Refine
Has Fulltext
- yes (2786) (remove)
Year of publication
Document Type
- Doctoral Thesis (2786) (remove)
Language
- English (2786) (remove)
Keywords
- Maus (61)
- Taufliege (61)
- Drosophila (39)
- Signaltransduktion (39)
- Topologischer Isolator (37)
- Thrombozyt (36)
- Genexpression (34)
- Tissue Engineering (31)
- Leistungsbewertung (29)
- T-Lymphozyt (28)
Institute
- Graduate School of Life Sciences (778)
- Theodor-Boveri-Institut für Biowissenschaften (482)
- Physikalisches Institut (208)
- Institut für Informatik (139)
- Institut für Theoretische Physik und Astrophysik (123)
- Institut für Organische Chemie (113)
- Institut für Mathematik (112)
- Institut für Psychologie (111)
- Institut für Pharmazie und Lebensmittelchemie (103)
- Julius-von-Sachs-Institut für Biowissenschaften (88)
Schriftenreihe
Sonstige beteiligte Institutionen
- Helmholtz Institute for RNA-based Infection Research (HIRI) (7)
- Fraunhofer-Institut für Silicatforschung ISC (5)
- Technische Hochschule Nürnberg Georg Simon Ohm (3)
- Deutsches Zentrum für Luft- und Raumfahrt (DLR), Institut für Raumfahrtsysteme (2)
- EMBL Heidelberg (2)
- Institut für Tierökologie und Tropenbiologie (2)
- Rudolf Virchow Center for Integrative and Translational Bioimaging, University of Würzburg (2)
- Universität Belgrad, Serbien (2)
- Universitätsklinikum Münster (2)
- Universitätsklinikum Würzburg (2)
ResearcherID
- B-1911-2015 (1)
- B-4606-2017 (1)
- C-2593-2016 (1)
- D-1250-2010 (1)
- I-5818-2014 (1)
- J-8841-2015 (1)
- M-1240-2017 (1)
- N-2030-2015 (1)
- N-3741-2015 (1)
EU-Project number / Contract (GA) number
- 311781 (1)
- 320377 (1)
- EU (FP7/ 2007-2013) (1)
The studies inventoried the species of the families Dytiscidae and Noteridae (Coleoptera) in Comoé National Park in northern Ivory Coast, West Africa and investigated the ecological role of temporary and permanent water bodies for the aestivation of these aquatic beetles. The ecological studies focused on the question how the beetles cope with the temporary loss of their aquatic habitats during dry season. The climate in the study area is characterised by a pronounced dry season from about November to March/April, in which the temporary ponds and creeks in the savannah entirely desiccate. The only available water bodies during dry season in Comoé National Park are the Comoé River, pools in some of its tributaries, and a few of the large savannah ponds. The taxonomic and faunistic analysis revealed a high species richness in the study area and yielded a total of twelve species of Noteridae in four genera and 95 species of Dytiscidae in 22 genera. Thirty of these species had not yet been reported from the Ivory Coast. A description of a new species in the genus Laccophilus is given, named L. comoensis in honour of the National Park. Strong incidences exist that the material includes more species yet unknown to science. Concerning the mode of aestivation, observations in pilot studies led to the working hypothesis that the beetles pass the dry season as adults in aquatic habitats. Consequently, presence of adults in aquatic habitats throughout the dry season and cyclic migration of adults between temporary and permanent water bodies was expected. Regular sampling of water bodies throughout the dry season and beginning rainy season yielded 33,705 individuals in 72 species and 26 genera. In all the sample periods Noteridae and / or Dytiscidae were recorded. The number of species per period was between 36 and 58. It is concluded that in Comoé National Park a) at least parts of the populations of the recorded species pass the dry season as adults and b) aquatic habitats serve as a refuge for aestivation of these adult beetles. In a rocky area in the riverbed of the permanent Comoé River four sets of studies were performed during dry and beginning rainy season. According to the working hypothesis beetles should be searching for adequate aquatic habitats as long as temporary savannah waters are becoming inhospitable and are falling dry. Seven rock pools in the riverbed of the Comoé River were artificially filled and thus offered for colonization at the peak of the dry season (end of January). After five days the rock pools were quantitatively sampled by completely emptying them. All the rock pools were colonized by Dytiscidae and / or Noteridae and with a total of 1,507 individuals in 26 species abundance and diversity were high. Habitats for aestivation are needed most, when the majority of the savannah waters are fallen dry. Little precipitation on February 18th 1999 had filled rock pools in the riverbed of the Comoé River but no pools in the savannah, where the rain was immediately absorbed by the very dry soil. An inventory of beetles was performed in 21 naturally filled rock pools five to 20 days after this precipitation. The sampling yielded 8,456 individuals in 41 species. Except the smallest, all rock pools contained beetles. The result showed that Dytiscidae and Noteridae utilise the rock pools as aquatic habitat during dry season. Beetles adapted to a highly seasonal environment like the aquatic system in the study area should be good colonizers. Sampling of four, respectively five rock pools at two occasions within 24 hours after the start of precipitation examined the potential of colonizers at that period (March). Prior to these precipitations the pools had been completely dry. Dytiscidae were already present in all rock pools and a total of 434 Dytiscidae in 14 species was found. The working hypothesis of cyclic migration suggests that the beetles should leave the rock pools at the onset of the rainy season when precipitation had filled temporary water bodies in the savannah. After several precipitation events an inventory of 13 rock pools of the Comoé River in May controlled for adult beetles. Only four species with 126 individuals were still found, of which Yolina chopardi contributed 81.7%. This species seems to differ from the other recorded species in the use of habitats, since it was never recorded in the savannah. In general, however, diversity and abundance of Dytiscidae and Noteridae in the rock pools, as expected, was low after the onset of the rainy season. During the entire study of the rock pools in the riverbed of the Comoé River 10,523 individuals in 44 species and 18 genera were collected. Thus, more than half of the species recorded in Comoé National Park were found in the rock pools. The results suggest that the Comoé River and the rock pools in the riverbed serve as aquatic retreat for adult Dytiscidae and Noteridae during dry season when temporary water bodies in the savannah are desiccated. The suggested cyclic migration between water bodies predicts that newly formed savannah waters are recolonized by the beetles at the onset of the rainy season. This colonization should be a) by adults and b) airborne. Two artificial ponds in the open savannah were offered only for aerial colonization at the beginning of the rainy season. The ponds were controlled for adult Noteridae and Dytiscidae daily during one continuous phase of eleven and a second one of 16 days (end of March to end of April). On every sampling date Noteridae or Dytiscidae were recorded. In the entire study 2,744 individuals in 44 species and 16 genera were collected. After precipitation, abundance and species richness increased. Thirty-five of the encountered species had been recorded in rock pools of the Comoé River before. The principal species in the artificial savannah ponds had been principal species in samplings of the rock pools as well. The results support the hypothesis of cyclic migration: most species of Dytiscidae and Noteridae of the Comoé National Park fly from desiccating savannah waters to permanent water bodies or water bodies holding water for extended times during dry season. They pass the dry season in these waters and fly back into the savannah after precipitation at the onset of the rainy season. Exceptions from this general rule are discussed.
In this work the supersymmetric seesaw model and its effects on low-energy leptonic observables and thermal leptogenesis have been systematically investigated. Precision measurements will increase the sensitivity on lepton-flavor violating decays, particularly on Br(l_j->l_i gamma) and also on electric and magnetic dipole moments in the near future. In order to improve also the accuracy of theoretical predictions for these processes, we have performed a full one-loop calculation of the underlying supersymmetric processes taking into account the lepton masses. Since the mechanism of soft supersymmetry breaking (SSB) is completely unknown, a novel analysis beyond the often studied minimal Supergravity scenarios has been performed. This way it has been demonstrated that in the considered mSUGRA, AMSB, GMSB and gaugino mediated scenarios, the ongoing search for Br(mu->e gamma) can constrain fundamental SSB parameters and/or the seesaw parameters. On the other hand, the basic parameters of thermal leptogenesis, such as the CP asymmetry in the decays of the lightest right-handed Majorana neutrino, provide probes of the unknown complex orthogonal R-matrix of the seesaw model.
The exploitation of landscapes increases fragmentation of valuable areas with high biodiversity. Consequently, many populations nowadays exist as metapopulations. In such cases, the balance between extinction and colonisation of patches determines the regional survival of species. To determine long term survival of species and to assess the impact of different management regimes proper knowledge of species habitat requirements as well as information on their dispersal behaviour is needed. The aim of this thesis was to develop methods and measures for the identification of suitable areas for grasshoppers and bush crickets, as well as to quantify the reachability of single patches by individuals. The first part of my work focuses on the quantification of habitat suitability for grasshoppers and bush crickets. Based on presence/absence data, I developed statistical habitat suitability models using logistic regression analyses. The resulting models are evaluated and validated in space and time. It turned out that habitat selection of the species mainly took place on an intermediate spatial scale. The relevant scale falls into the same range as the species’ mean dispersal distances. Besides the rather coarse grained factor ‘type of habitat’ structural factors as well as abiotic factors are correlated with the occurrence of the species. The model of S. lineatus, including the parameters ‘type of biotope’ and ‘vegetation height’ was most successful in predicting the occurrences of the bush cricket species. To further test whether the occurrence of species of different insect groups can be predicted with a common model, I tested the usefulness of the orthoptera models for the prediction of butterflies in the same region and vice versa. While transferability of the orthoptera models was poor, the model of the moth Z. carniolica performed quite successful. It included the proportion of suitable habitat as well as the occurrence of the two sucking plants C. jacea and S. columbaria as relevant factors. Z. carniolica is classified as stenoecious and thus represents other species typically found on fringes and mesoxerophytic grasslands. The high mobility of Z. carniolica simultaneously guarantees the reachability of regional suitable areas and thus ensures that the influence of the random effects of colonisation on the model are marginal. Unfortunately, the factors predicting habitat quality for a species are normally not available at the landscape level. Thus, they cannot be used for the prediction of occurrences without extensive censuses in the field. Nevertheless, my results show that the sole use of the variable ‘type of habitat’, which often is available landscape wide, will be sufficient for the classification of habitat suitability in a landscape. I conclude that for practical use in conservation biology the type of biotope can be used to predict occurrence of the studied species. Besides quality/quantity of suitable habitat, dispersal of individuals between patches is a key factor influencing the survival of populations. Thus, the second part of my work concentrates on theoretical as well as empirical studies on the dispersal behaviour of bush crickets. In field experiments I could show that the assumption of a dichotomous movement behaviour does not apply for bush crickets. Instead, movement pattern changes continuously with structural resistance, temperature, mortality risk and resource availability. This result is confirmed in my experiments on the behaviour of bush crickets at habitat borders. For different borders I could demonstrate different edge permeabilities. Additionally, I observed that grasshoppers could detect suitable habitat from a certain distance. Because the dispersal behaviour plays an important role in theoretical models, my empirical data can be used to parameterise such models. In addition to the influence of movement pattern on the reachability of suitable habitats, I could demonstrate, with simulation models, that the influence of the landscape context in which dispersal takes place has a critical impact on the exchange of individuals between patches. This effect is enhanced if mortality risk during dispersal is accounted for. The results from my studies on habitat suitability can be used to identify suitable habitat for grasshoppers and bush crickets in a landscape. Consequently, the potential suitability of an area as habitat, based on predictions on changes in the type of biotope by management regime, can be predicted. But this information alone is not sufficient to determine regional survival probability of a species. My investigations concerning the dispersal behaviour clearly show, that the reachability of suitable areas is dependent on the spatial configuration of patches and the structure of areas between habitats. Additionally, factors specific for individuals, like motivation and physiological factors play a crucial role for the reachability of suitable habitats.
In a variety of established tumour cell lines, but also in primary mammary epithelial cells metalloprotease-dependent transactivation of the EGFR, and EGFR characteristic downstream signalling events were observed in response to stimulation with physiological concentrations of GPCR agonists such as the mitogens LPA and S1P as well as therapeutically relevant concentrations of cannabinoids. Moreover, this study reveals ADAM17 and HB-EGF as the main effectors of this mechanism in most of the cancer cell lines investigated. However, depending on the cellular context and GPCR agonist, various different members of the ADAM family are selectively recruited for specific ectodomain shedding of proAR and/or proHB-EGF and subsequent EGFR activation. Furthermore, biological responses induced by LPA or S1P such as migration in breast cancer and HNSCC cells, depend on ADAM17 and proHB-EGF/proAR function, respectively, suggesting that highly abundant GPCR ligands may play a role in tumour development and progression. Moreover, EGFR signal transactivation could be identified as the mechanistic link between cannabinoid receptors and the activation of mitogen activated protein kinases (MAPK) ERK1/2 as well as pro-survival Akt/PKB signalling. Depending on the cellular context, cannabinoid-induced signal cross-communication was mediated by shedding of proAmphiregulin and/or proHB-EGF by ADAM17. Most importantly, our data show that concentrations of THC comparable to those detected in the serum of patients after THC administration accelerate proliferation of cancer cells instead of apoptosis and thereby may contribute to cancer progression in patients.
In this thesis a new and powerful approach for modeling laser cavity eigenmodes is presented. This approach is based on an eigenvalue problem for singularly perturbed partial differential operators with complex coefficients; such operators have not been investigated in detail until now. The eigenvalue problem is discretized by finite elements, and convergence of the approximate solution is proved by using an abstract convergence theory also developed in this dissertation. This theory for the convergence of an approximate solution of a (quadratic) eigenvalue problem, which particularly can be applied to a finite element discretization, is interesting on its own, since the ideas can conceivably be used to handle equations with a more complex nonlinearity. The discretized eigenvalue problem essentially is solved by preconditioned GMRES, where the preconditioner is constructed according to the underlying physics of the problem. The power and correctness of the new approach for computing laser cavity eigenmodes is clearly demonstrated by successfully simulating a variety of different cavity configurations. The thesis is organized as follows: Chapter 1 contains a short overview on solving the so-called Helmholtz equation with the help of finite elements. The main part of Chapter 2 is dedicated to the analysis of a one-dimensional model problem containing the main idea of a new model for laser cavity eigenmodes which is derived in detail in Chapter 3. Chapter 4 comprises a convergence theory for the approximate solution of quadratic eigenvalue problems. In Chapter 5, a stabilized finite element discretization of the new model is described and its convergence is proved by applying the theory of Chapter 4. Chapter 6 contains computational aspects of solving the resulting system of equations and, finally, Chapter 7 presents numerical results for various configurations, demonstrating the practical relevance of our new approach.
Subject of this work was to investigate the influence of nonadiabatic coupling on the dynamical changes of electron and nuclear density. The properties of electron density have neither been discussed in the stationary case, nor for excited electronic states or for a coupled electronic and nuclear motion. In order to remove these restrictions one must describe the quantum mechanical motion of all particles in a system at the same level. This is only possible for very small systems. A model system developed by Shin and Metiu [1, 2] contains all necessary physical ingredients to describe a combined electronic and nuclear motion. It consists of a single nuclear and electronic degree of freedom and the particle interaction is parameterized in such a way as to allow for a facile switching between and adiabatic (Born-Oppenheimer type) and a strongly coupled dynamics. The first part of the work determined the “static” properties of the model system: The calculation of electronic eigenfunctions, adiabatic potential curves, kinetic coupling elements and transition dipole moments allowed for a prediction of the coupled dynamics. The potentials obtained from different parameterization showed two distinct cases: In the first case the ground and first excited state are separated by a large energy gap which is the typical Born-Oppenheimer case; the second one exhibits an avoided crossing which results in a breakdown of the adiabatic approximation. Due to the electronic properties of the system, the quantum dynamics in the two distinct situations is very different. This was illustrated by calculating nuclear and electron densities as a function of time. In the Born-Oppenheimer case, the electron density followed the vibrational motion of the nucleus. This was demonstrated in two examples. In the strongly coupled case the wave packet did not exhibit features caused by nonadiabatic coupling. However, projections of the wave function onto the electronic states revealed the usual picture obtained from solutions of the nuclear Schrödinger equation involving coupled electronic states. In that case the nuclear motion triggered charge transfer via nonadiabatic coupling. The second part of the work demonstrated that the model system can easily be modified to yield binding situations often found in diatomic molecules. The different situations can be characterized in terms of bound and dissociative adiabatic potential curves. The investigation focussed on the case of an electronic predissociation, where the ground state is dissociative in the asymptotic limit of large internuclear distances. Within our model system we were able to demonstrate how the character of the electron density changes during the fragmentation process. In the third part we investigated the influence of external fields on the correlated dynamics of electron and nucleus. Employing adiabatic potential curves, the structure of absorption spectra can be understood within the weak-field limit. In the above described Born-Oppenheimer case the adiabatically calculated spectrum was in very good agreement with the exact one, whereas in the strongly coupled case the obtained spectrum was not able to resemble the exact one. Regarding the dynamics during a laser excitation process the time-dependent electron and nuclear densities nicely illustrated the famous Franck-Condon principle. The interaction with strong laser pulses lead to an excitation of many bound electronic and vibrational states. The electron density reflected the classical-like quiver motion of the electron induced by the fast variations of the electric field. The nucleus did not follow these fast oscillations because of its much larger mass. The last part of the work extended the original model system by including an additional electron. As a consequence of the Pauli principle, the spatial electronic wave function has to be either symmetric or anti-symmetric with respect to exchange of the two electrons. This corresponds to anti-parallel or parallel electron spins, respectively. The extended model already contains the physical properties of a many-electron system. Solving the time-dependent Schrödinger equation for a typical vibrational wave packet motion clearly indicated that the electron density is no longer suited to “localize” single electrons. We extended the definition of the electron localization function (ELF) to an exact, time-dependent wave function and demonstrated, how the ELF can be used to further characterize a coupled electron and nuclear motion. Finally, we gave an outlook of how to define electron localization in the case of anti-parallel electron spins. We derived a quantity similar to the ELF denoted “anti-parallel spin electron localization function” (ALF) and demonstrated that the ALF allows to follow time-dependent changes of the electron localization in a numerical example. [1] S. Shin, H. Metiu, J. Chem. Phys. 1995, 102, 9285. [2] S. Shin, H. Metiu, J. Phys. Chem. 1996, 100, 7867.
This work is subdivided into two main areas: resilient admission control and resilient routing. The work gives an overview of the state of the art of quality of service mechanisms in communication networks and proposes a categorization of admission control (AC) methods. These approaches are investigated regarding performance, more precisely, regarding the potential resource utilization by dimensioning the capacity for a network with a given topology, traffic matrix, and a required flow blocking probability. In case of a failure, the affected traffic is rerouted over backup paths which increases the traffic rate on the respective links. To guarantee the effectiveness of admission control also in failure scenarios, the increased traffic rate must be taken into account for capacity dimensioning and leads to resilient AC. Capacity dimensioning is not feasible for existing networks with already given link capacities. For the application of resilient NAC in this case, the size of distributed AC budgets must be adapted according to the traffic matrix in such a way that the maximum blocking probability for all flows is minimized and that the capacity of all links is not exceeded by the admissible traffic rate in any failure scenario. Several algorithms for the solution of that problem are presented and compared regarding their efficiency and fairness. A prototype for resilient AC was implemented in the laboratories of Siemens AG in Munich within the scope of the project KING. Resilience requires additional capacity on the backup paths for failure scenarios. The amount of this backup capacity depends on the routing and can be minimized by routing optimization. New protection switching mechanisms are presented that deviate the traffic quickly around outage locations. They are simple and can be implemented, e.g, by MPLS technology. The Self-Protecting Multi-Path (SPM) is a multi-path consisting of disjoint partial paths. The traffic is distributed over all faultless partial paths according to an optimized load balancing function both in the working case and in failure scenarios. Performance studies show that the network topology and the traffic matrix also influence the amount of required backup capacity significantly. The example of the COST-239 network illustrates that conventional shortest path routing may need 50% more capacity than the optimized SPM if all single link and node failures are protected.
