die Bindungsaktivität von konstitutiv aktiviertem NF-KB in DLD-1 Zellen für die PDTC induzierte IL-8 Expression zwingend erforderlich waren. Weiterhin war PDTC in der Lage in DLD-1 Zellen neben IL-8 auch die Expression von HO-1 und VEGF zu verstärken. Die Induktion von IL-8 durch PDTC war nicht nur auf DLD-1 Zellen beschränkt, sondern wurde auch in Caco-2 Zellen (ebenfalls Dickdarmkrebszellen) und in humanen mononukleären Blutzellen beobachtet. Die Verwendung von PDTC wird seit kurzem als Kombinationspräparat für Zytostatia zur Behandlung von verschiedenen bösartigen Tumoren, unter ihnen auch Darmkrebs, vorgeschlagen. Aus unseren Versuchen läßt sich ableiten, daß die Induktion von IL-8, HO-1 und VEGF die therapeutische Anwendung dieser Substanz nachteilig beeinflussen könnte. Dies ergibt sich daraus, daß alle drei genannten Faktoren durch proangiogene Wirkungen das Tumorwachstum fördern. Die Expression der induzierbaren Stickoxidsynthase und die Produktion von Stickoxid (NO) korreliert mit der Angiogenese bei verschiedenen Krebserkrankungen darunter Melanome, Tumore im Hals- und Kopfbereich und Darmkrebs. Da tumorbegünstigende Funktionen von NO mit vermehrter Angiogenese in Verbindung gebracht werden, wurden die Effekte von NO hinsichtlich der Produktion von ausgesuchten Chemokinen, die an der Steuerung des Tumorwachstums beteiligt sind, untersucht. Zu diesen Chemokinen gehören das proangiogene IL-8 sowie das tumorsuppressiv durch Interferon induzierbare Protein-10 (IP-10) und das Monokin induziert durch Interferon-y (MIG). Diese Chemokine werden, nach Stimulation mit IL- 1ß und lnterferon-? (IFN-?) von DLD-1 Zellen, ausgeschüttet. Unter diesen Bedingungen wird die IL-8 Freisetzung alleine durch IL-1ß vermittelt, aber nicht durch INFy. Im Gegensatz zu IL-8 hängt die Sekretion von IP-10 und MIG von der Aktivierung durch IFNy ab. Die Effekte von NO wurden analysiert indem DLD-1 Zellen mit dem NO-Donor DETA-NO inkubiert wurden. DETA-NO besitzt eine Halbwertzeit von 16,5h und simuliert damit die Effekte der endogenen NO-Synthase. Synthese und Freisetzung von IL-8 wurden durch die Behandlung mit NO stark gesteigert. Außerdem wurde in Zellen die dem NO-Donor ausgesetzt wurden die basale Sekretion des VEGF signifikant verstärkt. Dies steht im Gegensatz zur IL-Iß/IFNy-induzierten Produktion von IP-10 und MIG, beide wurden durch Koinkubation mit NO unterdrückt. Ebenso wurde die Regulation der IFNy abhängigen induzierbaren Stickoxidsynthase in DLD-1 Zellen von NO unterdrückt. Die vorliegenden Daten ergänzen vorherige Studien, in denen NO mit Tumorangiogenese und verstärkten Tumorwachstum in Verbindung gebracht wird. Die NO vermittelte Induktion von IL-8 und VEGF, ebenso wie die Verminderung der IP-10 and MIG Expression, könnte zu diesem Phänomen beitragen. Unsere Studien stützen die Hypothese, daß spezifische lnhibitoren der iNOS therapeutischen Nutzen bei humanen Neoplasien haben könnten.