Identification of rat NKT cells and molecular analysis of their surface receptor mediated activation
(2004)
Summary: Originally, NKT cells have been defined by their expression of T-cell receptor (TCR) and NK cell markers NKRP1A in human and NK1.1 (NKRP1C) in mouse. Most of these cells express CD1d-restricted TCR with a characteristic rearrangement- Va24JaQ/Vb11 in human and Va14Ja18/Vb8.2 in mouse, and have been implicated in playing an important role in first line defence and immunoregulation. The subject of this thesis was the characterisation of the hypothetical rat NKT cell population. In the mouse system, CD1d-restricted NK1.1+ T cells represented around 30% of intrahepatic and around 3% of splenic lymphocytes and could be visualised by staining with a-GalCer-loaded mouse CD1d tetramer. Rat NKRP1A+TCR+ cells, similar to mouse NKT cells, were predominantly expressed in the liver. However, their frequency was around 5 fold lower than the frequency of mouse intrahepatic lymphocytes. F344 rat NKT cells, in contrast to mouse CD4+ or DN NK1.1+ T lymphocytes, were of CD8 rather than CD4 phenotype, and did not bind to mCD1d-a-GalCer-tetramer. Since human hepatic CD1d-restricted Va24JQ+ T cells are not as frequent as their mouse counterparts and may express CD8- a marker not expressed by mouse CD1d-restricted cells, it is possible that the phenotype of F344 rat NKT cells corresponds more to the phenotype of human than mouse NKT cells. Similar to mouse NKT cells, F344 rat liver- and spleen-derived lymphocytes were able to produce IL-4 and IFN-g; when stimulated with the synthetic ligand a-GalCer in vitro. Therefore, the lack of binding of rat lymphocytes to mouse CD1d tetramer could not be due to their inability to respond to a-GalCer. To better characterise the reactivity of rat NKRP1A+TCR+ cells to a-GalCer, the rat invariant TCR was analysed. RT-PCR of liver lymphocytes with Va14-specific primers and subsequent cloning revealed a much weaker PCR signal for rat lymphocyte cDNA than for mouse cDNA. Furthermore the analysis of rat AV14JA18 sequences showed that the rat Va14+TCR invariant could be rearranged not only with AJ18 but also with other AJ segments. The low number of clones with in frame Va14Ja18 rearrangement could suggest that only a small proportion of liver lymphocytes were CD1d restricted NKT cells. Mouse and human NKT cells are able to recognise a-GalCer presented by the CD1d-b2 microglobulin complex, leading to their activation, proliferation and cytokine secretion. In order to compare the capacity of mouse and rat CD1d to present a-GalCer, rat CD1d was cloned. Sequence analysis and functional tests in vitro confirmed the structural and functional homology of rat CD1d with mouse CD1d. In parallel, to characterise the reactivity of rat NKRP1A+TCR+ cells to a-GalCer, rat Va14+TCR invariant was cloned and expressed in the TCR- T cell hybridoma BWr/mCD28. Rat Va14TCR+CD28+ transgenic cells secreted IL-2 upon aTCR/CD3 antibody stimulation, but were not specific for a-GalCer. Such cells were also negative in staining with mCD1d-a-GalCer tetramer. The lack of reactivity to a-GalCer and the lack of binding to mouse tetramer were probably caused by amino acid alterations, particularly at position 72 (51 according to IMTG nomenclature) of cloned rat TCRinv. Reversal of these “alterations” using molecular biology techniques was performed but the expression of this TCR on the surface of BWr/mCD28 cells could not be achieved. In contrast to rat TCRinv, mouse Va14+TCR was fully functional and was specific for mouse CD1d tetramer. KT12 hybridoma and BWr/mCD28 cells expressing mouse TCRinv, when stimulated with a-GalCer presented by primary CD1d+ cells or rCD1d transgenic cell lines, produced IL-2 in an Ag- and CD1d-dependent manner. Transgenic lines expressing TCR comprising mouse Va14 and rat Vb8.4 responded to a-GalCer presented by rat and mouse CD1d, and bound mCD1 tetramer. By contrast, cell lines expressing TCR comprising mouse Va14 and rat Vb8.2 responded only to a-GalCer presented by rCD1d and bound weakly to mCD1d tetramer. This suggests that germ line encoded regions of the b-chain (CDR2 or CDR4) bind to species-specific determinants of CD1d. The cytokine secretion of the cell lines was inhibited by anti-CD80 mAb, indicating the importance of CD80-CD28 costimulation in their activation. To check whether rat NKT cells may exist in other rat strains, the frequency and functions of NKRP1A+TCR+ in F344 and LEW rat were compared. F344 and LEW, two rat strains expressing different allelic CD1d forms, varied slightly in the level of CD1d expression, as assessed by staining with a newly generated CD1d specific monoclonal antibody. By contrast, these rat strains differed in terms of a-GalCer recognition. NKRP1A+TCR+ cells were less frequent in LEW than in F344 rats, and did not respond to a-GalCer or the analogue OCH in vitro, a result which is of special interest considering the susceptibility of LEW but not F344 rats to experimentally induced organ specific autoimmune diseases. In summary, the rat and mouse CD1d-invariant TCR systems show a high degree of structural and functional homology, but it seems that invariant NKT cells in rat, similar to such cells in human, occur at lower frequency than in mice. TCR transgenic cell line species-specific patterns of CD1d a-GalCer reactivity will provide a valuable tool for the mapping of CD1d/TCR contacts. Also monoclonal antibodies specific for rat and mouse CD1d, generated in this study, provide valuable tools to determine CD1d protein expression in various rat tissues and will help to better characterise functions of CD1d-restricted rat T cells.
The role of DNA supercoiling in the coordinated regulation of gene expression in Helicobacter pylori
(2004)
Summary Mechanisms of global gene regulation in bacteria are not well characterized yet. Changes in global or local supercoiling of chromosomal DNA are thought to play a role in global gene silencing and gene activation. In Helicobacter pylori, a bacterium with few dedicated transcriptional regulators, the structure of some promoters indicates a dependency on DNA topology. For example, the promoter of the major flagellar subunit gene flaA (ó28-dependent) has a shorter spacing of 13 nucleotides (nt) in comparison to the consensus promoter (15 nt). Supercoiling changes might be a mechanism of gene-specific and global transcriptional regulation in this bacterium. The aim of this study was to elucidate, if changes in global supercoiling have an influence on global gene regulation in H. pylori, and on the temporal regulation of the flagellar biosynthesis pathway in this organism. In the present work, global DNA supercoiling in H. pylori was visualized for the first time, by determining the supercoiling state of plasmids under different growth conditions. Using this method, we showed that cellular supercoiling was clearly growth phase-dependent in H. pylori. Coinciding with increased supercoiling during the growth phases, transcription of the flaA gene was increased, while the transcription of a second ó28-dependent gene with regular promoter spacing (HP0472) was reduced, supporting the hypothesis that growth phase-dependency of promoters might be mediated by changes of DNA topology. Supercoiling in H. pylori could be influenced in a reproducible fashion by inhibition of gyrase using novobiocin, which led to DNA relaxation and to a concomitant decrease of flaA transcript levels. Promoter spacer mutagenesis of the flaA promoter was performed. With flaA promoters of increased or reduced length, transcription of flaA was reduced, less susceptible to supercoiling changes, and, under specific conditions, inverted as compared to the wild type promoter. Transcriptional interdependence between the coupled topA-flaB genes and flaA was found by analysis of the flaA promoter mutants. Chromosomally linked gyrA-flgR, and topA-flaB genes were all dependent on supercoiling and coregulated with each other. Comprehensive transcript profiling (DNA microarrays) of wildtype H. pylori with and without novobiocin treatment identified a number of genes (10% of total genes), including flagellin, virulence and housekeeping genes, which were strongly dependent on and appeared to be synchronized by supercoiling changes (transcriptional up- or downregulation). These findings indicate a tightly coupled temporal regulation of flagellar biogenesis and metabolism in H. pylori, dependent on global supercoiling. A specific group of genes was also regulated in H. pylori by overexpression of Topoisomerase I, as detected by genome-wide analysis (DNA microarray). The DNA-bending protein HU is thought to be responsible for influencing the negative supercoiling of DNA, through its ability to wrap DNA. HU is encoded by the hup single gene in H. pylori, and constitutively expressed during the whole growth curve. An H. pylori hup mutant was constructed. H. pylori cells lacking HU protein were viable, but exhibited a severe growth defect. Our data indicate that the lack of HU dramatically changes global DNA supercoiling, indicating an important function of HU in chromosome structuring in H. pylori. Transcriptome analyses were performed and demonstrated that a total of 66 genes were differentially transcribed upon hup deletion, which include virulence genes and many other cell functions. The data indicate that HU might act as further important global regulator in H. pylori. Increased gene expression of heat shock proteins and a decreased transcription of the urease gene cluster may indicate a co-ordinated response of H. pylori to changes of environmental conditions in its specific ecological niche, mediated by HU. After the whole genomic sequences of H. pylori strains 26695 and J99 were published, two ORFs (HP0116 and HP0440) were presumptively annotated as topoisomerase I orthologs. HP0116 is the functional H. pylori topoisomerase I (TopA). HP0440 (topA2) was found in only few (5 of 43) strains. Western blot analysis indicated that TopA2 is antigenically different from TopA. TopA2 is transcribed in H. pylori, but the protein must be functionally different from TopA, since it is lacking one functionally essential zinc finger motif, and was not able to functionally complement a TopA-deficient E. coli. Like topA, topA2 was also transcribed in a growth phase-dependent manner. We did not find a function of TopA2 in DNA structuring or topology, but, in the present study, we were able for the first time to establish a unique function for TopA2 in global gene regulation, by comprehensive transcriptome analysis (DNA microarray). Transcriptome analysis showed that a total of 46 genes were differentially regulated upon topA2 deletion, which included flagellar genes and urease genes. These results suggest that TopA2 might act as a novel important regulator of both flagellar biosynthesis and urease in H. pylori.
Summary Using the facultative root hemiparasite Rhinanthus minor and Hordeum vulgare as a host, several aspects of water relations, the flows and partitioning of mineral nutrients, the flows, depositions and metabolism of abscisic acid (ABA) and zeatin type cytokinins (zeatin Z, zeatin riboside ZR, zeatin nucleotide ZN) within the host, the parasite and between host and parasite and the flows and partitioning of the transport metabolites mannitol in the parasite, and of sucrose in the host, have been studied during the study period 41 to 54 days after planting, i.e about 30 to 43 days after successful attachment of the parasite to the host. Water relations Extraction of xylem sap by the parasite from the host’s roots is facilitated by considerably higher transpiration per leaf area in the parasite than in the host and by the fact that stomata of attached Rhinanthus were wide open all day and night despite extremely high ABA concentrations in the leaves. By comparison, another related root hemiparasite, Melampyrum arvense, parasitising on various grasses in the field (botanic garden), showed normal diurnal stomatal behaviour. The abnormal behaviour of Rhinanthus stomata was not due to anatomical reasons as closure could be induced by applying high external ABA concentrations. Remarkable differences have been detected between the hydraulic conductance of barley seminal roots showing relatively low values, and that of Rhinanthus the seminal root showing very high values. The latter could be related to the observed high ABA concentrations in these roots. Whole plant water uptake, transpirational losses, growth-dependent deposition and the flows of water within the plants have been measured in singly growing Rhinanthus and Hordeum plants and in the parasitic association between the two. Water uptake, deposition and transpiration in Rhinanthus were dramatically increased after attachment to the barley host; most of the water used by the parasite was extracted as xylem sap from the host, thereby scavenging 20% of the total water taken up by the host’s roots. This water uptake by the parasitised host, however, due to a parasite induced reduction in the hosts growth, was decreased by 22% as compared to non- parasitised barley. The overall changes in growth-related water deposition in host and parasite pointed to decreased shoot and relatively favoured root growth in the host and to strongly favoured shoot growth and less strongly increased root growth only in the parasite. These changes in the host became more severe, when more than one Rhinanthus was parasitising one barley plant. Mineral nutrients relations 5 mM NO3- supply In parasitising Rhinanthus shoot growth was 12-fold, but root growth only twofold increased compared to the non-parasitising (very small) plants. On the other hand, in the Hordeum host, shoot dry matter growth was clearly reduced, by 33% in leaf laminae and by 52% in leaf sheaths, whereas root growth was only slightly reduced as a consequence of parasitism. Growth-dependent increments of total N and P and of K, Ca and Mg in parasitising Rhinanthus shoot were strongly increased, particularly increments of total N and P, which were 18 and 42 times, respectively, higher than in the small solitary Rhinanthus. On the other hand, increments of the above mineral nutrients in leaf sheaths of parasitised Hordeum vulgare were more strongly decreased than in leaf laminae in response to parasitic attack. Estimation of the flows of nutrients revealed that Rhinanthus withdrew from the host xylem sap about the same percentage of each nutrients: 18% of total N, 22% of P and 20% of K. Within the host almost all net flows of nutrient ions were decreased due to parasitism, but retranslocation from shoot to root-as related to xylem flow-was somewhat increased for all nutrients. Quantitative information is provided to show that the substantially increased growth in the shoot of attached Rhinanthus and the observed decrease in Hordeum shoot growth after infection were related to strongly elevated supply of nitrogen and phosphorus in the parasite and to incipient deficiency of these nutrients in the parasitised host. The flows of nutrients between host and parasite are discussed in terms of low selectivity of nutrient abstraction from the host xylem by the hemiparasite Rhinanthus minor. 1 mM NO3- or 1 mM NH4+ supply Rhinanthus shoot growth as measured by dry matter increase, was 19-fold (1 mM NO3-) and 15-fold (1 mM NH4+), but root growth only twofold (1 mM NO3-) and 2.9-fold (1 mM NH4+) increased-relative to singly growing Rhinanthus-when parasitising on host barley. In the Hordeum host, shoot dry matter growth was clearly reduced, whereas root growth was only slightly affected. Growth-dependent increments of total N and P and of K, Ca and Mg in parasitising Rhinanthus shoot were strongly increased, particularly increments of total N or of P, which were 20 or 53 times (1 mM NO3-) and 18 or 51 times (1 mM NH4+) , respectively, higher than those in solitary Rhinanthus. Within the host almost all net flows of nutrient ions were decreased due to parasitism. Flows of mannitol in parasite and sucrose flows in host barley When the plants were supplied with 5 mM NO3-, the biosynthesis of mannitol in Rhinanthus shoots increased 16-fold by parasitism, resulting in a 15-fold higher mannitol flow in the phloem and a 10-fold higher deposition in the shoot. Also the backward transport of mannitol in the xylem were increased 10-fold after attachment. Lower level nitrogen supply increased the deposition of mannitol in both single and attached Rhinanthus shoot and root. No mannitol was found in barley roots even in the direct vicinity of the haustoria. This indicates there are no backward transport of xylem sap from parasite to host. Compared to unparasitised barley, the net biosynthesis and deposition of sucrose in the shoot and the phloem flow was decreased substantially when plants were supplied with 5 mM NO3- or 1 mM NO3-. No sucrose has been detected in barley xylem sap and consequently there was no indication of a sucrose transfer from the host to the parasite. A possible involvement of mannitol in the abscisic acid relations of the parasite is discussed. ABA relations When the plants were supplied with 5 mM NO3-, there were weak or no effects of parasitism on ABA flows, biosynthesis and ABA degradation in barley. However, ABA growth-dependent deposition was significantly increased in the leaf laminae (3 fold) and in leaf sheath (2.4 fold), but not in roots. Dramatic changes in ABA flows, metabolism and deposition on a per plant basis, however, have been observed in Rhinanthus. Biosynthesis in the roots was 12-fold higher after attachment resulting in 14-fold higher ABA flows in the xylem. A large portion of this ABA was metabolised, a small portion was deposited. Phloem flows of ABA were increased 13-fold after attachment. The concentrations of ABA in tissues and xylem sap were higher in attached Rhinanthus by an order of magnitude than in host tissues and xylem sap. Similar dramatic difference existed when comparing the high concentrations in the xylem sap of single Rhinanthus with unparasitised barley. As compared to 5 mM NO3-, lower NO3- or 1 mM NH4+ supply doubled the ABA concentrations in barley leaf laminae, while having only small or no significant effects in the other organs. The possible special functions of ABA for the parasite are discussed. Zeatin type cytokinins relations Parasitism decreased, in the case of zeatin (Z), the synthesis (by 57%) in the root, xylem flows (by 56%) and metabolism (by 71%) in leaf laminae, however, increased the phloem flows of zeatin massively (3-fold) in host barley. The deposition of zeatin in the root of Rhinanthus and the flowing in xylem and phloem were 24, 12, 29-fold, respectively, increased after successfully attaching to the host barley. However, net biosynthesis of zeatin in Rhinanthus roots decreased by 39% after attachment. This indicates that a large portion (70%) of xylem flow of zeatin in attached Rhinanthus was extracted from the host. In singly growing Rhinanthus plants, the balance of zeatin deposition in the shoot was negative, i.e. zeatin was metabolised and exported back to root in the phloem. The xylem flows of zeatin riboside (ZR) in barley decreased by 39% after infected by Rhinanthus; phloem flow, which was 117% relative to xylem flow was less decreased (by 13%) after infection. Deposition of ZR has not been significantly affected in the leaf laminae, in leaf sheaths and roots. After parasitising on the host barley depositions in root, xylem flow and phloem flow increased 12, 18, 88–fold respectively in Rhinanthus. A large portion (57%) of xylem flow of ZR in attached Rhinanthus was extracted from the host. In single Rhinanthus increament of shoot zeatin riboside was negative and a substantial portion was degraded in shoot and the rest was retranslocated back to the root in the phloem. A significant depositions of Z and ZR were detected in the haustoria of the Rhinanthus/barley association. Flows and deposition of zeatin nucleotides also have been investigated. The possible physiological functions of the large quantities of Z and ZR derived from the host barley, for the improved growth and the stomatal opening in the parasitising Rhinanthus are discussed.