Cytochrome c oxidase is the terminal enzyme in the respiratory chain of mitochondria and aerobic bacteria. This enzyme ultimately couples electron transfer from cytochrome c to an oxygen molecule with proton translocation across the inner mitochondrial and bacterial membrane. This reaction requires complicated chemical processes to occur at the catalytic site of the enzyme in coordination with proton translocation, the exact mechanism of which is not known at present. The mechanisms underlying oxygen activation, electron transfer and coupling of electron transfer to proton translocation are the main questions in the field of bioenergetics. The major goal of this work was to investigate the coupling of electron transfer and proton translocation in cytochrome c oxidase from Paracoccus denitrificans. Different theoretical approaches have been used to investigate the coupling of electron and proton transfer. This thesis presents an internal water prediction scheme in the enzyme and a molecular dynamics study of cytochrome c oxidase from Paracoccus denitrificans in the fully oxidized state, embedded in a fully hydrated dimyristoylphosphatidylcholine lipid bilayer membrane. Two parallel molecular dynamics simulations with different levels of protein hydration, 1.125 ns each in length, were carried out under conditions of constant temperature and pressure using three-dimensional periodic boundary conditions and full electrostatics to investigate the distribution and dynamics of water molecules and their corresponding hydrogen-bonded networks inside cytochrome c oxidase. The average number of solvent sites in the proton conducting K- and D- pathways was determined. The highly fluctuating hydrogen-bonded networks, combined with the significant diffusion of individual water molecules provide a basis for the transfer of protons in cytochrome c oxidase, therefore leading to a better understanding of the mechanism of proton pumping. The importance of the hydrogen bonding network and the possible coupling of local structural changes to larger scale changes in the cytochrome c oxidase during the catalytic cycle have been shown.
Obwohl Böden unzweifelhaft ein signifikanter Pool von organischem Kohlenstoff sind, ist ihre Bedeutung als potenzielle langfristige Senke für atmosphärischen Kohlenstoff keineswegs klar. Trotz bedeutender wissenschaftlicher Forschritte aus den letzten Jahren zur Klärung der Kohlenstoffdynamik in Böden gibt es nach wie vor offene Fragen insbesondere hinsichtlich der spezifischen geochemischen Mechanismen, die für die Stabilisierung organischen Kohlenstoffs in Böden verantwortlich sind. Vor diesem Hintergrund besteht ein wesentliches Ziel der vorliegenden Dissertation darin, in unterschiedlichen Bodentypen die Konzentration von organischem Kohlenstoff und Stickstoff sowie die mineralogische Zusammensetzung zu untersuchen, um Hinweise auf einen möglichen Einfluss der Tonmineralogie, der spezifischen Oberfläche und der Oxidkonzentration auf die Stabilisierung organischen Materials zu ermitteln. Die Ergebnisse sollen einen Beitrag dazu liefern, die Mechanismen der Fixierung organischer Substanz in Böden besser zu verstehen und das vorhandene Wissen hierüber zu erweitern. Hierzu wurden fünf verschiedene Bodenprofile aus Hessen mit unterschiedlicher mineralogischer Zusammensetzung untersucht. Um die Auswirkungen verschiedener physikalischer und geochemischer Faktoren auf den Gehalt organischer Substanz in den untersuchten Böden festzustellen, wurden folgende Parameter untersucht: -Tonmineralogie, -organische Kohlenstoff- und Stickstoff-Konzentrationen, -%-Kationensättigung, -spezifische Oberfläche, -dithionit- und oxalatlösliche Gehalte an Fe, Al und Mn. Anhand dieser Parameter wurden weiterführende statistische Analysen unter Verwendung der Statistiksoftware SPSS für Windows durchgeführt, um mögliche statistische Zusammenhänge aufzudecken, die für die Stabilisierung von organischem Kohlenstoff in den betrachteten Böden verantwortlich sind. Die im Rahmen der vorliegenden Dissertation ermittelten Ergebnisse zeigen, dass der Tonanteil und die Tonmineralogie der untersuchten Böden nur einen begrenzten Einfluss auf die Stabilisierung organischer Substanz haben. Weiterhin wird gezeigt, dass die in der Literatur propagierte Beziehung zwischen spezifischer Oberfläche und der Konzentration organischen Kohlenstoffs nicht auf alle Böden anwendbar ist. Die Ergebnisse deuten darauf hin, dass die Präsenz von amorphen Eisen- und Aluminiumoxiden der wichtigste Einflussfaktor für die Fixierung von organischem Material in den untersuchten Böden ist. Die größeren Konzentrationen von organischem Kohlenstoff in den kleinsten Fraktionen (Feinschluff und Ton) der Profile sind vor allem darauf zurückzuführen, dass Oxide ebenfalls in diesen Fraktionen aufzufinden sind. Tonminerale haben demnach eine sekundäre Bedeutung, indem sie Komplexe mit den Oxiden bilden, die zur Stabilisierung von organischer Substanz führen können. Insgesamt deuten die Ergebnisse daraufhin, dass Böden keine geeignete Senke für die langfristige Speicherung von organischem Kohlenstoff sind. Obwohl Mechanismen wie die Adsorption von organischer Substanz an Oxide die Stabilisierung organischen Materials unterstützen, scheinen diese nicht stark genug zu sein, um eine permanente Speicherung von organischem Kohlenstoff zu bewirken.
A gene trap strategy was used to identify genes induced in hematopoietic cells undergoing apoptosis by growth factor withdrawal. IL-3 dependent survival of hematopoietic cells relies on a delicate balance between proliferation and apoptosis that is controlled by the availability of cytokines (Thompson, 1995; Iijima et al., 2002). From our previous results of gene trap assay, we postulated that transcriptionally activated antagonistic genes against apoptosis might actually block or delay cell death (Wempe et al., 2001) causing cells to have carcinogenic behavior. The analysis attempted to better understand the outcome of a death program following IL-3 deprivation and to identify those survival genes whose expression is affected by time dependent manner. As described in the chapter 4, there would be two major conclusions evident from the three separate experiments (Genetrap, Atlas cDNA array and Affymetrix chips): Firstly 56% of trapped genes, that are up-regulated by IL-3 withdrawal (28 of 50), are directly related to cell death or survival. Secondly, unlike most array technologies, gene trapping only selects for the transiently induced genes that is independent of pre-existing steady state mRNA levels. In regarding correlations of the genes with potential carcinogenesis, the pre-existing mRNA makes difficult to describe the unique characteristics of deregulated tumor tissue genes. For a joint project with Schering (Schering AG, Berlin), the genes of our GTSTs were examined. The first screen with custom array was used to look for whether the survival genes of our GTSTs are involved in various cancer cell lines, whilst the second screen with Matched Tumor/Normal Array was used to characterize if the selected seven genes (ERK3, Plekha2, KIAA1140, PI4P5Ka/g, KIAA0740, KIAA1036 and PEST domains) are transformation-related genes or not in different tumor tissues. Twenty-six genes were identified as either induced or repressed in one or more cell lines. Genetic information is expressed in complex and ever changing patterns throughout a life span of cells. A description of these patterns and how they relate to the tissue specific cancer is crucial for our understanding of the network of genetic interactions that underlie the processes of normal development, disease and evolution. The development of cancer and its progression is clearly a multiplex phenotype, as a function of time, involving dozens of primary genes and hundreds of secondary modifier genes. There would be a major conclusion evident from the three separate experiments (Genetrap, Affymetrix mouse chip and Matched Tumor/Normal Array): ERK3 could play a significant role in breast, stomach and uterus carcinogenesis with tissue specific regulations. It is clear that ERK3 is obvious putative survival gene in these tumor tissues. Especially, in breast tumors, seven times up-regulation was considerable and the activation of ERK3 could be a feature of breast tumors. My results imply that the unique deregulation of ERK3 is perhaps the major consequence of possible transformation of normal cells into malignant cancer cells, even though further analysis remains to be determined whether an alterated activity of associated survival genes is primarily responsible for a carcinogenesis. However unlike all the other known MAP Kinases, no stimuli and no nuclear substrates of ERK3 is reported. Therefore, it will be necessary first to determine the spectrum of substrates and to identify the proximal effectors for the ERK3 in breast carcinoma cells.