The availability of coherent soft x-rays through the nonlinear optical process of high-harmonic generation allows for the monitoring of the fastest events ever observed in the laboratory. The attosecond pulses produced are the fundamental tool for the time-resolved study of electron motion in atoms, molecules, clusters, liquids and solids in the future. However, in order to exploit the full potential of this new tool it is necessary to control the coherent soft x-ray spectra and to enhance the efficiency of conversion from laser light to the soft x-ray region in the harmonic-generation process. This work developed a comprehensive approach towards the optimization of the harmonic generation process. As this process represents a fundamental example of \emph{light}--\emph{matter} interaction there are two ways of controlling it: Shaping the generating laser \emph{light} and designing ideal states of \emph{matter} for the conversion medium. Either of these approaches was closely examined. In addition, going far beyond simply enhancing the conversion process it could be shown that the qualitative spectral response of the process can be modified by shaping the driving laser pulse. This opens the door to a completely new field of research: Optimal quantum control in the attosecond soft x-ray region---the realm of electron dynamics. In the same way as it is possible to control molecular or lattice vibrational dynamics with adaptively shaped femtosecond laser pulses these days, it will now be feasible to perform real-time manipulation of tightly bound electron motion with adaptively shaped attosecond light fields. The last part of this work demonstrated the capability of the herein developed technique of coherent soft-x-ray spectral shaping, where a measured experimental feedback was used to perform a closed-loop optimization of the interaction of shaped soft x-ray light with a sulfur hexafluoride molecule to arrive at different control objectives. For the optimization of the high-harmonic-generation process by engineering the conversion medium, both the gas phase and the liquid phase were explored both in experiment and theory. Molecular media were demonstrated to behave more efficiently than commonly used atomic targets when elliptically polarized driving laser pulses are applied. Theory predicted enhancement of harmonic generation for linearly polarized driving fields when the internuclear distance is increased. Reasons for this are identified as the increased overlap of the returning electron wavefunction due to molecular geometry and the control over the delocalization of the initial electronic state leading to less quantum-mechanical spreading of the electron wavepacket during continuum propagation. A new experimental scheme has been worked out, using the method of molecular wavepacket generation as a tool to enhance the harmonic conversion efficiency in `pump--drive' schemes. The latter was then experimentally implemented in the study of high-harmonic generation from water microdroplets. A transition between the dominant laser--soft-x-ray conversion mechanisms could be observed, identifying plasma-breakdown as the fundamental limit of high-density high-harmonic generation. Harmonics up to the 27th order were observed for optimally laser-prepared water droplets. To control the high-harmonic generation process by the application of shaped laser light fields a laser-pulse shaper based on a deformable membrane mirror was built. Pulse-shape optimization resulted in increased high-harmonic generation efficiency --- but more importantly the qualitative shape of the spectral response could be significantly modified for high-harmonic generation in waveguides. By adaptive optimization employing closed-loop strategies it was possible to selectively generate narrow (single harmonics) and broad bands of harmonic emission. Tunability could be demonstrated both for single harmonic orders and larger regions of several harmonics. Whereas any previous experiment reported to date always produced a plateau of equally intense harmonics, it has been possible to demonstrate ``untypical'' harmonic soft x-ray spectra exhibiting ``switched-off'' harmonic orders. The high degree of controllability paves the way for quantum control experiments in the soft x-ray spectral region. It was also demonstrated that the degree of control over the soft x-ray shape depends on the high-harmonic generation geometry. Experiments performed in the gas jet could not change the relative emission strengths of neighboring harmonic orders. In the waveguide geometry, the relative harmonic yield of neighboring orders could be modified at high contrast ratios. A simulation based solely on the single atom response could not reproduce the experimentally observed contrast ratios, pointing to the importance of propagation (phase matching) effects as a reason for the high degree of controllability observed in capillaries, answering long-standing debates in the field. A prototype experiment was presented demonstrating the versatility of the developed soft x-ray shaping technique for quantum control in this hitherto unexplored wavelength region. Shaped high-harmonic spectra were again used in an adaptive feedback loop experiment to control the gas-phase photodissociation reaction of SF$_6$ molecules. A time-of-flight mass spectrometer was used for the detection of the ionic fragments. The branching ratios of particular fragmentation channels could be varied by optimally shaped soft x-ray light fields. Although in one case only slight changes of the branching ratio were possible, an optimal solution was found, proving the sufficient technical stability of this unique coherent soft-x-ray shaping method for future applications in optimal control. Active shaping of the spectral amplitude in coherent spectral regions of $\sim$10~eV bandwidth was shown to directly correspond to shaping the temporal features of the emerging soft x-ray pulses on sub-femtosecond time scales. This can be understood by the dualism of frequency and time with the Fourier transformation acting as translator. A quantum-mechanical simulation was used to clarify the magnitude of temporal control over the shape of the attosecond pulses produced in the high-harmonic-generation process. In conjunction with the experimental results, the first attosecond time-scale pulse shaper could thus be demonstrated in this work. The availability of femtosecond pulse shapers opened the field of adaptive femtosecond quantum control. The milestone idea of closed-loop feedback control to be implemented experimentally was expressed by Judson and Rabitz in their seminal work titled ``Teaching lasers to control molecules''. This present work extends and turns around this statement. Two fundamentally new achievements can now be added, which are ``Teaching molecules to control laser light conversion'' and ``Teaching lasers to control coherent soft x-ray light''. The original idea thus enabled the leap from femtosecond control of molecular dynamics into the new field of attosecond control of electron motion to be explored in the future. The \emph{closed}-loop approach could really \emph{open} the door towards fascinating new perspectives in science. Coming back to the introduction in order to close the loop, let us reconsider the analogy to the general chemical reaction. Photonic reaction control was presented by designing and engineering effective media (catalysts) and controlling the preparation of educt photons within the shaped laser pulses to selectively produce desired photonic target states in the soft x-ray spectral region. These newly synthesized target states in turn could be shown to be effective in the control of chemical reactions. The next step to be accomplished will be the control of sub-femtosecond time-scale electronic reactions with adaptively controlled coherent soft x-ray photon bunches. To that end a time-of-flight high-energy photoelectron spectrometer has recently been built, which will now allow to directly monitor electronic dynamics in atomic, molecular or solid state systems. Fundamentally new insights and applications of the nonlinear interaction of shaped attosecond soft x-ray pulses with matter can be expected from these experiments.
This thesis is concerned with the development of an on-line in-situ device for a chemical characterisation of flowing aerosols. The thesis describes the principles and most important features of such a system, allowing also on-line measurements using Raman spectroscopy as a diagnostic technique An analysis of the effect of forced oscillations on the motion of the particle dispersed in a gas flow is given in Chapter 2. Also the most important particle parameters are introduced. A review of the particle/fluid interaction in laminar air flows and the response of the particle is presented. In Chapter 3 the behaviour of the particle under different external conditions (ion bombardment and electric fields) is extended. A brief review of the most important particle charging theories (diffusion, field, and alternating potential charging) shows, that the effect of the electrical properties (represented by the dielectric constant) of the particles affects the charging process. A non-contact method for particle charge measurement was also presented. In the second part of the chapter, the interaction between the electric field and the charged particle for the purpose of particle trapping is illustrated. The most common systems like the two or four ring electrodynamic balance and the quadrupole trap are pointed out. In Chapter 4 a short review of the possibility of using scattered light to study aerosol particles is presented. First, the conditions and the facilities of using the Mie theory for particle size and refractive index determination are mentioned, then some features concerning the classical treatment of the Raman effect are presented Supported by the theoretical considerations exposed in Chapter 2, 3, and 4 the construction and the tests of different devices are presented in Chapter 5. Following the goal of the thesis, first an overview of the used materials and methods for particle generation is presented. Then, the constructed charging devices are described (from the mechanical and electrical point of view) and compared by measuring the acquired charge on the particle. Charged particles can be trapped in different containers. Two types of axially symmetric electrodynamic balances (two ring or an extended four ring configuration) were presented. For a deeper understanding these systems were studied using analytic and numerical methods. Considering the presented purpose of the work another type of trapping system has been developed, namely the quadrupole trap. A similar theoretical characterisation (in term’s of Mathieu equation) as for the electrodynamic balance was presented pointing out some specific features of this system. The incoming particle stream will be focused to the centre of the system simultaneously also the applied DC and AC potential onto the tube electrodes, yields a stable trapping of one or more particles. Chapter 6 consists of two parts: the system for single particle and for many particles investigation. The individual devices presented in Chapter 5 are now put together. The first part presents the method and the experimental realisation of a set-up for solid particle injection. In order to suppress the phase injection disadvantage found for the electrodynamic balance a developed program processes the information obtained from a particle cloud through an adequate electronic detection system, and reduces the number of particles until just one single particle is trapped. The method for one particle investigation can be extended for many particles. Using the presented set-up the particles are moved from one quadrupole to another and transformed from a particle cloud to a particle stream. A linearity between an external vertical mounted detector and the formed image of the particle stream on the CCD camera has been observed and used for simultaneous detection of many particles by Raman spectroscopy. For both methods Raman results are presented. One limitation of Raman Spectroscopy is the relatively long integration time needed for adequate signal-to-noise ratio. There are two factors which influence the integration time: first the incident radiation and the detector sensitivity, and second the intensity of the Raman bands. Using a CCD detector, the desired detector sensitivity should be achieved. So, the improvement of the signal-to-noise ratio should be the next goal in the system development. In order to reduce the integration time an optical system including optic fibres and the integration of an FT-Raman module operating in the visible region is planed. The goal of this work was to develop and construct an instrument for on-line in-situ single particle investigation by Raman spectroscopy. With the presented experimental set-up and the developed program the purpose of the work, the on-line in-situ near atmospheric pressure aerosol investigation was achieved. The Raman spectroscopy has been used successfully for a chemical characterisation of the aerosol particles.
The success of diagnostic knowledge systems has been proved over the last decades. Nowadays, intelligent systems are embedded in machines within various domains or are used in interaction with a user for solving problems. However, although such systems have been applied very successfully the development of a knowledge system is still a critical issue. Similarly to projects dealing with customized software at a highly innovative level a precise specification often cannot be given in advance. Moreover, necessary requirements of the knowledge system can be defined not until the project has been started or are changing during the development phase. Many success factors depend on the feedback given by users, which can be provided if preliminary demonstrations of the system can be delivered as soon as possible, e.g., for interactive systems validation the duration of the system dialog. This thesis motivates that classical, document-centered approaches cannot be applied in such a setting. We cope with this problem by introducing an agile process model for developing diagnostic knowledge systems, mainly inspired by the ideas of the eXtreme Programming methodology known in software engineering. The main aim of the presented work is to simplify the engineering process for domain specialists formalizing the knowledge themselves. The engineering process is supported at a primary level by the introduction of knowledge containers, that define an organized view of knowledge contained in the system. Consequently, we provide structured procedures as a recommendation for filling these containers. The actual knowledge is acquired and formalized right from start, and the integration to runnable knowledge systems is done continuously in order to allow for an early and concrete feedback. In contrast to related prototyping approaches the validity and maintainability of the collected knowledge is ensured by appropriate test methods and restructuring techniques, respectively. Additionally, we propose learning methods to support the knowledge acquisition process sufficiently. The practical significance of the process model strongly depends on the available tools supporting the application of the process model. We present the system family d3web and especially the system d3web.KnowME as a highly integrated development environment for diagnostic knowledge systems. The process model and its activities, respectively, are evaluated in two real life applications: in a medical and in an environmental project the benefits of the agile development are clearly demonstrated.
One primary source for self-knowledge is social comparison. Often objective criteria for self-evaluations are not available or useful and therefore comparisons with other people play a crucial role in self-evaluations. But the question is whether social comparisons could indeed provide information about the self without consuming too much cognitive resources or time. Therefore, in this research I wanted to look at practice effects in social comparison and the particular significance of routine standards. Whereas traditional research on standard selection mostly focused on goal-oriented and strategic standard selection processes, this research sets out to integrate social cognitive knowledge, ideas, and methods. Researchers from many different fields agree that people’s behavior and thinking is not fully determined by rational choices or normative considerations. Quite the contrary, factors like knowledge accessibility, habits, procedural practice, stereotyping, categorization, and many more cognitive processes play an important role. The same may be true in social comparison and standard selection. In my research I demonstrate that efficiency concerns play an important role in social comparison. Since people may not be able to engage in a strategic standard selection whenever they engage in social comparison processes, there has to be a more efficient alternative. Using routine standards would be such an alternative. The efficiency advantage of routine standards may thereby be founded not only in the abandonment of a strategic but arduous standard selection process, but also in a higher efficiency of the comparison process itself. I therefore set out to show how the use of routine standards facilitates the social comparison processes. This was done in three steps. First, I replicated and improved our former research (Mussweiler & Rüter, 2003, JPSP) indicating that people really do use their best friends as routine standards to evaluate themselves. Second, I demonstrated that it is more efficient to compare with a routine standard than with another standard. In Studies 2 and 3 I therefore show that comparisons between the self and a routine standard (either a natural routine standard like the best friend or a experimentally induced routine standard based on practice) are faster and more efficient than comparisons with other standards. Finally, I looked at the underlying mechanism of the efficiency advantage of routine standards. The results of Studies 4 and 5 point out, that both general as well as specific practice effects occur with repeated comparisons. Whereas a specific practice effect implies the repeated processing of the same content (i.e., knowledge about the routine standard), general practice effects indicate that the pure process (i.e., comparing the self with a routine standard) becomes more efficient regardless whether new content (i.e., comparison relevant knowledge) has to be processed. Taken together, the efficiency advantage of routine standards during self-evaluation is based not only on the lack of necessity for an arduous standard selection, but is additionally supported by the facilitation of the comparison process itself. The efficiency of routine standards may provide an explanation as to why people base self-evaluations on comparisons with these standards and dispense with strategic considerations to select the most suitable standard.
Cellular proliferation, differentiation and survival in response to extracellular signals are controlled by the signal transduction pathway of Ras, Raf and MAP kinase. The Raf proteins are serine/threonine kinases with essential function in growth/differentiation/survival - related signal transduction events. In mammals, three functional (A-, B-, and C-Raf) genes were described. Biochemical studies suggest overlapping and differential utilization of Raf isozymes. However, the frequent co-expression of Raf isozymes and their multiple activators and effectors impedes the full understanding of their specific roles. The elucidation of these roles is important due to the involvement of the Ras/Raf/MEK/MAP kinase cascade in human disorders especially in tumor development and progression. B-Raf was shown to posses the strongest kinase activity among Raf kinases and display antiapoptotic properties. Mice deficient in B-Raf show overall growth retardation and die between E10.5 and E12.5 of vascular defects caused by excessive death of differentiated endothelial cells. To elucidate the redundancy of Raf isozymes during embryonic development and to rescue B-Raf-/- (KO) phenotype, B-Raf alleles were disrupted by introducing A-Raf cDNA under the control of endogenous B-Raf promoter. The resulting BRaf A-Raf/A-Raf (KIN) phenotype depends on genetic background. The living embryos displaying normal development but size reduction were found with low incidence at E12.5d-16.5d. All of them displayed the rescue of vascular system. One adult p20 mouse without any visible defects in development and behavior was obtained. On the other hand, the processes of neurogenesis and neural precursors migration in survived embryos were disturbed which led in some cases to underdevelopment of different brain compartments. TUNEL and cell proliferation (PCNA staining) assays revealed more apoptotic (E13.5d) and less proliferating(E12.5d cells within ventricular and sub-ventricular zones of brain ventricles and in striatum of KIN embryos. In addition, more apoptotic cells were detected in many other tissues of E13.5d and in lung of E16.5d KIN embryos but not in adult KIN mouse. p20 KIN mouse demonstrated reduced fraction of neural precursor cells in sub-granular zone of hippocampus and mature neurons in olfactory bulb. The other processes of neurogenesis were not disturbed in adult KIN animal. Fibroblasts obtained from KIN embryos demonstrated less proliferative ability and were more susceptible to apoptotic stimuli compared to WT. This was accompanied by the reduction of active ERK and Akt required for survival, and with decrease of inactive phosphorylated BAD. The kinetic of both ERK and Akt phosphorylation upon serum stimulation was delayed. All these data indicate that moderate A-Raf kinase activity can prevent the endothelial apoptosis but is not enough to completely rescue the other developmental consequences.
The development and in-depth characterization of new fluoroaryl functionalized ORMOCER® materials (inorganic-organic hybrid polymers) for optical waveguide applications in telecommunication is presented. The preparation of the materials included precursor silane synthesis, hydrolysis/polycondensation of organoalkoxysilane mixtures, and photolithographic processing of the resulting oligosiloxane resins in order to establish the inorganic-organic hybrid network. During all stages of ORMOCER® preparation, structure-property relations were deduced from characterization data, particularly with respect to low optical loss in the important near-infrared spectral region as well as refractive index. With the aid of molecular modeling, structural characteristics of oligomeric intermediates were visualized, which was found valuable in the fundamental understanding of the material class. The material development started with the syntheses of a variety of commercially unavailable fluorinated and unfluorinated arylalkoxysilanes by means of Grignard and hydrosilylation pathways, respectively. A survey of silane optical properties, particularly their absorptions at the telecom wavelengths 1310 nm and 1550 nm, gave an impulse to the choice of suitable precursors for the preparation of low-loss ORMOCER® resins. Accordingly, precursor silane mixtures and hydrolysis/polycondensation reaction conditions were chosen and optimized with regard to low contents of C-H and Si-OH functions. Thus, absorptions as low as 0.04 dB/cm at 1310 nm and 0.18 dB/cm at 1550 nm, respectively, could be obtained from an oligosiloxane resin based on pentafluorophenyltrimethoxysilane (1) mixed with pentafluorophenyl(vinyl)-dimethoxysilane (5). In order to improve the organic crosslinkability under photolithographic processing conditions, further resins on the basis of the aforementioned were prepared, which additionally incorporated the styrene-analogous precursor 4-vinyltetrafluorophenyl-trimethoxysilane (4). Thus, ORMOCER® resins with low optical losses of 0.28 dB/cm at 1310 nm and 0.42 dB/cm at 1550 nm, respectively, were prepared, which exhibited excellent photopatternability. The manufacture of micropatterns such as optical waveguide structures by UV-photolithography under clean room conditions was the final stage of material synthesis. The optimization of processing parameters allowed the preparation of test patterns for the determination of optical, dielectrical and mechanical properties. A low optical loss of 0.51 dB/cm at 1550 nm could be measured on a waveguide manufactured from a photopatternable fluoroaryl functionalized ORMOCER®. The structural characterization of liquid resins as well as cured ORMOCER® samples was accomplished chiefly with solution and solid state 29Si-NMR spectroscopy, respectively. Particularly for polycondensates incorporating species based on more than one precursor silane, the spectra showed a high degree of complexity. An additional challenge arouse from the partial loss of fluoroaryl groups during ORMOCER® condensation and curing, which resulted in even more condensation products. Thus, in order to provide a basis for resin analysis, first the hydrolysis/condensation reactions of the isolated precursors were investigated under reaction time-resolution with NMR spectroscopy at low temperature. Backed by signal assignments in these single-precursor systems, the respective species could also be identified in the complex resin spectra, allowing for their quantitative interpretation. The structural characterization was rounded out by IR spectroscopy and SAXS analyses. With the help of molecular modeling, the experimental data were finally transferred into a three-dimensional image of an organosiloxane oligomer, which is representative for a photopatternable fluoroaryl functionalized ORMOCER® resin. The combination of low-temperature NMR, which made the characterization of polycondensates possible, with oligomer modeling paved the way to a further understanding of ORMOCER® resin systems. On the basis of this visualization of structural characteristics, e.g. properties such as organic crosslinkability of oligomers were discussed in the light of steric features within the molecular structure. Thus, new possibilities were established for the systematic optimization of ORMOCER® formulations. Structure-property relations with respect to optical loss and refraction, as determined within this work, follow trends, which are in accordance with the literature. Particularly the direct comparison of data derived from analogous fluorinated and unfluorinated ORMOCER® resins showed that fluorination results in significant decrease in NIR optical loss. Additionally, different unfluorinated aryl functionalized systems with varying aliphatic C-H content were compared. In case of a lower aliphatic content, a widening effect on the 1310 nm window was found. This is due to a shift of arylic C-H vibrations (1145 nm) towards lower wavelengths compared to aliphatic C-H (1188 nm). Finally, on the basis of NIR spectra of analogous fluorinated resins with low and high silanol content, respectively, a significant impact of (Si)O-H groups on the 1550 nm window was demonstrated, while the 1310 nm window was unaffected. This is due to O-H vibrations with a maximum at 1387 nm and further bands at higher wavelength. The index of refraction was drastically lowered due to fluorination. Thus, the analogous fluorinated and unfluorinated ORMOCER® resins had indices of 1.497 and 1.570, respectively, in the VIS region. For the fluorinated systems, refraction did not change significantly during organic cross-connection and hardbake. In conclusion, the new fluoroaryl functionalized ORMOCER® systems represent low-loss materials for telecom applications. In addition, in-depth characterization during material development allowed the proposal of structure-property relations, particularly with respect to optical properties, which are of considerable importance for future developments.
The present work consist of two major parts. The first part, extending over chapters 1, 2, 3 and 4, addresses the design and construction of a device capable of determining the shell thickness and the core size for monolayer spherical particles in a flow. The second part containing chapters 5, 6, 7, 8, 9 and 10, concentrate on the use of Raman spectroscopy as a space application, namely for use as a tool for in situ planetary investigations. This part directly addresses the MIRAS project, a study run under the auspices of Federal Ministry of Education and Research, BMBF and German Aerospace Center, DLR under national registration number 50OW0103. MIRAS stands for "Mineral Investigation by in situ Raman Spectroscopy". Microcapsule Sizing by Elastic Light Scattering The industrial development of processes based on microcapsules depends on the possibility to provide clear and complete information about the properties of these microcapsules. However, the tools for an easy and efficient determination of the microcapsule properties are lacking, several methods being often required to describe adequately the microcapsule behavior. Methods for evaluating the individual size and size distribution of both the core and the shell are required together with methods for measuring the mechanical strength, stability in appli-cation media, permeability of the shell, etc. Elastic light scattering measurements provide a possible way of determining properties such as core size, shell size and refractive index. The design and con-struction of a device capable of measuring the above mentioned parameters for a core-shell particle is the subject of the first part of this thesis. The basic principle of measurement for the device proposed here consists of an-alyzing one particle at a time by recording the elastic light scattering pattern at angles between approx. 60 and 120 grad. By comparing the experimentally recorded phase functions with the previously calculated phase functions stored in a database, the geometry of the scattering object can be identified. In our case the geometry is characterized by two parameters: the shell thickness and the core radius. In chapter 2 a short overview on the methods used for sizing microparticles is given. Different sizing methods are compared, and the advantages and disadvan-tages for the general problem of sizing are shortly discussed. It is observed that all sizing methods that are based on elastic light scattering theories are ensemble methods. Chapter 3 focusses on the theories used for calculating the theoretical scattering patterns with emphasize on the Mie theory. The generalization of Mie theory for layered particles is shortly presented and the far field intensity approximations are discussed. The last chapter (4) of this first part describes the experimental approach for building an automatic microcapsule sizer. The approach started by O. Sbanski [76] with the development of a software packet for calculating and storing theoret-ical phase functions for core-shell particles was continued with the designing and construction of a measuring device. The hardware construction and the software with all implemented corrections imposed by the individual setup components are described in detail. For the laser, the monochromaticity, the intensity profile of the beam as well as the planarity of the equi-phase fronts are taken into consid-eration. The flow cell with three different designs is described, and the influences of the employed design on the light scattering patterns are discussed together with the optical system used for recording the experimental phase functions. The detection system formed by two identical linear CCD arrays is presented together with the software approach used for data acquisition. Ways of improving the quality and the speed of the analyzing process are discussed. The final section presents measurements run on samples made of homogeneous spheres and also on samples containing industrial microcapsules. Mineral Investigation by in situ Raman Spectroscopy The envisaged future planetary missions require space-born instruments, which are highly miniaturized with respect to volume and mass and which have low needs of power. A micro Raman spectrometer as a stand alone device on a planetary surface (e.g. Mars) offers a wide spectrum of possibilities. It can assess the chemical analysis via determination of the mineral composition, detect organic molecules in the soil, identify the principal mineral phases, etc. The technical developments in the last years have introduced a new generation of small Raman systems suitable for robotic mineral characterization on planetary surfaces [20, 95]. Two different types of spectrometer were considered for the MIRAS study. As supporting laboratory experiments for the MIRAS study, the measure-ments on standard minerals and on SNC Mars meteorites are discussed in chapter 6. The following SNC meteorites have been investigated: Sayh al Uhaymir 060, Dar al Gani 735, Dar al Gani 476, Northwest Africa 856, Los Angeles, Northwest Africa 1068 and Zagami. Pyrite as a hitherto undescribed phase in the picritic (olivin-phyric) shergottite NWA 1068 as well as reduced carbon (e.g. graphite) and anatase in the shergottite Say al Uhaymir 060 are new findings for this class of meteorites. A detailed description of the proposed designs for MIRAS, with the compo-nents used for building the test version on a breadboard is covered in chapter 7. The scientific as well as the mission requirements imposed on the instrument are discussed. The basic design is presented and the main components that are brought together to build the device being the laser unit, the Raman head, the Rayleigh filtering box, and the spectral sensor (spectrometer with a matching de-tector) are described. The two proposed designs, one based on an acousto-optic tunable filter (AOTF) and the other based on a dispersive hadamard transform spectrometer are compared to each other. The actual breadboard setup with the detailed description of the components follows in Section 7.3. Further de-velopment of a Raman spectrometer for planetary investigations is proposed in combination with a microscope as part of the Extended-MIRAS project. The software developed for controlling the breadboard version of MIRAS is described in chapter 8 together with a short description of the structure of a relational database used for in house spectra management. The measuring pro-cedures and the data processing steps are presented. Spectra acquired with the MIRAS breadboard version based on the AOTF are shown in chapter 9. The final chapter addresses a rather different possibility of using Raman spectroscopy for planetary investigations. The chapter summarizes the content of four tech-nical notes that were established within the study contracted by the European Space Agency with firma Kayser-Threde in Munich concerning the possibility of applying Raman spectroscopy in the field of remote imaging.
The present thesis encompasses two parts. The first supramolecular part focuses on the development of new flexible self-assembling zwitterions as building blocks for supramolecular polymers. In the second part, the aim was to develop bioorganic receptors for amino acids and dipeptides in aqueous media. Both research projects are based on the guanidiniocarbonyl pyrrole 1 as a new efficient binding motif for the complexation of carboxylates in polar solution.A necessary requirement for the realization of these research projects was to develop an efficient and mild synthetic approach for the cationic guanidiniocarbonyl pyrroles in general. The harsh reaction conditions of the previously used method and the problematic purification of the cationic guanidinocarbonyl pyrroles so far prevented a more extensive exploration in bioorganic and supramolecular research. In the course of this work I successfully developed a new synthesis starting with mono tBoc-protected guanidine that was coupled with a benzyl protected pyrrole carboxylic acid. After deprotection of the benzyl group, a key intermediate in the newly developed synthesis, the tBoc-protected guanidinocarbonyl pyrrole acid, was obtained. This new, mild and extremely efficient synthetic approach for the introduction of acyl guanidines is now the standard procedure in our group for the preparation of both solution and solid-phase guanidiniocarbonyl pyrroles. With this facile method at hand, a new class of flexible zwitterions, in which a carboxylate is linked via an alkyl chain to a guanidiniocarbonyl pyrrole cation was synthesized. The self-aggregation and the influence of the length and therefore flexibility of the alkyl spacer on the structure and stability of the formed aggregates were studied in solution and gas phase. In solution the aggregation was studied by NMR-dilution experiments in DMSO which suggest that flexible zwitterions with n = 1, 3 and 5 form oligomers. For n = 1, highly stable helical aggregates with nanometer size are formed. In the gas phase studies the stability and the fragmentation kinetics of a series of sodiated dimeric zwitterions with n = 2, 3 and 5 were investigated. This was done by infrared multiphoton dissociation Fourier transform ion cyclotron resonance mass spectrometry (IRMPD-FT-ICR-MS). These kinds of studies can be used in the future for a more directed design of supramolecular building blocks The bioorganic research part comprises three different projects. In a first project I synthesized four new arginine analogues which can be implemented in peptides as a substitute for arginine. Therefore, I developed the new multi-step synthesis shown below for these arginine analogues. As a test for their application in normal solid phase synthesis, I successfully prepared a tripeptide sequence Ala-AA1-Val (AA: arginine analogue. In a second project I studied the influence of additional ionic interactions within our binding motif. I synthesized a di-cationic and a tris-cationic receptor and evaluated the binding properties via NMR titration experiments against a variety of amino acids. Especially, the tris-cationic receptor was capable to strongly complex amino acids. The association constants were about a factor of 100 higher than those for the guanidiniocarbonyl pyrroles known so far. Even in 90 %water/10 % DMSO the association constants determined by NMR titration were extremely high with values around Kass = 2000 M-1. In the third project I developed a de-novo designed receptor for C-terminal dipeptides in a beta-sheet conformation based on molecular calculations. This receptor was studied in NMR and also UV titration experiments. In 40 % water/ 60 % DMSO the association constants were too strong to be measured by NMR titration experiments. Therefore, the complexation properties of 12 were studied by UV titration in water (with 10 % DMSO added for solubility reasons) with various dipeptides and amino acids as substrates. The data show that 12 binds dipeptides very efficiently even in water with association constants Kass > 10000 M-1, making 12 one of the most effective dipeptide receptors known so far. In contrast to that, simple amino acids are bound up to ten times less efficiently (Kass > 1000 M-1) than dipeptides. In the series of dipeptides studied the complex stability increases depending on the side chains present in the order Gly < Ala < Val which is a result of the decreasing flexibility of the peptide and the increasing hydrophobicity of the side chains. The binding properties of this receptor are superior to any other dipeptide receptor reported so far. Within my thesis I have not only developed an essential, mild and efficient synthetic approach for guanidiniocarbonyl pyrroles in general, but also a new binding motif for the complexation of amino acids 15, 11 and in addition a dipeptide receptor 12 that is superior to all dipeptides receptors known so far.
Nitric oxide production by tobacco plants and cell cultures under normal conditions and under stress
(2004)
Nitric oxide (NO) is a gaseous free radical involved in the regulation of diverse biochemical and physiological processes in animals. During the last decade, evidence has accumulated that NO might also play an important role as a second messenger in plants. Of special interest were observations that NO was involved in a signal chain leading to the hypersensitive response (HR) in incompatible plant-pathogen interactions. In contrast to animals, plants have probably several enzymes that may produce NO. Potential candidates are: Cytosolic nitrate reductase (NR; EC 1.6.6.1), plasma-membrane (PM)-nitrite: NO reductase (Ni:NOR), nitric oxide synthase (NOS; EC 1.14.13.39) and Xanthine dehydrogenase (XDH; EC 1.1.1.204). The major goal of this work was to quantify NO production by plants, and to identify the enzymes responsible for NO production. As a major method, NO production by tobacco leaves or cell suspensions was followed under normal, non-stress conditions, and under biotic stress, through on-line measurement of NO emission into the gas phase (chemiluminescence). Plants used were tobacco wild-type (N. tabacum cv Xanthi or cv Gatersleben), NR-free mutants grown on ammonium in order to prevent NR induction, plants grown on tungstate to inhibit synthesis of functional MoCoenzymes, and a NO-overproducing nitrite reductase (NiR)-deficient transformant. Induction of HR in tobacco leaves and in cell suspensions was achieved using the fungal peptide elicitor cryptogein. Non-elicited leaves from nitrate-grown plants showed a typical NO-emission pattern where NO-emission was low in dark, higher in the light and very high under dark-anaerobic conditions. Even at maximum rates, NO production in vivo was only a few percent of total NR activity (NRA). Consistent with that, with a solution of purified NR as a simple, “low quenching” system, NO-emission was also about 1 % of NRA. Thus, NO scavenging by leaves and stirred cell suspensions appeared small and NO-emission into purified air should give a reliable estimate of NO production. NO-emission was always high in a NiR-deficient transformant which accumulated nitrite, and NO-emission was completely absent in plants or cell suspensions which did not contain NR. Thus, in healthy plants or cell suspensions, NO-emission was exclusively due to the reduction of nitrite to NO, mainly by cytosolic NR. In addition to nitrite, cytosolic NADH appears as an important factor limiting NO production. Unexpectedly, plants (in absence of NR) were able to reduce nitrite to NO under anaerobic conditions through an unknown enzyme system that was not a MoCo-enzyme and was cyanide-sensitive. When infiltrated into leaves at nanomolar concentrations, the fungal elicitor cryptogein provoked cell death in tobacco leaves and cell suspensions. The HR could be prevented by the NO-scavengers PTIO or c-PTIO, suggesting that NO production was indeed required for the HR. However, the product of the reaction of c-PTIO with NO, c-PTI, also prevented cell death without quenching NO emission. Thus, prevention of cell death by c- PTIO is no proof for an involvement of NO. No differences were found in the HR induction between NR-free plants and/or cell suspensions and WT plants. Thus, NR appears not necessary for the HR. Further, and in contrast to literature suggestions, a continuously high NO-overproduction by a NiR-free mutant did not interfere with the development of the HR. Most surprisingly, no additional NO-emission from tobacco leaves was induced by cryptogein at any phase of the HR. In contrast, some NO-emission, paralleled by nitrite accumulation, was detected 3-6 h after cryptogein addition with nitrate grown cell suspensions, but not with NR free, ammonium- grown cells. Thus, induction of NO-emission by cryptogein appeared somehow correlated with NR and nitrite, at least in cell suspensions. But since cryptogein induced the HR even in NR-free cell suspensions, this nitrite-related NO- emission was not required for cell death. NOS inhibitors neither prevented cell death nor did they affect nitrite-dependent NO-emission. Thus, in total these data question the often proposed role of NO as a signal in the HR, and of NOS as source for NO.
The point of departure for the present work has been the following free boundary value problem for analytic functions $f$ which are defined on a domain $G \subset \mathbb{C}$ and map into the unit disk $\mathbb{D}= \{z \in \mathbb{C} : |z|<1 \}$. Problem 1: Let $z_1, \ldots, z_n$ be finitely many points in a bounded simply connected domain $G \subset \mathbb{C}$. Show that there exists a holomorphic function $f:G \to \mathbb{D}$ with critical points $z_j$ (counted with multiplicities) and no others such that $\lim_{z \to \xi} \frac{|f'(z)|}{1-|f(z)|^2}=1$ for all $\xi \in \partial G$. If $G=\mathbb{D}$, Problem 1 was solved by K?nau [5] in the case of one critical point, and for more than one critical point by Fournier and Ruscheweyh [3]. The method employed by K?nau, Fournier and Ruscheweyh easily extends to more general domains $G$, say bounded by a Dini-smooth Jordan curve, but does not work for arbitrary bounded simply connected domains. In this paper we present a new approach to Problem 1, which shows that this boundary value problem is not an isolated question in complex analysis, but is intimately connected to a number of basic open problems in conformal geometry and non-linear PDE. One of our results is a solution to Problem 1 for arbitrary simply connected domains. However, we shall see that our approach has also some other ramifications, for instance to a well-known problem due to Rellich and Wittich in PDE. Roughly speaking, this paper is broken down into two parts. In a first step we construct a conformal metric in a bounded regular domain $G\subset \mathbb{C}$ with prescribed non-positive Gaussian curvature $k(z)$ and prescribed singularities by solving the first boundary value problem for the Gaussian curvature equation $\Delta u =-k(z) e^{2u}$ in $G$ with prescribed singularities and continuous boundary data. This is related to the Berger-Nirenberg problem in Riemannian geometry, the question which functions on a surface R can arise as the Gaussian curvature of a Riemannian metric on R. The special case, where $k(z)=-4$ and the domain $G$ is bounded by finitely many analytic Jordan curves was treated by Heins [4]. In a second step we show every conformal pseudo-metric on a simply connected domain $G\subseteq \mathbb{C}$ with constant negative Gaussian curvature and isolated zeros of integer order is the pullback of the hyperbolic metric on $\mathbb{D}$ under an analytic map $f:G \to \mathbb{D}$. This extends a theorem of Liouville which deals with the case that the pseudo-metric has no zeros at all. These two steps together allow a complete solution of Problem 1. Contents: Chapter I contains the statement of the main results and connects them with some old and new problems in complex analysis, conformal geometry and PDE: the Uniformization Theorem for Riemann surfaces, the problem of Schwarz-Picard, the Berger-Nirenberg problem, Wittich's problem, etc.. Chapter II and III have preparatory character. In Chapter II we recall some basic results about ordinary differential equations in the complex plane. In our presentation we follow Laine [6], but we have reorganized the material and present a self-contained account of the basic features of Riccati, Schwarzian and second order differential equations. In Chapter III we discuss the first boundary value problem for the Poisson equation. We shall need to consider this problem in the most general situation, which does not seem to be covered in a satisfactory way in the existing literature, see [1,2]. In Chapter IV we turn to a discussion of conformal pseudo-metrics in planar domains. We focus on conformal metrics with prescribed singularities and prescribed non-positive Gaussian curvature. We shall establish the existence of such metrics, that is, we solve the corresponding Gaussian curvature equation by making use of the results of Chapter III. In Chapter V we show that every constantly curved pseudo-metric can be represented as the pullback of either the hyperbolic, the euclidean or the spherical metric under an analytic map. This is proved by using the results of Chapter II. Finally we give in Chapter VI some applications of our results. [1,2] Courant, H., Hilbert, D., Methoden der Mathematischen Physik, Erster/ Zweiter Band, Springer-Verlag, Berlin, 1931/1937. [3] Fournier, R., Ruscheweyh, St., Free boundary value problems for analytic functions in the closed unit disk, Proc. Amer. Math. Soc. (1999), 127 no. 11, 3287-3294. [4] Heins, M., On a class of conformal metrics, Nagoya Math. J. (1962), 21, 1-60. [5] K?nau, R., L?gentreue Randverzerrung bei analytischer Abbildung in hyperbolischer und sph?ischer Geometrie, Mitt. Math. Sem. Giessen (1997), 229, 45-53. [6] Laine, I., Nevanlinna Theory and Complex Differential Equations, de Gruyter, Berlin - New York, 1993.
The experimental work of this thesis addresses the questions of whether established cell lines injected into murine blastocysts find their way back home and seed preferentially at the site of their origin. Furthermore, can they change their fate and differentiate to unrelated cell types when exposed to the embryonic environment. This survey was based on the fact that different cell lines have different potentials in developing embryos, dependent on their cellular identity. The cell lines used in this survey were AGM region-deriving DAS 104-4, DAS 104-8 cells, yolk sac-deriving YSE cells and bone marrow-deriving FDCP mix cells. These cells were injected into mouse blastocysts. Donor cells were traced in developing embryos via specific markers. Analysis of the embryos revealed that DAS cells are promiscuous in their seeding pattern, since they were found in all analysed tissues with similar frequencies. YSE cells showed preferences in seeding yolk sac and liver. YSE donor cells in chimaeric tissues were not able to change their immuno-phenotype, indicating that they did not change their destiny. Analysis of adult mice did not reveal any of YSE-derived cells donor contribution. In contrast, FDCP mix cells mostly engrafted haematopoietic tissues, although the embryos analysed by in situ hybridization had donor signals frequently in cartilage primordia, heads, and livers. Analysis of whether FDCPmix-derived cells found in foetal livers were of haematopoietic or hepatocytes nature showed that progeny of injected FDCP mix cells do not differentiate into cells that express a hepatocyte-specific marker. Further analysis showed that FDCPmix-derived donor cells found in brain express neural or haematopoietic markers. In order to reveal if they transdifferentiate to neurons or fuse with neurons/glial cells, nuclear diameters of donor and recipient cells were determined. Comparison of the nuclear diameters of recipient and donor cells revealed no differences. Therefore this suggests that progeny of FDCP mix in brain are not fusion products. Analysis of adult mice tissues revealed that presence of FDCP mix-derived cells was the highest in brains. These results confirmed the assumption that the developmental potential of the analysed cells cannot be easily modified, even when exposed to early embryonic environment. Therefore one can conclude that the analysed cell types had different homing patterns depending on their origins.