Zahnwale sind die einzige Säugetiergruppe, die umfassend an ein Leben im Wasser angepasst ist und dabei ein aktives Sonarsystem zur Orientierung nutzt. Wahrscheinlich produzieren alle Zahnwalarten sonische oder ultrasonische Klicklaute, deren Echos die Tiere zu einem drei-dimensionalen "akustischen Bild" zusammensetzen. Im Gegensatz zu den meisten anderen Säugetieren produzieren Zahnwale diese Laute im Nasen-Komplex durch einen pneumatisch betriebenen Mechanismus. Jedoch spielt auch der Kehlkopf dabei eine wichtige Rolle, indem er den nötigen Luftdruck in der Nase erzeugt. Die Ergebnisse werden in Bezug auf die physikalischen Voraussetzungen eines Bio-Sonars in einer aquatischen Umwelt interpretiert. Um die morphologischen Eigenschaften (Struktur, Form, Topographie) der Organe im Kopf verschiedener Zahnwalarten vollständig zu erfassen, wurden diese mittels Computertomographie und Magnetresonanztomographie gescannt. Daraufhin wurden die Köpfe makroskopisch präpariert und histologische Schnitte von Gewebeproben angefertigt. Schließlich wurden die Ergebnisse durch digitale dreidimensionale Rekonstruktionen vervollständigt. Diese Studie basiert zum größten Teil auf der Untersuchung von Schweinswalen (Phocoena phocoena) und Pottwalen (Physeter macrocephalus). Zum Vergleich wurden fetale und postnatale Individuen anderer Zahnwalarten herangezogen wie Delphinartige (Delphinus delphis, Stenella attenuata, Tursiops truncatus), Flussdelphinartige (Pontoporia blainvillei, Inia geoffrensis) und der Zwergpottwal (Kogia breviceps). Im Allgemeinen konnte durch die morphologischen Daten dieser Studie die einheitliche "phonic lips-Hypothese der Schallproduktion bei Zahnwalen, wie sie von Cranford, Amundin und Norris [J. Morphol. 228 (1996): 223-285] aufgestellt wurde, bestätigt werden. Diese Hypothese beschreibt eine ventilartige Struktur in der Nasenpassage, den sogenannten "monkey lips/dorsal bursae complex" (MLDB) als Schallgenerator. Der pneumatische Mechanismus lässt die beiden Hälften des MLDB aufeinanderschlagen und erzeugt damit die initiale Schallschwingung im Gewebe ("phonic lips"). Diese Vibration wird über die Melone, einen großen Fettkörper in der vorderen Nasenregion der Zahnwale, fokussiert und in das umgebende Wasser übertragen. Die akzessorischen Nasensäcke und spezielle Schädel- und Bindegewebestrukturen können zu der Fokussierung beitragen. Obwohl die Echolotsignale der Schweinswale sehr spezialisiert zu sein scheinen, weisen die Übereinstimmungen in der Topographie und in der Form der Nasenstrukturen im Vergleich zu Delphinen und Flussdelphinartigen (Pontoporia und Inia) auf eine ganz ähnliche Funktion der Nase bezüglich der Produktion und Emission von Echolotschall hin. Allerdings gibt es einige anatomische Besonderheiten im Nasenkomplex des Schweinswals, welche die besondere Pulsstruktur der Sonarsignale erklären könnte. Diese werden in der Dissertation diskutiert. Bei einem Vergleich der Nasenmorphologie der Pottwale einerseits und der nicht-pottwalartigen Zahnwale andererseits fällt vor allem der Grad der Asymmetrie ins Auge. Im Gegensatz zu dem oben für Delphine und Schweinswale beschrieben Mechanismus betreiben Pottwale die Schallproduktion an den "monkey lips" mit Luft, die im rechten Nasengang unter Druck gesetzt wird (und nicht im nasopharyngealen Raum). Zudem könnte durch Änderung des Luftvolumens im rechten Nasengang die Schalltransmission zwischen den Fettkörpern, und somit die Schallemission, kontrolliert werden. In diesem theoretischen Szenario fungiert der breite rechte Nasengang als eine Art "akustische Schranke", welche zwischen zwei verschiedenen Modi der Klickproduktion wechselt: Der erste Modus mit luftgefülltem Nasengang führt zur Produktion der Kommunikationsklicks ("coda clicks") und der zweite Modus zur Aussendung von Echolotklicks, wenn der Nasengang kollabiert ist. Somit scheinen die zentrale Position und die nahezu horizontale Orientierung des rechten Nasengangs im Kopf der Pottwale als Schnittstelle (Schranke) zwischen den beiden großen Fettkörpern mit dem Mechanismus der Schallproduktion bei veränderten Luftvolumina korreliert zu sein. Die hier beschriebenen und andere Ergebnisse dieser Dissertation deuten darauf hin, dass die