Although the role of B-cells in autoimmunity is not completely understood, their importance in the pathogenesis of autoimmune diseases has been more appreciated in the past few years. It is now well known that they have roles in addition to (auto) antibody production and are involved by different mechanisms in the regulation of T-cell mediated autoimmune disorders. The evolution of an autoimmune disease is a dynamic process, which takes a course of years during which complex immunoregulatory mechanisms shape the immune repertoire until the development of clinical disease. During this course, the B-cell repertoire itself is influenced and a change in the distribution of immunoglobulin heavy and light chain genes can be observed. B-cell depletive therapies have beneficial effects in patients suffering from rheumatoid arthritis (RA), highlighting also the central role of B-cells in the pathogenesis of this disease. Nevertheless, the mechanism of action is unclear. It has been hypothesised that B-cell depletion is able to reset deviated humoral immunity. Therefore we wanted to investigate if transient B-cell depletion results in changes of the peripheral B-cell receptor repertoire. To address this issue, expressed immunoglobulin genes of two patients suffering from RA were analysed; one patient for the heavy chain repertoire (patient H), one patient for the light chain repertoire (patient L). Both patients were treated with rituximab, an anti-CD20 monoclonal antibody that selectively depletes peripheral CD20+ B-cells for several months. The B-cell repertoire was studied before therapy and at the earliest time point after B-cell regeneration in both patients. A longer follow-up (up to 27 months) was performed in patient H who was treated a second time with rituximab after 17 months. Heavy chain gene analysis was carried out by nested-PCR on bulk DNA from peripheral B-cells using family-specific primers, followed by subcloning and sequencing. During the study, patient H received two courses of antibody treatment. B-cell depletion lasted 7 and 10 months, respectively and each time was accompanied by a clinical improvement. Anti-CD20 therapy induced two types of changes in this patient. During the early phase of B-cell regeneration, we noticed the presence of an expanded and recirculating population of highly mutated B-cells. These cells expressed very different immunoglobulin VH genes compared before therapy. They were class-switched and could be detected for a short period only. The long-term changes were more subtle. Nevertheless, characteristic changes in the VH2 family, as well as in specific mini-genes like VH3-23, 4-34 or 1-69 were noticed. Some of these genes have already been reported to be biased in autoimmune diseases. Also in autoimmune diseases, in particular in RA, clonal B-cells have been frequently found in the repertoire. B-cell depletion with anti-CD20 antibody resulted in a long term loss of clonal B-cells in patient H. Thus, temporary B-cell depletion induced significant changes in the heavy chain repertoire. For the light chain gene analysis, the repertoire changes were analysed separately for naive (CD27-) and memory (CD27+) B-cells. Individual CD19+ B-cells were sorted into CD27- and CD27+ cells and single cell RT-PCR was performed, followed by direct sequencing. During the study, patient L received one course of antibody treatment. B-cell depletion lasted 10 months and the light chain repertoire was studied before and after therapy. Before therapy, some differences in the distribution of VL and JL genes were observed between naive and memory B-cells. In particular, the predominant usage of Jk-proximal Vk genes by the CD27- naive B-cells indicated that the receptor editing was less frequent in this population compared to memory cells. In VlJl rearrangements also, some evidence for decreased receptor editing was noticed, with the overrepresentation of the Jl2/3 gene segments. The CDR3 regions of naive and memory cells showed different characteristics: the activity of the terminal deoxynucleotidyl transferase and exonuclease in Vl(5’) side was greater in memory cells. Also in the light chain repertoire, we observed some changes induced by the B-cell depletive therapy. There was a tendency of a less frequent usage of Jk-proximal Vk genes in the naive population. Some Vl genes, previously described in autoimmune diseases and connected to rheumatoid factor activity, such as 3p, 3r, 1g, were not found after therapy. The different characteristics of the CDR3 regions of VlJl rearrangements were not observed anymore. Very significantly, the ratio Vk to Vl was shifted toward a greater usage of Vk genes in the naive population after therapy. Taken together, these results indicate that therapeutic transient B-cell depletion by anti-CD20 antibody therapy modulates the immunoglobulin gene repertoire in the two RA patients studied. Measurable changes were observed in the heavy chain as well as in the light chain repertoire, which may be relevant to the course of the disease. This also supports the notion that the composition of the B-cell repertoire is influenced by the disease and that B-cell depletion can reset biases that are typically found in autoimmune diseases.
In the last years more than one hundred microbial genomes have been sequenced, many of them from pathogenic bacteria. The availability of this huge amount of sequence data enormously increases our knowledge on the genome structure and plasticity, as well as on the microbial diversity and evolution. In parallel, these data are the basis for the scientific “revolution” in the field of industrial and environmental biotechnology and medical microbiology – diagnostics and therapy, development of new drugs and vaccines against infectious agents. Together with the genomic approach, other molecular biological methods such as PCR, DNA-chip technology, subtractive hybridization, transcriptomics and proteomics are of increasing importance for research on infectious diseases and public health. The aim of this work was to characterize the genome structure and -content of the probiotic Escherichia coli strain Nissle 1917 (O6:K5:H31) and to compare these data with publicly available data on the genomes of different pathogenic and non-pathogenic E. coli strains and other closely related species. A cosmid genomic library of strain Nissle 1917 was screened for clones containing the genetic determinants contributing to the successful survival in and colonization of the human body, as well as to mediate this strain’s probiotic effect as part of the intestinal microflora. Four genomic islands (GEI I-IVNissle 1917) were identifed and characterized. They contain many known fitness determinants (mch/mcm, foc, iuc, kps, ybt), as well as novel genes of unknown function, mobile genetic elements or newly identified putative fitness-contributing factors (Sat, Iha, ShiA-homologue, Ag43-homologues). All islands were found to be integrated next to tRNA genes (serX, pheV, argW and asnT, respectively). Their structure and chromosomal localization closely resembles those of analogous islands in the genome of uropathogenic E. coli strain CFT073 (O6:K2(?):H1), but they lack important virulence genes of uropathogenic E. coli (hly, cnf, prf/pap). Evidence for instability of GEI IINissle 1917 was given, since a deletion event in which IS2 elements play a role was detected. This event results in loss of a 30 kb DNA region, containing important fitness determinants (iuc, sat, iha), and therefore probably might influence the colonization capacity of Nissle 1917 strain. In addition, a screening of the sequence context of tRNA-encoding genes in the genome of Nissle 1917 was performed to identify genome wide potential integration sites of “foreign” DNA. As a result, similar “tRNA screening patterns” have been observed for strain Nissle 1917 and for the uropathogenic E. coli O6 strains (UPEC) 536 and CFT073. I. Summary 4 The molecular reason for the semi-rough phenotype and serum sensitivity of strain Nissle 1917 was analyzed. The O6-antigen polymerase-encoding gene wzy was identified, and it was shown that the reason for the semi-rough phenotype is a frame shift mutation in wzy, due to the presence of a premature stop codon. It was shown that the restoration of the O side-chain LPS polymerization by complementation with a functional wzy gene increased serumresistance of strain Nissle 1917. The results of this study show that despite the genome similarity of the E. coli strain Nissle 1917 with the UPEC strain CFT073, the strain Nissle 1917 exhibits a specific set of geno- and phenotypic features which contribute to its probiotic action. By comparison with the available data on the genomics of different species of Enterobacteriaceae, this study contributes to our understanding of the important processes such as horizontal gene transfer, deletions and rearrangements which contribute to genome diversity and -plasticity, and which are driving forces for the evolution of bacterial variants. At last, the fim, bcs and rfaH determinats whose expression contributes to the mutlicellular behaviour and biofilm formation of E. coli strain Nissle 1917 have been characterized.
Summary The nature of the chemical bond is a topic under constant debate. What is known about individual molecular properties and functional groups is often taught and rationalized by explaining Lewis structures, which, in turn, make extensive use of the valence concept. The valence concept distinguishes between electrons, which do not participate in chemical interactions (core electrons) and those, which do (single, double, triple bonds, lone-pair electrons, etc.). Additionally, individual electrons are assigned to atomic centers. The valence concept is of paramount success: It allows the successful planning of chemical syntheses and analyses, it explains the behavior of individual functional groups, and, moreover, it provides the “language” to think of and talk about molecular structure and chemical interactions. The resounding success of the valence concept may be misleading to forget its approximative character. On the other hand, quantum mechanics provide in principle a quantitative description of all chemical phenomena, but there is no discrimination between electrons in quantum mechanics. From the quantum mechanical point of view there are only indistinguishable electrons in the field of the nuclei, i.e., it is impossible to assign a given electron to a particular center or to ascribe a particular purpose to individual electrons. The concept of indistinguishability of micro particles is founded on the Heisenberg uncertainty relation, which states, that wavepackets diverge in the 6N dimensional phase space, such that individual trajectories can not be identified. Hence it is a deep-rooted and approved physical concept. As an introduction to the present work density partitioning schemes were discussed, which divide the total molecular density into chemically meaningful areas. These partitioning schemes are intimately related to either the concepts of bound atoms in a molecule (as in the Atoms In Molecules theory (AIM) according to Bader or as in the Hirshfeld partitioning scheme) or to the concept of chemical structure in the sense of Lewis structures, which divide the total molecular density into core and valence density, where the valence density is split up again into bonding and non-bonding electron densities. Examples are early and recent loge theories, the topological analysis by means of the Electron Localization Function (ELF), and the Natural Bond Orbital (NBO) approach. Of these partitioning schemes, the theories according to Bader (AIM), to Becke and Edgecomb (ELF) and according to Weinhold (NBO and Natural Resonance Theory, NRT), respectively, were reviewed in detail critically. Points of criticism were explicated for each of the mentioned theories. Since theoretically derived electron densities are to be compared to experimentally derived densities, a brief introduction into the theory of X-ray di®raction experiments was given and the multipole formalism was introduced. The procedure of density refinement was briefly discussed. Various suggestions for improvements were developed: One strategy would be the employment of model parameters, which are to a maximum degree mutually orthogonal, with the object of minimizing correlations among the model parameters, e.g., to introduce nodal planes into the radial functions of the multipole model. A further suggestion involves the guidance of the iterative refinement procedure by an extremum principle, which states, that when di®erent solutions to the least squares minimization problem are available with about the same statistical measures of quality and with about the same residual density, then the solution is to prefer, which yields a minimum density at the bond critical point (BCP) and a maximum polarity in terms of the ratio of distances between the BCP and the nuclei. This suggestion is based on the well known fact, that the bond polarity (in terms of the ratio of distances between the BCP and the respective nuclei) is underestimated in the experiment. Another suggestion for including physical constraints is the explicit consideration of the virial theorem, e.g., by evaluating the integration of the Laplacian over the entire atomic basins and comparing this value to zero and to the value obtained from the integration of the electron gradient field over the atomic surface. The next suggestion was to explicitly use the electrostatic theorem of Feynman (often also denoted as Hellmann-Feynman theorem), which states, that the forces onto the nuclei can be calculated from the purely classical electrostatic forces of the electron distribution and the nuclei distribution. For a stationary system, these forces must add to zero. This also provides an internal quality criterion of the density model. This can be performed in an iterative way during the refinement procedure or as a test of the final result. The use of the electrostatic theorem is expected to reduce significantly correlations among static density parameters and parameters describing vibrations, since it is a valuable tool to discriminate between physically reasonable and artificial static electron densities. All of these mentioned suggestions can be applied as internal quality criteria. The last suggestion is based on the idea to initiate the experimental refinement with a set of model parameters, which is, as much as possible close to the final solution. This can be achieved by performing periodic boundary conditions calculations, from which theoretically created files are obtained, which contain the Miller indices (h, k, l) and the respective intensity I. This file is used for a model parameter estimation (refinement), which excludes vibrations. The resulting parameters can be used for the experimental refinement, where, in a first step, the density parameters are fixed to determine the parameters describing vibrations. For a fine tuning, again the electrostatic theorem and the other above mentioned suggestions could be applied. Theoretical predictions should not be biased by the method of computation. Therefore the dependence of the density analyzing tools on the level of calculation (method of calculation/basis set) and on the substituents in complex chemical bonding situations were evaluated in the second part of the present work. A number of compounds containing formal single and double sulfur nitrogen bonds was investigated. For these compounds, experimental data were also available. The calculated data were compared internally and with the experimental results. The internal comparison was drawn with regard to questions of convergency as well as with regard to questions of consistency: The resulting molecular properties from NBO/NRT analyses were found to be very stable, when the geometries were optimized at the respective level of theory. This stability is valid for variations in the methods of calculation as well as for variations in the basis set. Only the individual resonance weights of the contributing Natural Lewis Structures differed considerably depending on the level of calculation and depending on the substituents. However, the deviations were in both cases to a large extent within a limit which preserves the descending order of the leading resonance structure weights. The resulting bond orders, i.e., the total, covalent and ionic bond order from NRT calculations, were not affected by the shift in the resonance weights. The analysis of the bond topological parameters resulted in a discrimination between insensitive parameters and sensitive parameters. The stable parameters do neither depend strongly on the method of calculation nor on the basis set. Only minor variation occurs in the numerical values of these parameters, when the level of calculation is changed or even when other functional groups (H, Me, or tBu) are employed, as long as the methods of calculation do not drop considerably below a standard level. The bond descriptors of the sulfur nitrogen bonds were found to be also stable with respect to the functional groups R = H, R = Me, and R = tBu. Stable parameters are the bond distance, the density at the bond critical point (BCP) and the ratio of distances between the BCP and the nuclei A and B, which varies clearly when considering the formal bond type. For very small basis sets like the 3-21G basis set, this characteristic stability collapses. The sensitive parameters are based on the second derivatives of the density with respect to the coordinates. This is in accordance with the well known fact, that the total second derivative of the density with respect to the coordinates is a strongly oscillating function with positive as well as negative values. A profound deviation has to be anticipated as a consequence of strong oscillations. lambda3, which describes the local charge depletion in the direction of the interaction line, is the most varying parameter. A detailed analysis revealed that the position of the BCP in the rampant edge of the Laplacian distribution is responsible for the sensitivity of the numerical value of lambda3 in formal double bonds. Since the slope of the Laplacian assumes very high values in its rampant edge, a tiny displacement of the BCP leads already to a considerable change in lambda3. This instability is not a failure of the underlying theory, but it yields de facto to a considerable dependence of sensitive bond topological properties on the method of calculation and on the applied basis sets. Since the total second derivative is important to judge on the nature of the bond in the AIM theory (closed shell interactions versus shared interactions), the changes in lambda3 can lead to differing chemical interpretations. The comparison of theoretically derived bond topological properties of various sulfur nitrogen bonds provides the possibility to measure the self consistency of this data set. All data sets clearly exhibit a linear correlation between the bond distances and the density at the BCP on one hand and between the bond distances and the Laplacian values at the BCP on the other hand. These correlations were almost independent of the basis set size. In this context, the linear regression has to be regarded exclusively as a descriptive statistics tool. There is no correlation anticipated a priori. The formal bond type was found to be readily deducible from the theoretically obtained bond topological descriptors of the model systems. In this sense, the bond topological properties are self consistent despite of the numerical sensitivity of the derivatives, as exemplified above. Often, calculations are performed with the experimentally derived equilibrium geometries and not with optimized ones. Applying this approach, the computationally costly geometry optimizations are saved. Following this approach the bond topological properties were calculated using very flexible basis sets and employing the fixed experimental geometry (which, of course, includes the application of tBu groups). Regression coe±cients similar to those from optimized geometries were obtained for correlations between bond distances and the densities at the BCP as well as for the correlation between bond distances and the Laplacian at the BCP, i.e. the approach is valid. However, the data points scattered less and the coe±cient of correlation was clearly increased when geometry optimizations were performed beforehand. The comparison between data obtained from theory and experiment revealed fundamental discrepancies: In the data set of bond topological parameters from the experiment, the behavior of only 2 out of 3 insensitive parameters was comparable to the behavior of the theoretically obtained values, i.e. theoretical and experimental bond distances as well as theoretical and experimental densities at the BCP correlate. From the theoretically obtained data it was easy to deduce the formal bond type from the position of the BCP, since it changed in a systematic manner. The respective experimentally obtained values were almost constant and did not change systematically. For the SN bonds containing compounds, the total second derivative assumes exclusively negative values in the experiment. Due to the different internal behavior, experimentally and theoretically sensitive bond topological values could not be compared directly. The qualitative agreement in the Laplacian distribution, however, was excellent. In the third and last part of this work, the application to chemical systems follows. Formal hypervalent molecules, i.e. molecules where some atoms are considered to hold more than 8 electrons in their valence shell, were investigated. These were compounds containing sulfur nitrogen bonds (H(NtBu)2SMe, H2C{S(NtBu)2(NHtBu)}2, S(NtBu)2 and S(NtBu)3) and a highly coordinated silicon compound. The set of sulfur nitrogen compounds also contained a textbook example for valence expansion, the sulfur triimide. For these molecules, experimental reference values were available from high resolution X-ray experiments. The experimental results were in the case of the sulfur triimide not unique. Furthermore, from the experimental bond topological data no definite conclusion about the formal bonding type could be drawn. The situation of sulfur nitrogen bonds in the above mentioned set of molecules was analyzed in terms of a geometry discussion and by means of a topological analysis. The methyl-substituted isolated molecules served as model compounds. For the interpretation of the bonding situation additional NBO/NRT calculations were preformed for the sulfur nitrogen compounds and an ELF calculation and analysis was performed for the silicon compound. The ELF analysis included not only the presentation and discussion of the ELF-isosurfaces (eta = 0.85), but also the investigation of populations of disynaptic valence basins and the percentage contributions to these populations of the individual atoms when the disynaptic valence basins are split into atomic contributions according to Bader’s partitioning scheme. The question of chemical interest was whether hypervalency is present in the set of molecules or not. In the first case the octet rule would be violated, in the second case Pauling’s verdict would be violated. While the concept of hypervalency is well established in chemistry, the violation of Pauling’s verdict is not. The quantitative numbers of the sensitive bond topological values from theory and experiment were not comparable, since no systematic relationship between the experimentally and theoretically determined sensitive bond descriptors was found. However, the insensitive parameters are in good agreement and the qualitative Laplacian distribution is, with few exceptions, in excellent agreement. The formal bonding type was deduced from experimental and theoretical topological data by considering the number and shape of valence shell charge concentrations in proximity to the sulfur and nitrogen centers. The results from NBO/NRT calculations confirmed the findings. All employed density analyzing tools AIM, ELF and NBO/NRT coincided in describing the bonding situation in the formally hypervalent molecules as highly polar. A comparison and analysis of experimentally and theoretically derived electron densities led consistently to the result, that regarding this set of molecules, hypervalency has to be excluded unequivocally.
A theory of managed floating
(2003)
After the experience with the currency crises of the 1990s, a broad consensus has emerged among economists that such shocks can only be avoided if countries that decided to maintain unrestricted capital mobility adopt either independently floating exchange rates or very hard pegs (currency boards, dollarisation). As a consequence of this view which has been enshrined in the so-called impossible trinity all intermediate currency regimes are regarded as inherently unstable. As far as the economic theory is concerned, this view has the attractive feature that it not only fits with the logic of traditional open economy macro models, but also that for both corner solutions (independently floating exchange rates with a domestically oriented interest rate policy; hard pegs with a completely exchange rate oriented monetary policy) solid theoretical frameworks have been developed. Above all the IMF statistics seem to confirm that intermediate regimes are indeed less and less fashionable by both industrial countries and emerging market economies. However, in the last few years an anomaly has been detected which seriously challenges this paradigm on exchange rate regimes. In their influential cross-country study, Calvo and Reinhart (2000) have shown that many of those countries which had declared themselves as ‘independent floaters’ in the IMF statistics were charaterised by a pronounced ‘fear of floating’ and were actually heavily reacting to exchange rate movements, either in the form of an interest rate response, or by intervening in foreign exchange markets. The present analysis can be understood as an approach to develop a theoretical framework for this managed floating behaviour that – even though it is widely used in practice – has not attracted very much attention in monetary economics. In particular we would like to fill the gap that has recently been criticised by one of the few ‘middle-ground’ economists, John Williamson, who argued that “managed floating is not a regime with well-defined rules” (Williamson, 2000, p. 47). Our approach is based on a standard open economy macro model typically employed for the analysis of monetary policy strategies. The consequences of independently floating and market determined exchange rates are evaluated in terms of a social welfare function, or, to be more precise, in terms of an intertemporal loss function containing a central bank’s final targets output and inflation. We explicitly model the source of the observable fear of floating by questioning the basic assumption underlying most open economy macro models that the foreign exchange market is an efficient asset market with rational agents. We will show that both policy reactions to the fear of floating (an interest rate response to exchange rate movements which we call indirect managed floating, and sterilised interventions in the foreign exchange markets which we call direct managed floating) can be rationalised if we allow for deviations from the assumption of perfectly functioning foreign exchange markets and if we assume a central bank that takes these deviations into account and behaves so as to reach its final targets. In such a scenario with a high degree of uncertainty about the true model determining the exchange rate, the rationale for indirect managed floating is the monetary policy maker’s quest for a robust interest rate policy rule that performs comparatively well across a range of alternative exchange rate models. We will show, however, that the strategy of indirect managed floating still bears the risk that the central bank’s final targets might be negatively affected by the unpredictability of the true exchange rate behaviour. This is where the second policy measure comes into play. The use of sterilised foreign exchange market interventions to counter movements of market determined exchange rates can be rationalised by a central bank’s effort to lower the risk of missing its final targets if it only has a single instrument at its disposal. We provide a theoretical model-based foundation of a strategy of direct managed floating in which the central bank targets, in addition to a short-term interest rate, the nominal exchange rate. In particular, we develop a rule for the instrument of intervening in the foreign exchange market that is based on the failure of foreign exchange market to guarantee a reliable relationship between the exchange rate and other fundamental variables.