Gestalt und das Ausmaß der Nasenasymmetrie nicht mit der systematischen Zugehörigkeit der jeweiligen Art korrelieren, sondern durch den jeweiligen Typus des Sonarsystems als Ausdruck einer bestimmten ökologischen Anpassung bedingt sind. Bei Zahnwalen ist der Kehlkopf charakterisiert durch eine rostrale Verlängerung des Kehldeckels und der beiden Stellknorpel, die ein gänseschnabelartiges Rohr bilden, das von einem starken Sphinktermuskel umrundet und dabei in Position gehalten wird. Auf diese Weise ist das Atemrohr vollständig vom Digestionstrakt getrennt. Aus anatomischer Sicht ist es wahrscheinlich, dass die Schallerzeugung bei Zahnwalen durch eine Kolbenbewegung des Kehlkopfes in Richtung der Choanen zustande kommt, wodurch der Luftdruck im Nasenbereich erzeugt wird. Die Kontraktion des Sphinktermuskels als einem muskulösen Schlauch erzeugt wahrscheinlich die größte Kraft für diese Kolbenbewegung. Jedoch dürften die Muskelgruppen, die den Kehlkopf und das Zungenbein am Unterkiefer und an der Schädelbasis aufhängen, signifikant zur Druckerhöhung beitragen.
The endothelin B receptor belongs to the rhodopsin-like G-protein coupled receptors family. It plays an important role in vasodilatation and is found in the membranes of the endothelial cells enveloping blood vessels. During the course of this work, the production of recombinant human ETB receptor in yeast, insect and mammalian cells was evaluated. A number of different receptor constructs for production in the yeast P. pastoris was prepared. Various affinity tags were appended to the receptor N-and C-termini to enable receptor detection and purification. The clone pPIC9KFlagHisETBBio, with an expression level of 60 pmol/mg, yielded the highest amount of active receptor (1.2 mg of receptor per liter of shaking culture). The expression level of the same clone in fermentor culture was 17 pmol/mg, and from a 10L fermentor it was possible to obtain 3 kg of cells that contained 20-39 mg of the receptor. For receptor production in insect cells, Sf9 (S. frugiperda) suspension cells were infected with the recombinant baculovirus pVlMelFlagHisETBBio. The peak of receptor production was reached at 66 h post infection, and radioligand binding assays on insect cell membranes showed 30 pmoL of active receptor /mg of membrane protein. Subsequently, the efficiency of different detergents in solubilizing the active receptor was evaluated. N-dodecyl-beta-D-maltoside (LM), lauryl-sucrose and digitonine/cholate performed best, and LM was chosen for further work. The ETB receptor was produced in mammalian cells using the Semliki Forest Virus expression system. Radioligand binding assays on membranes from CHO cells infected with the recombinant virus pSFV3CAPETBHis showed 7 pmol of active receptor /mg of membrane protein. Since the receptor yield from mammalian cells was much lower than in yeast and insect cells, this system was not used for further large-scale receptor production. After production in yeast and insect cells, the ETB receptor was saturated with its ligand, endothelin-1, in order to stabilize its native form. The receptor was subsequently solubilized with n-dodecyl-beta-D-maltoside and subjected to purification on various affinity matrices. Two-step affinity purification via Ni2+-NTA and monomeric avidin proved the most efficient way to purify milligram amounts of the receptor. The purity of the receptor preparation after this procedure was over 95%, as judged from silver stained gels. However, the tendency of the ETB receptor produced in yeast to form aggregates was a constant problem. Attempts were made to stabilize the active, monomeric form of the receptor by testing a variety of different buffer conditions, but further efforts in this direction will be necessary in order to solve the aggregation problem. In contrast to preparations from yeast, the purification of the ETB receptor produced in insect cells yielded homogeneous receptor preparations, as shown by gel filtration analysis. This work has demonstrated that the amounts of receptor expressed in yeast and insect cells and the final yield of receptor, isolated by purification, represent a good basis for beginning 3D and continuing 2D crystallization trials.
Hepatitis E virus (HEV) is a positive-stranded RNA virus with a 7.2 kb genome that is capped and polyadenylated. The virus is currently unclassified : the organisation of the genome resembles that of the Caliciviridae but sequence analyses suggest that it is more closely related to the Togaviridae. HEV is an enterically transmitted virus that causes both epidemics and sporadic cases of acute hepatitis in many countries of Asia and Africa but only rarely causes disease in more industrialised countries. Initially the virus was believed to have a limited geographical distribution. However, serological studies suggest that that HEV may be endemic also in the United states and Europe even though it infrequently causes overt disease in these countries. Many different animal species worldwide recently have been shown to have antibodies to HEV suggesting that hepatitis E may be zoonotic. Although two related strains have been experimentally transmitted between species, direct transmission from animal to a human has not been documented. Our main objective in this study is to evaluate the suitability of current available HEV antibody assays for use in low-endemicity areas such as in Germany. Methods: We selected sera on the basis of at least borderline reactivity in the routinely used Abbot EIA. Most were tested as part of routine screening of long-term expatriates in endemic countries. The following assays (recombinant antigens : ORF2 and ORF3) were used: Abbot EIA, Genelabs ELISA, Mikrogen recomBlot and a 'Prototype' DSL-ELISA. We observed a wide range of sensitivity ( average of 56.8%) and specificity ( an average of 61.4%) in these used assays. These results implies that , these assays might be unreliable for detection of HEV infection in areas where hepatitis E is not endemic. However, most anti- HEV assays have not been correlated with the HEV RNA determined by reverse transcription. Many of these unexpected results and discrepancies can be alluded to the following reasons: I. The choice and the size of the HEV antigen. II. Duration of the antibody persistence III. A cross reactivity with different agent IV. Due to geographic species V. A low sensitivity of the available assays. VI. And infection with non-pathogenic HEV strain. (zoonotic strain?). We therefore suggest that, further studies will be required to improve the sensitivity and specificity of the available commercial assays on the market.
In the present study the cryo-immunogold technique was used and optimized for investigating the ultrastructure and immunolabeling of synaptic proteins. It is evidently a suitable method for the localization of membrane proteins since the antigens are not treated with any chemical denaturation before immunolabeling except for the fixation and since the antigens are directly exposed to the surface of the cryo-ultrasections. The v-SNARE VAMP II and the vesicle-associated proteins SV2 and Rab3A were detected extensively at small vesicles in the mossy fiber terminals. The t-SNARE SNAP-25, and N-type and P/Q type Ca2+ channels were allocated to the plasma membrane both at the active zone and outside the active zone. SNAP-25 and N-type Ca2+ channels appeared also at synaptic vesicles. A significantly increased immunolabeling of VAMP II, SV2, Rab3A, SNAP-25 and N-type Ca2+ channels was found at the active zones of fast synapses, indicating a concentration of these proteins at sites of exocytosis. The widespread distribution of the t-SNARE SNAP-25 at the axonal plasma membrane reveals that membrane-targeting specificity cannot be determined solely by v/t-SNARE interactions. Additional control components are required to assure the docking and exocytosis of the synaptic vesicles at active zones. The novel protein Bassoon was only found at active zones of central synapses and showed the highest specific labeling among all proteins investigated. Its labeling pattern implies an association of Bassoon with the presynaptic dense projections, the structural guide for vesicle exocytosis. The involvement of Bassoon in the organization of the neurotransmitter release site suggests that Bassoon may play an important role in determining the specificity