Summary: In the present work, two important negative regulators of T cell responses in rats were examined. At the molecular level, rat CTLA-4, a receptor important for deactivating T cell responses, was examined for the expression pattern and in vitro functions. For this purpose, anti-rat CTLA-4 mAbs were generated. Consistent with the studies in mice and humans, rat CTLA-4 was detectable only in CD25+CD4+ regulatory T cells in unstimulated rats, and was upregulated in all activated T cells. Cross-linking rat CTLA-4 led to the deactivation of anti-TCR- and anti-CD28 stimulated (costimulation) T cell responses such as reduction in activation marker expression, proliferation, and cytokine IL-2 production. Although T cells stimulated with the superagonistic anti-CD28 antibody alone without TCR engagement also increased their CTLA-4 expression, a delayed kinetics of CTLA-4 upregulation was found in cells stimulated in this way. The physiological relevance of this finding needs further investigation. At the cellular level, rat CD25+CD4+ regulatory T cells were examined here in detail. Using rat anti-CTLA-4 mAbs, the phenotype of CD25+CD4+ regulatory T cells was investigated. Identical to the mouse and human Treg phenotype, rat CD25+CD4+ T cells constitutively expressed CTLA-4, were predominantly CD45RC low, and expressed high level of CD62L (L-selectin). CD25+CD4+ cells proliferated poorly and were unable to produce IL-2 upon engagement of the TCR and CD28. Furthermore, rat CD25+CD4+ cells produced high amounts of anti-inflammatory cytokine IL-10 upon stimulation. Importantly, freshly isolated CD25+CD4+ T cells from naïve rats exhibited suppressor activities in the in vitro suppressor assays. In vitro, CD25+CD4+ regulatory T cells proliferated vigorously upon superagonistic anti-CD28 stimulation and became very potent suppressor cells. In vivo, a single injection of CD28 superagonist into rats induced transient accumulation and activation of CD25+CD4+ regulatory T cells. These findings suggest firstly that efficient expansion of CD25+CD4+ cells without losing their suppressive effects (even enhance their suppressive activities) can be achieved with the superagonistic anti- CD28 antibody in vitro. Secondly, the induction of disproportional expansion of CD25+CD4+ cells by a single injection of superagonistic anti-CD28 antibody in vivo implies that superagonistic anti-CD28 antibody may be a promising candidate in treating autoimmune diseases by causing a transient increase of activated CD25+CD4+ T cells and thus tipping ongoing autoimmune responses toward selftolerance.
This study investigates the credit channel in the transmission of monetary policy in Germany by means of a structural analysis of aggregate bank loan data. We base our analysis on a stylized model of the banking firm, which specifies the loan supply decisions of banks in the light of expectations about the future course of monetary policy. Using the model as a guide, we apply a vector error correction model (VECM), in which we identify long-run cointegration relationships that can be interpreted as loan supply and loan demand equations. In this way, the identification problem inherent in reduced form approaches based on aggregate data is explicitly addressed. The short-run dynamics is explored by means of innovation analysis, which displays the reaction of the variables in the system to a monetary policy shock. The main implication of our results is that the credit channel in Germany appears to be effective, as we find that loan supply effects in addition to loan demand effects contribute to the propagation of monetary policy measures.
A CD8+ cell-mediated host defense relies on cognate killing of infected target cells and on local inflammation induced by the secretion of IFN-g. Using assays of single cell resolution, it was studied to what extent these two effector function of CD8+ cells are linked. Granzyme B (GzB) is stored in cytolytic granules of CD8+ cells and its secretion is induced by antigen recognition of these cells. Following entry into the cytosol GzB induces apoptosis in the target cells. It was measured whether GzB release by individual CD8+ cells is accompanied by the secretion of IFN-gƒnƒnand of other cytokines. HIV peptide libraries were tested on bulk peripheral blood mononuclear cells and on purified CD4+ and CD8+ cells obtained from HIV infected individuals. The library included a panel of previously defined HLA class I restricted HIV peptides and an overlapping 20-mer peptide-series that covered the entire gp120 molecule. To characterize the in vivo differentiation state of the T-cells, freshly isolated lymphocytes were tested in assays of 24h duration. The data showed that only ~20% of the peptides triggered the release of both GzB and IFN-g from CD8+ cells. The majority of the HIV peptides induced either GzB or IFN-g, ~40% in each category. The GzB positive, IFN-g negative CD8+ cells did not produce IL-4 or IL-5, which suggests that they do not correspond to Tc2 cells but represent a novel Tc1 subclass, which was termed Tc1c. Also the IFN-g positive, GzB negative CD8+ cell subpopulation represents a yet undefined CD8+ effector cell lineage that was termed Tc1b. Tc1b and Tc1c cells are likely to make different, possibly antagonistic contributions to the control of HIV infection. Since IFN-g activates HIV replication in latently infected macrophages, the secretion of this cytokine by Tc1b cells in the absence of killing may have adverse effects on the host defense. In contrast, cytolysis by Tc1c cells in the absence of IFN-g production might represent the protective class of response. Further studies in the field of Tc1 effector cell diversity should lead to valuable insights for management of infections and developing rationales for vaccine design.
The present investigation report a protocol to obtain dendritic cells (DC) that protects mice against fatal leishmaniasis. DC were generated from bone marrow precursors, pulsed with leishmanial antigen and activated with CpG oligodeoxinucleotides. Mice that were vaccinated with these cells were strongly protected against the clinical and parasitological manifestations of leishmaniasis and developed a Th1 immune response. protection was solid and long-lasting, and was also dependent of the via of administration. Whe the mechanism of protection was studied, it was observed that the availability of the cytokine interleukin-12 at the time of vaccination was a key requirement, but that the source of this cytokine is not the donor cells but unidentified cells from the recipients.
Nowadays, robotics plays an important role in increasing fields of application. There exist many environments or situations where mobile robots instead of human beings are used, since the tasks are too hazardous, uncomfortable, repetitive, or costly for humans to perform. The autonomy and the mobility of the robot are often essential for a good solution of these problems. Thus, such a robot should at least be able to answer the question "Where am I?". This thesis investigates the problem of self-localizing a robot in an indoor environment using range measurements. That is, a robot equipped with a range sensor wakes up inside a building and has to determine its position using only its sensor data and a map of its environment. We examine this problem from an idealizing point of view (reducing it into a pure geometric one) and further investigate a method of Guibas, Motwani, and Raghavan from the field of computational geometry to solving it. Here, so-called visibility skeletons, which can be seen as coarsened representations of visibility polygons, play a decisive role. In the major part of this thesis we analyze the structures and the occurring complexities in the framework of this scheme. It turns out that the main source of complication are so-called overlapping embeddings of skeletons into the map polygon, for which we derive some restrictive visibility constraints. Based on these results we are able to improve one of the occurring complexity bounds in the sense that we can formulate it with respect to the number of reflex vertices instead of the total number of map vertices. This also affects the worst-case bound on the preprocessing complexity of the method. The second part of this thesis compares the previous idealizing assumptions with the properties of real-world environments and discusses the occurring problems. In order to circumvent these problems, we use the concept of distance functions, which model the resemblance between the sensor data and the map, and appropriately adapt the above method to the needs of realistic scenarios. In particular, we introduce a distance function, namely the polar coordinate metric, which seems to be well suited to the localization problem. Finally, we present the RoLoPro software where most of the discussed algorithms are implemented (including the polar coordinate metric).
The present work consists of two parts. The first one deals with theoretical questions and tests the performance of orbitals obtained from a self-interaction free KS method, the LHFapproach, in multireference ab initio methods. The purpose of this part is to enable a more efficient computation of excitation energies, which is important for the spectroscopic characterization of many organic and bioorganic molecules. The second part focuses on bioorganic questions and studies the base pairing properties of the purine base xanthine in order to explain, e.g., the unusually high stability of selfpairing xanthine alanyl-PNA double strands and the mutagenicity of xanthine formed in DNA. Part1: In contrast to HF- and standard DFT-methods, the LHF-approach leads to a fully bound virtual orbital spectrum, because Coulomb self interactions are exactly canceled in the LHFansatz. Furthermore, the energies of the occupied orbitals are not upshifted, like it is the case for standard DFT-methods, so that Koopmans' theorem remains valid. In line with this, also the occupied LHF-orbitals are somewhat more compact than standard DFT-orbitals. The present work shows that both properties are of great benefit for MR methods. The virtual LHF-orbitals are well optimized and allow an efficient description of excited states and static correlation in both MRCI- and MRPT2-approaches. Furthermore, the higher compactness of the occupied LHF- compared to standard DFT-orbitals leads to a better description of the center ion of Rydberg states. However, for each of the two advantages mentioned at least one example molecule has been found, for which LHF-orbitals actually perform worse than HF-and/or standard DFT-orbitals. This shows, that even though LHF virtual orbitals allow an excellent MRCI- and MRPT2-description for the electronically excited states of a large number of molecules, this cannot be generalized and their performance needs to be tested for each individual case. In the second part of the present work, the base pairing properties of xanthine and xanthine derivatives were studied. The purpose of this part was to find an explanation for the unexpectedly high stability of the xanthine alanyl PNA double strand. Furthermore, it was analyzed, why xanthine, that is formed from guanine in DNA under chemical stress, is able to form mismatched base pairs with the pyrimidine base thymine. Stability of xanthine alanyl PNA: In the first step, the regioisomer present in the considered alanyl PNA was identified to be the N7-regioisomer of xanthine by a theoretical analysis of the 13C-NMR spectrum. To analyze the stability of the xanthine self-pairing, a simplified model was set up, in which the stability of the PNA double strand was explained solely by the energy contributions from H-bonding and base stacking. For that purpose, the dimerization and stacking energies for the xanthine-xanthine, guaninecytosine, adenine-thymine and xanthine-2,6-diaminopurine base pairs were computed using DFT and MP2 methods. Solvent effects were taken into account by the conductor like screening model. The influence of the peptide backbone on the stacking geometry was considered by force field optimizations. While the individual contributions from hydrogen bonding and stacking do not correlate with the melting temperature Tm, the sum of both correlates linearly with Tm. This correlation is somewhat surprising, because this means that the effects of the entropy and the molecular water environment either cancel or are similar for all systems compared. In this model, the stability of the xanthine selfpairing mainly stems from an enlarged stacking interaction, while the H-bonds give only minor contributions to the stability of the xanthine selfpaired double strand of alanyl-PNA. Base pairing properties of N9-Xanthine: The computation of the base pairing properties of N9-xanthine revealed a strong variation in the individual H-bond strengths for the selfpairing of xanthine, that range from -4 to -11 kcal/mol in the gas phase and -2.5 to -5 kcal/mol in polar solvent. By comparison with model systems it was shown that the strong variance of the H-bond strength is mainly due to attractive or repulsive secondary electrostatic interactions. For the homodimer of hypoxanthine it was shown that the increase of aromaticity in the pyrimidine ring upon dimer formation leads to a strengthening of the hydrogen bonds. Mutagenicity of hypoxanthine and xanthine: Several neutral and anionic Watson-Crick base pairs of xanthine were computed with MP2- and DFT-methods in order to explain the mutagenicity of hypoxanthine and xanthine. Also basepairs involving tautomeric forms of xanthine and hypoxanthine were considered. To evaluate the dimerization energies found, the dimers were classified into pairings that have the exact geometry of the canonical base pairs and those that realize a distorted Watson-Crick pairing mode. The computations show that a stable pairing which realizes the exact geometry of a canonical Watson Crick base pairing is only possible for the pairing of xanthine to cytosine, however, the base pairs are only weakly bound. The dimerization energies of both the neutral and the anionic pairing is around 0 kcal/mol, so that the xanthine-cytosine base pairs are incorporated into DNA solely because the base pairs fulfill the geometric demands of DNA polymerase, but it does not profit from any additional stabilization due to hydrogen bonding. The bonding that in the Watson-Crick pairing mode xanthine has almost no affinity to cytosine is in correspondence with the experimental result that the cytosine-xanthine base pair is incorporated into DNA at a much lower rate than the cytosine-guanine base pair, which has a very strong hydrogen bonding. While the affinity of xanthine to cytosine is very low, the computations predict that xanthine is able to form a stable Watson-Crick pairing with thymine. However, the pairing has a somewhat distorted Watson-Crick geometry, so that its high stability is outbalanced by the worsened fit to the binding pocket of DNA-polymerase. As a consequence, the xanthinethymine pairing is incorporated into DNA not at a faster, but only at a rate comparable to that of the xanthine-cytosine pairing.
The aim of current work was contribution to the long-term ongoing project on developing human IL-5 agonists/antagonists that intervene with or inhibit IL-5 numerous functions in cell culture and/or in animal disease models. To facilitate design of an IL-5 antagonist variant or low-molecular weight mimetics only capable of binding to the specific receptor alpha chain, but would lack the ability to attract the receptor common β-chain and thus initiate receptor complex activation it is necessary to gain the information on minimal structural and functional epitopes. Such a strategy was successfully adopted in our group on example of Interleukin 4. To precisely localize minimal structural epitope it is essential to have structure of the ligand in its bound form and especially informative would be structure of complex of the ligand and its specific receptor alpha chain. For this purpose large quantities (tens of milligrams), retaining full biological activity IL-5 and extracellular domain of IL-5 specific receptor α-chain were expressed in a bacterial expression system (E.coli). After successful refolding proteins were purified to 95-99% Stable and soluble receptor:ligand complex was prepared. Each established purification and refolding procedures were subjected to optimization targeting maximal yields and purity. Produced receptor:ligand complex was applied to crystallization experiments. Microcrystals were initially obtained with a flexible sparse matrix screening methodology. Crystal quality was subsequently improved by fine-tuning of the crystallization conditions. At this stage crystals of about 800x150x30µm in size can be obtained. They possess desirable visible characteristics of crystals including optical clarity, smooth facecs and sharp edges. Crystals rotate plane polarized light reflecting their well internal organization. Unfortunately relative slimness and sometimes cluster nature of the produced crystals complicates acquisition of high-resolution dataset and resolution of the structure. With some of obtained crystals diffraction to a resolution up to 4Å was observed.
The Middle and Upper Jurassic sedimentary successions of Alborz in northern Iran and Koppeh Dagh in northeastern Iran comprise four formations; Dalichai, Lar (Alborz) and Chaman Bid, Mozduran (Koppeh Dagh). In this thesis, the biostratigraphy, lithostratigraphy, microfacies, depositional environments and palaeobiogeography of these rocks are discussed with special emphasis on the abundant ammonite fauna. They constitute a more or less continuous sequence, being confined by two tectonic events, one at the base, in the uppermost part of the Shemshak Formation (Bajocian), the so-called Mid-Cimmerian Event, the other one at the top (early Cretaceous), the so-called Late-Cimmerian Event. The lowermost unit constitutes the uppermost member of a siliciclastic and partly continental depositional sequence known as Shemshak Formation. It contains a fairly abundant ammonite fauna ranging in age from Aalenian to early Bajocian. The following unit (Dalichai Formation) begins everywhere with a significant marine transgression of late Bajocian age. The following four sections were measured: The Dalichai section (97 m) with three members; the Golbini-Jorbat composite section (449 m) with three members of the Dalichai Formation (414 m) and two members of the Lar Formation (414 m); the Chaman Bid section (1556 m) with seven members, and the Tooy-Takhtehbashgheh composite section (567 m) with three members of the Chaman Bid Formation (567 m) and four members of the Mozduran Formation (1092 m). Altogether, 80 species of ammonites from the Dalichai and Chaman Bid formations belonging to 30 genera and 16 families are described. Among the taxa Phylloceratidae are most abundant, followed by Ataxioceratidae, Perisphinctidae, and Cardioceratidae. Pachyceratidae are the least common family. The ammonite fauna is of low diversity and is concentrated in several levels. Some of the ammonite genera and species are recorded from Iran for the first time. These include Pachyceras lalandei, Cardioceras praecordatum, Microbajocisphinctes sp., Geyssantia geyssanti, Larcheria schilli, Passendorferia sp., Sequeirosia sp., Phanerostephanus subsenex, Nothostephanus sp., Nannostephanus cf. subcomutus, Parawedekindia callomoni, Physodoceras sp., Extrenodites sp.. Biostratigraphically, thirty ammonite zones have been recognized for the Middle and Upper Jurassic successions at the four studied sections. Based on ammonites, the Dalichai Formation ranges from the Upper Bajocian to Callovian (Dalichai section) and from the Upper Bajocian to Lower Tithonian (Golbini-Jorbat section), the Chaman Bid Formation ranges from the ?Bathonian to Lower Tithonian (Chaman Bid section) and from the Upper Bajocian to Middle Kimmeridgian (Tooy-Takhtehbashgheh section), the Lar Formation ranges from the Middle to Upper Tithonian (Golbini-Jorbat section), and the Mozduran Formation from the Upper Kimmeridgian to ?Tithonian. Forty-four Microfacies types are briefly described. They were grouped into 16 facies associations, which then were interpreted in terms of their palaeoenvironments. They are part of a carbonate system consisting of a platform and adjacent slope to basin. Five major environments are represented: Tidal flat, shelf lagoon, and platform margin barrier as parts of the carbonate platform, and slope to basin representing open marine conditions. The sediments of the Dalichai and Chaman Bid formations are the slope and basinal sediments of the diachronous Lar and Mozduran formations, which formed an extensive carbonate platform in the Middle and Upper Jurassic.
The first part of this work focuses on the characterization of systems which complex electronic structures require the application of multi-reference methods. The anti-tumor efficacy of the natural product Neocarzinostatin is based on the formation of diradicals and causes DNA cleavage and finally cytolysis. Computations on model systems performed in the present work show the influence of structural features on the mode of action and the efficacy of this antitumor-antibiotic. The cyclization of systems related to the enyne-cumulene framework like the enyne-allenes was investigated earlier and relations to the more unusual class of enyne-ketenes are analyzed. The class of enyne-ketenes (and also the enyne-allenes) show a broad spectrum of possible intermediates (diradicals, zwitterions, allenes). The electronic structures of these intermediates are also possible for the (heteroatom substituted) 1,2,4-cyclohexatriene and a model for their energetic sequence based on high-level multi-reference computations is proposed. In all three projects the application of multi-reference approaches is necessary to obtain a comprehensive picture of the reactivity and electronic structure but also shows up the limits inherently existing in the currently available programs with respect to the size of the molecules. In the second part, algorithms for a multi-reference Moller-Plesset perturbation theory (MR-MP2) program, designed to perform large-scale computations, were developed and implemented. The MR-MP2 approach represents the most cost-effective multireference ansatz and requires an efficient evaluation of the Hamilton matrix for which an algorithm is designed to instantly recognize only non-vanishing matrix elements and to employ the recurring interaction patterns of the Hamilton matrix. The direct construction of the Hamilton matrix is additionally parallelized to work on cluster environments.
The main aim of this work was the classification of highly polar E–N (E = Al, Si, P) and Li–E’ (E’ = C, N, O) bonds in terms of ionic (closed-shell) or covalent (shared) interactions. To answer this question the experimentally determined electron density was analyzed using Bader’s theory of ‘Atoms in Molecules’ (AIM). This allows a quantitative evaluation of properties derived from the electron density, such as the Laplacian, the ellipticitiy and the ratio of the highest charge concentration perpendicular to the bond path, to the largest charge depletion along the bonding vector. Most of these properties were monitored along the entire bonding region and not limited to the BCP as in former studies. The analyses are completed by the calculation of the electronic energy densities Hl at the BCPs and the integration of atomic basins also defined within the AIM theory. The electrostatic potential (ESP) was computed from the multipole parameters to reveal preferred reactive sites of the structures under investigation. Apart from that, the multipole formalism was applied to problematic crystal structures in order to open this method for twinned samples or those including disordered groups in the molecule.
Synthesis of (RS)-5-amino-3-aryl (methyl)-pentanoic acid hydrochlorides, 3 aminomethyl-5-chloro-benzoic acid hydrochloride and (RS)-4-amino-3-(4`-ethynyl(iodo)-phenyl)-butanoic acid hydrochlorides have been accomplished. The aim of their synthesis was to evaluate their GABABR agonist activity and to derive a model which will correlate their structure with the observed pEC50. The GABABR agonist activity of the prepared compounds has been determined in functional assay based on calcium measurement in vitro using tsA cells transfected with GABAB1b/GABAB2/Gαq-z5. Reviews on the neurotransmitter receptors (ligand-gated ion channel receptors and G protein-coupled receptors), their agonists and antagonists have been given in the general part of this work. A detailed discussion on the strategy followed for the synthesis of the designed compounds as well as the starting materials and intermediates has been described and illustrated in Schemes 2-6. The synthesized compounds were evaluated for their GABABR agonist activity. Furthermore, these compounds were docked in the available 3D homology model of GABABR using the program FlexiDock implemented in SYBYL software. Subsequently, we derived a predictive model which correlates the experimentally determined pEC50 with the calculated binding energy of certain baclofen analogues and homologues. In addition, we used the program DISCO (DIStance COmparisons) implemented in SYBYL software to find the pharmacophore features of GABAB agonists.
In the last years it became evident that many cytokines do not only bind to their specific cell surface receptors but also interact with components of the extracellular matrix. Mainly in Drosophila, several enzymes were identified, that are involved in glycosaminoglycan synthesis. Mutations in these enzymes mostly result in disturbances of several signaling pathways like hedgehog, wingless, FGF or dpp. In most cases it was, due to these pleiotropic effects, not possible to examine the relevance of matrix interactions for single pathways. The aim of this work was to examine the relevance of matrix interactions for the TGF-ß superfamily member DPP. Based on the fact that DPP is highly homologous to human BMP-2, the basic N-terminus of mature DPP was mutated, which has been shown to contain a heparin-binding site in BMP-2. Thus, a wildtype variant (D-MYC), a deletion variant (D-DEL), which lacked the whole basic part of the N-terminus and a duplication variant (D-DUP), which contained a second copy of the basic core moitiv, were generated. In order to characterise the variants biochemically, they were expressed in E.coli and refolded in a bioactive form. In chicken limbbud assay, the deletion variant was much more active than the wildtype variant, comparable to data of BMP-2. By means of biacore mesurements with the immobilised ectodomain of the high affinity type I receptor thick veins, it could be demonstrated, that the variants differ only in matrix binding and not in their receptor affinity. Different matrix binding was shown by Heparin FPLC. The biological relevance of the matrix interaction of DPP was examined in transgenic flies. To allow expression of the different variants under the control of various Gal4 driver lines, they were cloned behind an UAS-promoter site. In early tracheal development, a strong dependence of DPP signaling on matrix binding was observed. While ectopic expression of the deletion variant caused only minor defects, the branching pattern was strongly disturbed by overexpression of wildtype and duplication variant. Ubiquitous expression of the variants in the wing imaginal disc caused overproliferation of the disc and expansion of the omb target gene expression. The extent of phenotypes correlated with the matrix binding ability of the variants. Corresponding disturbances of the wing vein pattern was observed in adult flies. By the crossing of different dpp allels, transheterozygous animals were created, that lack dpp only in imaginal discs. Expression of the variants under the control of a suitable dpp-Gal4 driver line revealed insights into the biological relevance of matrix binding on DPP gradient formation and specific target gene activation in wing imaginal discs. It was shown, that all variants were able to generate a functional DPP gradient with correct expression of the target genes omb and spalt. Again a correlation between extent of target gene domains and matrix binding ability of the corresponding variants was found. Thus by mutating the N-terminus of DPP, it could be shown that this is responsible for DPP`s matrix interaction. Also the relevance of matrix binding of DPP in different tissues was examined. It turned out, that the reorganisation of tracheal branching by DPP strongly depends on matrix interactions wheras the establishing of a gradient in wing imaginal discs depends only gradually on matrix interactions. Based on these data a model for the action of DPP/TGFßs as morphogens was established. While a deletion of matrix binding leads to a decrease in specific bioactivity of the cytokine, the latter is increased by additional matrix binding sites.
The human retina is a multilayered neuroectodermal tissue specialized in the transformation of light energy into electric impulses which can be transmitted to the brain where they are perceived as vision. Since the retina is easily accessible and functional aspects are directly recordable, the study of this tissue has been at the forefront of neuroscience research for over a century. Studies have revealed that the distinct functions of the retina require a large degree of differentiation which is achieved by the coordinated function of approximately 55 different cell types. The highly structured anatomy and the functional differentiation of the retina is a result of its distinctive transcriptome and proteome. Due to the complexity of the retina it has been difficult to estimate the number of genes actively transcribed in this tissue. Great efforts in the elucidation of retinal disease genes have led to the identification of 139 retina disease loci with 90 of the corresponding genes cloned thus far . In contrast to the success in the hereditary disorders, efforts to identify the genetic factors conferring manifestations known as age-related macular degeneration (AMD) have revealed sparse results. AMD is a retinal disease affecting a significant percentage of the older population. This disorder is likely due to exogenic as well as genetic factors. To further our understanding of retinal physiology and facilitate the identification of genes underlying retinal degenerations, particularly AMD, our efforts concentrated on the systematic analysis of the retinal transcriptome. Since approximately half of all retinal degeneration-associated genes identified to date are preferentially expressed in retina, it is plausible that the investigation of gene expression profiles and the identification of retina-expressed transcripts could be an important starting point for characterizing candidate genes for the retinal diseases. The expressed sequence tags approach included the assessment of all retinal expressed sequence tags (EST) clusters indexed in the UniGene database and of 1080 single-pass ESTs derived from an in-house generated human retina suppression subtracted hybridization (SSH) cDNA library. In total, 6603 EST clusters were evaluated during this thesis and detailed in-silico analysis was performed on 750 EST clusters. The expression of the genes was evaluated using reverse transcriptase-polymerase chain reaction (RT-PCR), followed by confirmation using quantitative reverse transcriptase-polymerase chain reaction (qRT-PCR), as well as conventional and virtual Northern blot analysis. The expression profiling of 337 selected EST clusters led to the identification of 111 transcripts, of which 60 are specific or abundant to the retina, 3 are expressed at high levels in the retinal pigment epithelium (RPE), and 48 are expressed in brain as well as in retina. The EST approach used to select candidate transcripts allowed us to assess the effectiveness of the two available resources, the UniGene database and the retinal SSH (retSSH) cDNA library. From the results obtained, it is evident that the generation of suppression subtracted libraries to identify cell-specific transcripts constitutes the most straight-forward and efficient strategy. In addition to the high percentage of candidate genes that are identified from an SSH cDNA library, it has the added benefit that genes expressed at low levels can be identified. Furthermore, comparison of our retina-enriched gene set with previously published studies demonstrated only limited overlap of the identified genes further confirming the valuable source of retinal genes from our retinal SSH cDNA library. The effort of our and other groups has resulted in the establishment of the full-length coding sequence of 55 of the 111 genes uniquely or preferentially expressed in the retina. Using various methods such as bioinformatical analysis, EST assembly, cDNA library screening, and rapid amplification of cDNA ends (RACE) a number of genes were cloned in the scope of this thesis including C1orf32, C4orf11, C7orf9, C12orf7, C14orf29, DAPL1, and GRM7. Bioinformatic analyses and cDNA library screening were used to isolate the full-length cDNA sequence and determine the genomic organization of C7orf9, also identified as RFRP. This 1190 bp retina-specific transcript from chromosome 7p15.3 encodes a precursor protein for at least two small neuropeptides, referred to as RFRP-1 and RFRP-3. Since C7orf9 is localized in the critical region for dominant cystoid macular dystrophy (CYMD) its role in the pathology was investigated. Southern blot analysis and sequencing of samples from two affected individuals of the original pedigree used to localize the disease gene excluded the gene from involvement in this disease. Multiple isoforms of the C12orf7 gene were assembled from a number of clones identified from library screenings, PCR amplifications, and RACE experiments. The gene variants, transcribed from chromosome 12q13.13, have been found to be expressed exclusively in retina. Because of the multiple alternative splicing of the gene, we can only speculate about the nature of the protein it encodes. The longest transcript, which includes all six exons plus the last intervening sequence, encodes a 471 aa protein which contains a nuclear localization signal and five ankyrin repeats. The existence of many isoforms is also observed in mouse suggesting that they may have a relevant role in cellular physiology. Five novel splice variants of the glutamate metabotropic receptor 7 (GRM7) resulting from the use of alternative 3’-end exons were identified and characterized. One of the novel variants, GRM7_v3, encodes a 924 aa protein and is therefore the longest putative GRM7 protein reported to date. Even though they are not retina-specific, the isoforms are preferentially expressed in the nervous system. Although the functional properties of the specific carboxyl-termini are still unclear, it is known that axon targeting of GRM7_v1 is mediated by the last 60 aa of the protein. Hence the novel isoforms may direct the protein to specific subcellular localizations. The C1orf32 gene, preferentially expressed in retina, is organized in 10 exons and is transcribed from chromosome 1q24.1. Bioinformatic analyses of the 639 aa putative protein not only identified the mouse and rat orthologous genes but also the LISCH7 gene as a potential member of the same family. Since the LISCH7 protein has been shown to function as a low density lipoprotein receptor, the C1orf32 protein may be involved in retinal lipid homeostasis. Disturbances in lipid metabolism have been proposed as one of the pathways involved in AMD etiology. Thus, the role of C1orf32 in this complex disease should be investigated. Expression analyses of the death-associated protein-like 1 (DAPL1) gene revealed that it is expressed in both the retina and the RPE at high levels. The 552 bp transcript encodes a 107 aa putative protein and is transcribed from chromosome 2q24.1. In-silico analyses identified an additional 12 related proteins from various species which share high similarity constituting a novel protein family. The similarity to the death-associated-protein (DAP) is particularly interesting since this protein has been found to be indispensable for programmed cell death. Therefore, DAPL1 is an excellent candidate for retinal disease as apoptosis is generally the ultimate cause in retinal degeneration. The retina-specific C4orf11 and C14orf29 genes localized on chromosome 4q21.22 and 14q22.1, respectively, are both transcribed in more than one isoform. The encoded proteins do not contain any known domains but because of their retina-specific expression they may be important for proper retinal physiology. As part of the long-term goals of the project, several of the cloned genes are being genotyped to construct single nucleotide polymorphism (SNP) maps. Projects to investigate haplotype frequencies of candidate genes in large cohorts of controls and AMD patients are ongoing. Thus, by establishing a collection of 111 genes expressed exclusively or preferentially in the retina, the present work has laid the foundation for future research in retinal diseases.
Density arrested AKR-2B cells die rapidly in response to serum starvation or treatment by Anisomycin. Cell death is associated with typical hallmarks of apoptosis including membrane blebbing and chromatin condensation but lacks energy dissipation in mitochondria and intranucleosomal fragmentation. During apoptosis a considerable DEVDase activity has been detected which seemed to be represented by a single enzyme. This enzyme had typical effector caspase characteristics, like caspase-3, but exhibited an unusual high KM values of ~100 µM and its large subunit exhibited a molecular weight of 19 kDa, instead of expected 17 kDa. In the present study, this enzyme was identified to be caspase-3 with the help of the generation of recombinant mcaspase-3 protein. N-terminal sequencing of the recombinant mcaspase-3 protein revealed that its prodomain cleavage site differs from that in the human homologue (Asp-9 instead of Asp-28). Thus the large subunit of active caspase-3 was found to be 19 kDa. Furthermore the KM value of recombinant mcaspase-3 was ~100 µM in perfect agreement with that found in cell extracts. Affinity labeling in combination with 2D-GE confirmed that indeed caspase-3 is activated as the main executioner in AKR-2B cells during apoptosis. Since the receptor mediated pathway has already been excluded previously [129], a possible involvement of mitochondria mediated pathway in the activation of caspase-3 was examined. Gel filtration experiments revealed that caspase-3 is mainly eluted as free enzyme and in lower levels within the differently sized high molecular weight complexes of ~600 kDa and 250 kDa in response to serum starvation or Anisomycin treatment. Though the apparent molecular weight of the complexes containing caspase-3 are in accordance with recently published data, they were devoid of Apaf-1 and caspase-9. Apparently, mitochondria mediated pathway is also not involved since neither formation of high molecular weight complexes of Apaf-1 nor cleavage of caspase-9 was observed. Thus, the activation of caspase-3 is caused by a noncanonical pathway during apoptosis. In addition a new 450 kDa complex containing activated caspase-6 was found in response to serum starvation which is clearly separated from caspase-3 containing complexes. Generally caspase-3 has been found to be responsible for most of the morphological changes during apoptosis. One of those is intranucleosomal fragmentation. Although caspase-3 was found to be the main executioner caspase in AKR-2B cells the lack of the intranucleosomal fragmentation led to examine its localization. As detected by overexpression of the Caspase-3-GFP fusion construct in AKR-2B, procaspase-3 was localized in the cytoplasm, wheras the active caspase-3 was mainly found in the membrane blebs and partially in the cytoplasm. Clearly no nuclear localization of active caspase-3 was detected. These data gave first hints on the mechanism of degradation of AKR-2B cells demonstrating that cytoplasmic membrane is the primary site of activation of caspase-3. The possible role of caspase-12 and ER stress mediated pathway of apoptosis was also examined in AKR-2B cells. Kinetic studies showed that caspase-12 is activated at the same time together with caspase-3 in response to serum starvation or Anisomycin treatment resulting in two cleavage products of 47 kDa and 35 kDa, respectively. It was therefore examined whether these two caspases were eluted in the same complexes. Gel filtration experiments revealed that caspase-12 is released as free enzyme during apoptosis. To date all the studies have identified that caspase-12 is specifically activated in response to ER stress. After serum starvation or Anisomycin addition there was no increase of the protein expression level of the chaperone protein Grp 78 which is known to be higly elevated in response to ER stress indicating that both treatments did not lead to ER stress. In contrast treatment with ER stressor substances i.e. Thapsigargin, A23187 (ionophore) induced an ER stress in AKR-2B which lead to unspecifically degradation of caspase-12. Thus it is unlikely that caspase-12 is activated in response to ER stress in AKR-2B cells. However, after the in vitro addition of recombinant caspase-3 to cytosolic extracts caspase-12 is cleaved into 47 kDa and 35 kDa fragments similiar to those observed in vivo. In conclusion the present data demostrated that caspase-12 is activated in AKR-2B cells during apoptosis triggered through pathways that do not involve (the) ER stress and provided evidence that caspase-3 might be involved in activation of caspase-12. Thus the present study in AKR-2B cells gives hints for the existence of additional pathways for apoptosis other than the classical ones.
In the current work, several well-known pharmaceuticals (1,4-dihydrazinophthalazine sulfate, caffeine, and papaverine hydrochloride) and new organometallic compounds (nickel(II) cupferronato complexes NiL2An, L = PhN2O2-, n = 1, A = o-phenanthroline (1), o,o’-bipyridine (2) and n = 2, A = H2O (3), o-NH2Py (4), o-C6H4(NH2)2 (5); silylene-bridged dinuclear iron complexes [Cp(OC)2Fe]2SiX2 (X = H (6), F (7), Cl (8), Br (9), I (10)); 3-silaoxetane 3,3-dimethyl-2,2,4,4-tetraphenyl-1-oxa-3-silacyclobutane (11) and 3-silathietane 3,3-dimethyl-2,2,4,4-tetraphenyl-1-sila-3-thiacyclobutane (12) compounds), which have successfully been characterized by using vibrational spectroscopy in conjunction with accurate density functional theory (DFT) calculations, are presented. The DFT computed molecular geometries of the species of interest reproduced the crystal structure data very well and in conjunction with IR and Raman measurements helped us to clarify the structures of the compounds, for which no experimental data were available; and this, especially for the new organometallic compounds, where the X-Ray analysis was limited by the non-availability of single crystals (3, 5, 10). Furthermore, a natural population analysis (NPA) and natural bond orbital (NBO) calculations together with a detailed analysis of the IR and Raman experimental as well as calculated spectra of the new organometallic compounds, allowed us to study some special bonding situations (1-12) or to monitor the structural changes observed with the change in temperature during the Raman experiments (11, 12). By combining these two methods (DFT and vibrational spectroscopy), the auspicious results obtained on the organometallic compounds 6-12 and overall in literature, made us confident of the power of theoretical calculations in aiding the interpretation of rich SERS spectra by solving some interesting issues. Consequently, the Raman and SERS spectra of well-known pharmaceuticals (1,4-dihydrazinophthalazine sulfate, caffeine, and papaverine hydrochloride) or new potentially biological active organometallic complexes (1-5), that were synthetized by our coworkers, were discussed with the assistance of the accurate results obtained from DFT calculations (structural parameters, harmonic vibrational wavenumbers, Raman scattering activities), and many previous incomplete assignments have been analyzed and improved. This allowed us to establish the vibrational behavior of these biological compounds near a biological artificial model at different pH values or concentrations (Ag substrate), taking into account that information about the species present under particular conditions could be of great importance for the interpretation of biochemical processes. The total electron density of molecules and the partial charges situated on selected atoms, which were determined theoretically by NPA, allowed us to establish the probability of different atoms acting as an adsorptive site for the metal surface. Moreover, a closer examination of the calculated orbitals of molecules brought further arguments on the presence or absence of the photoproducts at the Ag surface during the irradiation (1,4-dihydrazinophthalazine sulfate). Overall, the results provide a benchmark illustration of the virtues of DFT in aiding the interpretation of rich vibrational spectra attainable for larger polyatomic adsorbates by using SERS, as well as in furnishing detailed insight into the relation between the vibrational properties and the nature of the Ag substrate-adsorbate bonding. Therefore, we strongly believe that theoretical calculations will become a matter of rapidly growing scientific and practical interest in SERS.