of vesicle docking and fusion. In the neurosecretory endings of neurohypophysis the synaptic proteins VAMP II, SNAP- 25, SV2, Rab3A, and the N-type Ca2+ channels showed a preferential labeling over microvesicles. Moreover, the immunolabeling intensity of these proteins over microvesicles corresponded closely to that over synaptic vesicles. This suggests that these synaptic proteins share an identical association with synaptic vesicle and microvesicles. A significant labeling of SNAP-25, the N-type Ca2+ channels and VAMP II was also detected at the plasma membrane near the clustered microvesicles, indicating the competence of microvesicles for docking and exocytosis along the plasma membrane in the absence of active zones. No significant labeling of VAMP II, SNAP-25, SV2 and N-type Ca2+ channel was observed at the membrane of neurosecretory granules. This is in agreement with the notion that synaptic vesicles and microvesicles possess regulatory mechanisms for exocytosis different from those of granules. In contrast, a/ß-SNAP and NSF were found on the granules, and Rab3A and the P/Q-type Ca2+ channels on granules in a subset of terminals. Rab3A is associated specifically with the oxytocin-containing granule population. Interestingly, some plasma membrane proteins, such as SNAP-25 and even N-type Ca2+ channels and P/Q-type Ca2+ channels, were observed not only at the plasma membrane but also at the vesicular organelles. This suggests that these vesicular organelles may be involved in transporting newly synthesized proteins from the soma to the plasma membrane of the terminal. Furthermore, the vesicular pool of the Ca2+ channels may serve in the stimulationinduced translocation into the plasma membrane when required. Using the conventional preembedding method with Epon and the post-embedding method with LR Gold, VAMP II was localized at vesicular organelles of varying size and on horseradish peroxidase filled endocytic organelles in cultured astrocytes, with and without stimulation in the presence of the horseradish peroxidase. This indicates that VAMP II is involved in the cycle of vesicular exocytosis and endocytosis in astrocytes. U373 cells are capable of expressing all three members of the synaptic SNARE complex (v-SNARE VAMP II, t-SNARE syntaxin I and SNAP25). This indicates the competence of U373 to carry out regulated exocytosis by means of the classical SNARE mechanism. In addition, the ubiquitous v-SNARE cellubrevin and the endosome-associated small GTPbinding protein Rab5 could be expressed in U373 cells. All recombinant synaptic proteins investigated in U373 cells revealed a punctuate cellular distribution under the fluorescence microscope, suggesting that they are mainly associated with intracellular compartments. The cryo-electron microscopy provided direct evidence for the association of all expressed proteins with electron-lucent vesicular organelles. It further supports the potential of U373 MG cells to release low molecular weight messengers by a regulated exocytosis mechanism. In addition, myc-VAMP II was found on dispersed granules. Probably, VAMP II also participates in the exocytosis event of granules in U373 cells. Gold labeling for the two presumptive t-SNAREs syntaxin I and SNAP-25 in U373 cells was confined to the vesicular organelles. At the ultrastructural level no significant labeling was identified at the plasma membrane. The high level of colocalization of the two SNARE proteins VAMP II and syntaxin I in the cell body and in cell processes suggests that the two proteins are mostly sorted into identical vesicular organelles. A partial colocalization of VAMP II and cellubrevin as well as of VAMP II and Rab5 was observed under the fluorescence microscope. At the ultrastructural level, a colocalization of VAMP II and cellubrevin as well as of VAMP II and Rab5 was found on some clustered vesicles. The partial colocalization of VAMP II and cellubrevin implies that they similarly function as v-SNAREs. The partial colocalization of Rab5 with VAMP II in U373 cells suggests that the endosomal protein Rab5 is associated with VAMP II-containing organelles during some stages of their life cycle.
The focus of this study were Celtic gold coins excavated from the Martberg, a Celtic oppidium and sanctuary, occupied in the first century B.C. by a Celtic tribe known as the Treveri. These coins and a number of associated coinages, were characterised in terms of their alloy compositions and their geochemical and isotopic signatures so as to answer archaeological and numismatic questions of coinage development and metal sources. This required the development of analytical methods involving; Electron Microprobe (EPMA), Laser Ablation-ICP-MS, solution Multicollector-ICPMS and LA-MC-ICP-MS. The alloy compositions (Au-Ag-Cu-Sn) were determined by EPMA on a small polished area on the edge of the coins. A large beam size, 50µm (diameter), was used to overcome the extreme heterogeneity of these alloys. These analyses were shown to be representative of the bulk composition of the coins. The metallurgical development of the coinages was defined and showed that the earlier coinages followed a debasement trend, which was superceded by a trend of increasing copper at the expense of sliver while gold compositions remained stable. This change occurred with the appearance of the inscribed "POTTINA" coinage, Scheers 30/V. Two typologically different coinages, Scheers 16 and 18 ("Armorican Types") were found to have markedly different compositions which do not fit into the trends described above. A Flan for a gold coin, which may indicate the presence of a mint at the Martberg, was found to have an identicle weight and composition as the Scheers 30/I coins, which preceeded the majority of the coins found at the Martberg in the coin development chronology. The trace element anaylses were made by Laser Ablation-ICPMS using an AridusTM desolvating nebuliser to introduce matrix matched solution standards to calibrate the measurements, which were then normalised to 100%. Quantitative results were obtained for the following elements: Sc, Ti, Cr, Mn, Co, Ni, Cu, Zn, Se, Ru, Rh, Pd, Ag, Sb, Te, W, Ir, Pt, Pb, Bi. The remaining elements remain problematic as they produced incorrect standardisations mainly due to chemical effects in solution such as adsorption onto the beaker walls or oxidation : V, Fe, Ga, Ge, As, Mo, Sn, Re, Os, Hg. Changes in the sources of Au, Ag and Cu were observed during the development of the coinages through the variation of trace elements, which correlate positively with the major components of the coin alloys. Changes in the Pt/Au ratios show that the Scheers 23 coins contain distinctly different gold from the later coinages and that the Scheers 18 gold source was also different. Te/Ag was used to show that the Sch.23 coins also contained different silver and some subgroups were observed in the Sch. 30/V coins. A major change in copper source is indicated by the sudden increase of Sb and Ni with the introduction of the Sch. 30/V coins (POTTINA), which can be linked to a similar change in copper observed in the contemporary silver coinage, Sch. 55 (with a ring). Lead isotopic analyses were made by solution- and Laser Ablation - MC-ICP-MS, The laser technique proved to be in good agreement with the solution analyses with precisions between 1 and 0.1%o (per mil). The development of the laser method opens the way for easy and virtually non-destructive Pb isotopic determinations of ancient gold coins. The results showed that Sch. 23 is very different from the following coinages, Sch. 16 and 18 are also different, forming their own group, and all the later "Eye" staters (Sch. 30/I-VI) lie on a mixing line controlled by the addition of copper from a Mediterranean source, probably Sardinia or Spain. An indication of gold and silver sources should be possible with further analyses of the Sch. 23 and Rainbow Cup gold coins and the Sch. 54 and 55 silver coinages. Copper Isotopic analyses were made by solution- and Laser Ablation - MC-ICP-MS. Both techniques require further development to produce more reproducible results. The results show that there appears to be a trend to more positive d Cu65 values for the later coinages and that the link between the copper used in the Sch. 30/V (POTTINA) coins and the silver Sch. 55 (with a ring) coins is also shown by similarly postive d Cu65 values. The full suite of analyses were also made on samples of gold from the region. They were mostly composed of "placer gold", alluvial gold found in rivers. It was found that when a study is restricted to a limited number of deposits or areas then it is possible to distinguish between deposits based on the concentration of those elements which are least affected by transport related alteration processes. These elements include; the PGE's, due to their refractory nature, and those elements which are usually present in high enough concentrations to remain relatively unaffected, eg: Cu, Pb and Sb. Due to the nature of the coin alloy it is not possible to link the gold used in the coins studied here with gold deposits, as the large amounts of Ag and Cu, added to the coin alloys, have masked the Au signature. However, further Pb isotopic analyses of gold deposits should prove useful in determining from which regions Celtic gold was derived.