During the Mesoproterozoic large volumes of magma were repeatedly emplaced within the basement of NW Namibia. Magmatic activity started with the intrusion of the anorthositic rocks of the Kunene Intrusive Complex (KIC) at 1,385-1,347 Ma. At its south-eastern margin the KIC was invaded by syenite dykes (1,380-1,340 Ma) and younger carbonatites (1,140-1,120 Ma) along ENE and SE trending faults. Older ferrocarbonatite intrusions, the ‘carbonatitic breccia’, frequently contain wallrock fragments, whereas subordinate ferrocarbonatite veins are almost xenolith-free. Metasomatic interaction between carbonatite-derived fluids and the neighbouring and incorporated anorthosites led to the formation of economically important sodalite deposits. Investigated anorthosite samples display the magmatic mineral assemblage of Pl (An37-75) ± Ol ± Opx ± Cpx + Ilm + Mag + Ap ± Zrn. Ilmenite and pyroxene are surrounded by narrow reaction rims of biotite and pargasite. During the subsolidus stage sporadic coronitic garnet-orthopyroxene-quartz assemblages were produced. Thermobarometry studies on amphiboles yield temperatures of 985-950°C whereas the chemical composition of coronitic garnet and orthopyroxene indicate a subsolidus re-equilibration of the KIC at conditions of 760 ± 100°C and 7.3 ± 1 kbar. In the syenites Kfs, Pl, Hbl and/or Cpx crystallized first, followed by a second generation of Kfs, Hbl, Fe-Ti oxides and Ttn. Crystallization of potassium feldspar occurred under temperatures of 890-790°C. For the crystallization of hastingsite pressures of 6.5 ± 0.6 kbar are obtained. In order to constrain the source rocks of the two suites, oxygen isotope analyses of feldspar as well as geochemical bulk rock analyses were carried out. In case of the anorthosites, the general geochemical characteristics are in excellent agreement with their derivation from fractionated basaltic liquids, with the d18O values (5.88 ± 0.19 ‰) proving their derivation from mantle-derived magmas. The results obtained for the felsic suite, provide evidence against consanguinity of the anorthosites and the syenites, i.e. (1) compositional gaps between the geochemical data of the two suites, (2) trace element data of the felsic suite points to a mixed crustal-mantle source, (3) syenites do not exhibit ubiquitous negative Eu-anomalies in their REE patterns, which would be expected from fractionation products of melts that previously formed plagioclase cumulates and (4) feldspar d18O values from the syenites fall in a range of 7.20-7.92 ‰, which, however, is about 1.6 ‰ higher than the average d18O of the anorthosites. Conformably, the crustal-derived felsic and the mantle-derived anorthositic suite are suggested to be coeval but not consanguineous. Their spatial and temporal association can be accounted for, if the heat necessary for crustal melting is provided by the upwelling and emplacement of mantle-derived melts, parental to the anorthosites. In order to constrain the source of the 1,140-1,120 Ma carbonatites and to elucidate the fenitizing processes, which led to the formation of the sodalite, detailed mineralogical and geochemical investigations, stable isotope (C,O,S) analyses and fluid inclusion measurements (microthermometrical studies and synchrotron-micro-XRF analyses) have been combined. There is striking evidence that carbonatites of both generations are magmatic in origin. They occur as dykes with cross-cutting relationships and margins disturbed by fenitic aureoles, and contain abundant flow-oriented xenoliths. The mineral assemblage of both carbonatite generations of Ank + Cal + Ilm + Mag + Bt ± Ap ± pyrochlore ± sulphides in the main carbonatite body and Ank + Cal + Mag ± pyrochlore ± rutile in the ferrocarbonatite veins, their geochemical characteristics and the O and C isotope values of ankerite (8.91 to 9.73 and –6.73 to –6.98, respectively) again indicate igneous derivation, with the 18O values suggesting minor subsolidus alteration. NaCl-rich fluids, released from the carbonatite melt mainly caused the fenitization of both, the incorporated and the bordering anorthosite. This process is characterized by the progressive transformation of Ca-rich plagioclase into albite and sodalite. Applying conventional geothermobarometry combined with fluid-inclusion isochore data, it was possible to reconstruct the P-T conditions for the carbonatite emplacement and crystallization (1200-630°C, 4-5 kbar) and for several mineral-forming processes during metasomatism (e.g. formation of sodalite: 800-530°C). The composition and evolutionary trends of the fenitizing solution were estimated from both the sequence of metasomatic reactions within wallrock xenoliths in the carbonatitic breccia and fluid inclusion data. The fenitizing solutions responsible for the transformation of albite into sodalite can be characterised as of NaCl-rich aqueous brines (19-30 wt.% NaCl eq.), that contained only minor amounts of Sr, Ba, Fe, Nb, and LREE.
Age related macular degeneration (AMD) is the leading cause of visual impairment in the elderly and the major cause of blindness in the developed world. To date, the molecular mechanisms underlying the disease are not well understood although in recent years a primary involvement of the retinal pigment epithelium (RPE) has become evident. The aim of the present study is to systematically analyse genes which are differentially expressed in the RPE, and to assess their possible association with mechanisms and pathways likely to be related to retinal disease, in particular AMD. Towards this goal, 2379 expressed sequence tags (ESTs) were established from an inhouse generated RPE cDNA library. This library was constructed by using the suppression subtraction hybridization (SSH) technique which normalises redundant sequences and ensures enrichment of rare transcripts. In a first phase, 1002 ESTs were sequenced and subjected to comprehensive alignment with public nucleotide and protein databases. A search of the 1002 ESTs against the human genome draft sequence yielded 168 known genes, 51 predicted genes, 15 unknown transcripts and 41 clones with no significant similarity. Reverse Northern blot hybridization was performed for 318 EST clusters to identify abundantly expressed genes in the RPE and to prioritize subsequent analyses. Representative clones were spotted onto a nylon membrane and hybridized with cDNA probes of driver (heart and liver) and tester (RPE) used in the cDNA library construction. Subsequently, 107 EST clusters were subjected to Northern blot hybridizations. These analyses identified 7 RPE-specific, 3 retina-specific, 7 RPE/retina-specific, and 7 tissue restricted transcripts, while 29 EST clusters were ubiquitously expressed, and evaluation was not possible for another 54 EST clusters. Of the 24 transcripts with specific or restricted expression, 16 clones were selected for further characterization. The predicted gene MGC2477 and 2 novel isoforms of the human transient receptor potential cation channel, subfamily M, member 3 (TRPM3) were cloned and further described in detail. In addition, polymorphic variations for these 2 genes as well as for the human MT-Protocadherin gene were determined. For MGC2477, 15 single nucleotide polymorphisms (SNPs) were identified, with 13 having a frequency of the minor allele greater than 20%. 10 of the 15 SNPs have not been reported in so far in public SNP repertoires. Partial assessment of the TRPM3 gene yielded 35 SNPs. Of these, 30 (85.7%) were highly frequent (0.17-0.5%), and 14 (40%) were novel. The MT-Protocadherin gene revealed 35 SNPs, including 28 (80%) with high frequency of the minor allele. 23 (65.7%) were novel SNPs. These SNPs will be used to construct the most common haplotypes. These will be used in case/control association studies in 400 AMD patients and 200 ethnically and aged matched controls to assess a possible contribution of these genes in the etiology of AMD.
Soluble guanylyl cyclase (sGC) is the best established receptor for nitric oxide (NO) and regulates a great number of important physiological functions. Surprisingly, despite the wellappreciated roles of this enzyme in regulation of vascular tone, smooth muscle cell proliferation, platelet aggregation, renal sodium secretion, synaptic plasticity, and other functions, extremely little is known about the regulation of sGC activity and protein levels. To date, the only well-proven physiologically relevant sGC regulator is NO. In the present study, some additional possibilities for sGC regulation were shown. Firstly, we evaluated the ability of different NO donors to stimulate sGC. Significant differences in the sGC stimulation by SNP and DEA/NO were found. DEA/NO stimulated sGC much stronger than did SNP. Interestingly, no correlation between the sGC protein and maximal activity distribution was found in rat brain regions tested, suggesting the existence of some additional regulatory mechanisms for sGC. The failure of SNP to stimulate sGC maximally might be one of the reasons why the lack of correlation between the distribution of sGC activity and proteins in brain was not detected earlier. Prolonged exposure of endothelial cells to NO donors produced desensitization of the cGMP response. This desensitization cannot be explained by increased PDE activity, since PDE inhibitors were not able to prevent the NO donor-induced decrease of the maximal cGMP response in endothelial cells. The failure of SH-reducing agents to improve the cGMP response after its desensitization by NO suggests that a SH-independent mechanism mediates NO effects. Demonstration that the potency of the recently described activator of oxidized (heme-free) sGC, BAY58-2667, to stimulate sGC increases after prolonged exposure of the cells to an NO donor, DETA/NO, suggests that oxidation of heme may be a reason for NOinduced desensitization of sGC and decrease in sGC protein level. Indeed, the well-known heme-oxidizing agent ODQ produces a dramatic decrease in sGC protein levels in endothelial cells and BAY58-2667 prevents this effect. Although the mechanism of sGC activation and stabilization by BAY58-2667 is unknown, this substance is an interesting candidate to modulate sGC under conditions where sGC heme iron is oxidized. Very little is known about regulation of sGC by intracellular localization or translocation between different intracellular compartments. In the present study, an increase in sGC sensitivity to NO under membrane association was demonstrated. Treatment of isolated lung with VEGF markedly increased sGC in membrane fractions of endothelial cells. Failure of VEGF to stimulate sGC membrane association in cultured endothelial cells allows us to propose a complex mechanism of regulation of sGC membrane association and/or a transient character of sGC membrane attachment. A very likely mechanism for the attachment of sGC to membranes is via sGCinteracting proteins. These proteins may participate also in other aspects of sGC regulation. The role of the recently described sGC interaction partner, Hsp90, was investigated. Shortterm treatment of endothelial cells with an Hsp90 inhibitor does not affect NO donor or calcium ionophore-stimulated cGMP accumulation in the cells. However, inhibition of Hsp90 results in a rapid and dramatic decrease in sGC protein levels in endothelial cells. These effects were unrelated to changes in sGC transcription, since inhibition of transcription had much slower effect on sGC protein levels. In contrast, inhibitors of proteasomes abolished the reduction in sGC protein levels produced by an Hsp90 inhibitor, suggesting involvement of proteolytic degradation of sGC proteins during inhibition of Hsp90. All these data together suggest that Hsp90 is required to maintain mature sGC proteins. In conclusion, in the present study it was demonstrated that multiple mechanisms are involved in the regulation of sGC activity and its sensitivity to NO. Oxidation of sGC heme by NO seems to be one of the mechanisms for negative regulation of sGC in the presence of high or prolonged stimulation with NO. Another possible means of regulating sGC sensitivity to NO is via the intracellular translocation of the enzyme. It has been also demonstrated here that attachment of sGC to the membrane fraction results in an apparent increase in the enzyme sensitivity to NO. Additionally, Hsp90 was required to maintain sGC protein in endothelial and other cell types. However, we could not find any acute affect of Hsp90 on sGC activity, as reported recently. All these findings demonstrate that the regulation of sGC activity and protein level is a much more complex process than had been assumed earlier.
There is substantial interest in the identification of genes underlying susceptibility to complex human diseases because of the potential utility of such genes in disease prediction and therapy. The complex age-related macular degeneration (AMD) is a prevalent cause of legal blindness in industrialized countries and predominantly affects the elderly population over 75 years of age. Although vision loss in AMD results from photoreceptor cell death in the central retina, the initial pathogenesis likely involves processes in the retinal pigment epithelium (RPE) (Liang and Godley, 2003). The goal of the current study was to identify and characterize genes specifically or abundantly expressed in the RPE in order to determine more comprehensively the transcriptome of the RPE. In addition, our aim was to assess the role of these genes in AMD pathogenesis. Towards this end, a bovine cDNA library enriched for RPE transcripts was constructed in-house using a PCR-based suppression subtractive hybridization (SSH) technique (Diatchenko et al., 1996, 1999), which normalizes for sequence abundance and achieves high enrichment for differentially expressed genes. CAP3 (Huang and Madan, 1999) was used to assemble the high quality sequences of all the 2379 ESTs into clusters or singletons. 1.2% of the 2379 RPE-ESTs contains vector sequences and was excluded from further analysis. 5% of the RPE-ESTs showed homology to multipe chromosomes and were not included in further assembly process. The rest of the ESTs (2245) were assembled into 175 contigs and 509 singletons, which revealed approximately 684 unique genes in the dataset. Out of the 684, 343 bovine RPE transcripts did not align to their human orthologues. A large fraction of clones were shown to include a considerable 3´untranslated regions of the gene that are not conserved between bovine and human. It is the coding regions that can be conserved between bovine and human and not the 3’ UTR (Sharma et al., 2002). Therefore, more sequencing from the cDNA library with reclustering of those 343 ESTs together with continuous blasting might reveal their human orthologoues. To handle the large volume of data that the RPE cDNA library project has generated a highly efficient and user-friendly RDBMS was designed. Using RDBMS data storage can be managed efficiently and flexibly. The RDBMS allows displaying the results in query-based form and report format with additional annotations, links and search functions. Out of the 341 known and predicted genes identified in this study, 2 were further analyzed. The RPE or/and retina specificity of these two clones were further confirmed by RT-PCR analysis in adult human tissues. Construction of a single nucleotide polymphism (SNP) map was initiated as a first step in future case/control association studies. SNP genotyping was carried out for one of these two clones (RPE01-D2, now known as RDH12). 12 SNPs were identified from direct sequencing of the 23.4-kb region, of which 5 are of high frequency. In a next step, comparison of allele frequencies between AMD patients and healthy controls is required. Completion of the expression analysis for other predicted genes identified during this study is in progress using real time RT-PCR and will provide additional candidate genes for further analyses. This study is expected to contribute to our understanding of the genetic basis of RPE function and to clarify the role of the RPE-expressed genes in the predisposition to AMD. It may also help reveal the mechanisms and pathways that are involved in the development of AMD or other retinal dystrophies.
The study deals with the area of the allosteric modulation of the muscarinic M2 receptors. The allosteric modulators have an influence on binding of orthosteric ligands (agonists and antagonists) to the classical orthosteric binding site of the muscarinic M2-receptors. The modulators are able to enhance (positive cooperativity) or decrease (negative cooperativity)the affinity of ligands to the orthosteric binding site. The allosteric binding site is located at the entrance of the receptor binding pocket. It is less conserved than the orthosteric binding site which is located in a narrow cavity created by the seven transmembrane domains. Consequently, development of subtype selective allosteric ligands is easier than subtypeselective muscarinic agonists or antagonists. Furthermore, subtype selectivity can be achieved by differently cooperative interactions between the allosteric and orthosteric ligand at different receptor subtypes. For example, the allosteric modulators that are positively cooperative with ACh at M1 receptors and neutrally cooperative at the other receptor subtypes could be beneficial for treatment of the Alzheimer’s disease. Bisquaternary analogues of the Strychnos alkaloid caracurine V are among the most potent allosteric modulators of muscarinic M2-receptors. The very rigid ring skeleton comprises the pharmacophoric elements of two positively charged nitrogens at an approximate distance of 10 surrounded by two aromatic ring systems in a distinct spatial arrangement. Owing to the close structural relationship of caracurine V salts to the strong muscle relaxants toxiferine and alcuronium, they are likely to exhibit neuromuscular blocking activity, which would limit their usefulness as research tools and make the therapeutical use impossible. Reduction of the caracurine V ring skeletons to structural features responsible for good allosteric potency could possibly lead to compounds with negligible neuromuscular blocking activity and very high affinity to the allosteric binding site at M2 receptor. Thus, the aim of this study was to synthesize and pharmacologically evaluate analogues of a novel heterocyclic ring system, which comprises the pharmacophoric elements mentioned previously. The key step of the synthesis of the desired 6,7,14,15-tetrahydro[1,5]diazocino[1,2-a:6,5-a]-diindole ring system (6) involved the intermolecular double N-alkylation of the bromoethylindole (5), which was prepared from the known indolyl methylacetate (3) by reduction of the ester group to alcohol and subsequent substitution by bromine. 3 could be prepared in three steps involving N,N-dibenzylation of tryptamine followed by introduction of the dimethyl malonate moiety at C-2 of indole ring and a subsequent demethoxycarbonylation. The total synthesis of 6,7,14,15-tetrahydro[1,5]diazocino[1,2-a:6,5-a]diindole ring system (6) is shown in Scheme 24. In order to examine the influence of the length of the side-chain on muscarinic activity,exchange of the ethylamine moieties of 14 by the methylamino groups was planned. This should be accomplished by dimerization of the unsubstituted 2-bromoethylindole (32), and subsequent Mannich aminomethylation of the resulting unsubstituted pentacyclic ring. The total synthesis of the 6,7,14,15-tetrahydro-15aH-azocino[1,2-a:6,5-b]diindole ring system(35) is shown in Scheme 25. 32 was prepared from indole-2-carboxylic acid in six steps involving reduction of the acid to the corresponding alcohol 26, benzoylation of 26 followed by nucleophilic substitution with KCN, hydrolysis of the cyanide 28 to indolyl acetic acid 29,reduction of 29 to the corresponding alcohol 30, and finally bromination of 30 to give the bromide 32. Since dimerization attempts of 32 provided only 2-vinylindole (33), the tosylate 34 was used as starting material for the intermolecular alkylation to give exclusively an isomeric pentacyclic ring system, 7,14,15-tetrahydro-15aH-azocino[1,2-a:6,5-b]diindole (35). The formation of the novel, asymmetric ring skeleton can be explained by the ambident nucleophilic character of the indolyl anion that can be alkylated either at nitrogen or at C-3 of indole ring. 35 was subjected to a Mannich reaction to give 2,13-dimethylaminoalkylated product 37 as well as small amounts of the 13-monosubstituted compound (36). The geometry of novel ring systems 6 was elucidated by means of NMR spectroscopy and semiempirical calculations. The diazocinodiindole ring skeleton of 6 exists in chloroform solution at room temperature in a twisted-boat conformation, as indicated by 600 MHz ROESY experiment, vicinal coupling constants within the eight-membered ring, and AM1 calculations. In order to obtain potent allosteric ligands, the new heterocycles 6 and 37 were quarternized with methyliodide to the corresponding ammonium salts 14 and 38, respectively. Additionally, the N,N -diallylsalts of 37 (compound 39) was prepared. The allosteric effect of 14, 38, and 39 on the dissociation of the orthosteric radioligand [3H]Nmethylscopolamine([3H]NMS) and their effects on [3H]NMS equilibrium binding were studied in homogenates of porcine heart ventricles. The concentration of an allosteric agent for a half-maximum effect on orthosteric ligand dissociation (EC50,diss) corresponds to a 50 % occupancy of the liganded receptors by the respective allosteric test compounds. Due to the presence of two benzyl groups on each nitrogen in the side chains of 14, its binding affinity can be best compared with that of N,N -dibenzylcaracurinium V dibromide (EC50,diss = 69 nM). Compound 14 exhibited the comparable affinity to N,N -dibenzylcaracurinium V dibromide with EC50,diss = 54 nM. This result suggested that replacement of the bulky benzyl groups of 14 by smaller substitutents will probably increase the allosteric potency, since dimethyl- and diallylcaracurinium salts showed a 5-fold increase of binding affinity relative to the dibenzyl analogue. Even though the new azocinodiindole ring system of 38 and 39, is not included in the caracurine V ring skeleton, it comprises the essentially pharmacophoric elements of allosteric potency. Due to the different spatial arrangements of the aromatic rings, as well as to different internitrogen distances in both ring systems, compound 38 and 39 exhibited 4-fold lower M2 binding affinity (EC50,diss = 35 and 48 nM, respectively) than the corresponding caracurine V analogues. This study deals with the synthesis of the first representative (Compound 6) of a novel pentacyclic ring system derived from caracurine V. The high allosteric potency of its dimethyl analogue reveals the [1,5]diazocino[1,2-a:6,5-a]-diindole ring system as a new promising lead structure for allosteric modulators of muscarinic M2 receptors. Future research will be focused on structural modifications of the new ring system in order to increase the affinity to the muscarinic receptors. Furthermore, the binding affinities of the new synthesized compounds to the muscle type of nicotinic ACh-receptor should reveal structural features responsible for the muscarinic/nicotinic selectivity.
The mammalian Vasodilator Stimulated Phosphoprotein (VASP) is a founding member of the Ena/VASP family of proteins that includes Drosophila Enabled (ena), the mammalian Ena homologue (Mena) and the Ena-VASP-like protein (Evl). VASP was initially discovered and characterized as a substrate for cGMP- and cAMP-dependent protein kinases (cGKs and cAKs). Ena/VASP proteins are involved in Actin-filament formation, plasma membrane protrusion, acceleration of Actin-based motility of Listeria and the establishment of cell-cell adhesion. Moreover, Ena/VASP proteins have been implicated as inhibitory factors in repulsive axon guidance and inhibition of plasma membrane activity and random motility in fibroblast. In order to study the physiological function of VASP, VASP-deficient mice had been generated in the laboratory by homologous recombination. VASP-/- mice showed hyperplasia of megakaryocytes in the bone marrow and spleen and a two-fold increase in thrombin- and collagen-induced platelet activation. To further investigate the cellular function of VASP, I established cardiac fibroblast cell lines derived from both wild type and VASP-/- mice. Both cell lines presented similar growth rates and normal contact dependent-growth inhibition but showed differences in morphology, migration and adhesion. Adherent VASP-/- cells, despite normal Mena and Evl expression levels, were highly spread. VASP-/- cells covered about twice the substrate surface area as wild type cells, while the cell volumes were unchanged. This shape difference suggests that VASP is involved in the regulation of spreading. Since the small GTPases Rac and Cdc 42 and their effector p21-activated kinase (Pak) are key regulators of lamellipodia formation and cell spreading, I analyzed this signalling pathway in VASP-/- cells stimulated with Platelet Derived Growth Factor-BB (PDGF-BB) or fetal calf serum. In wild type cells Rac and Pak were rapidly and transiently activated by PDGF or serum; however, in the absence of VASP both Rac and Pak activation was dramatically prolonged. The Rac/Pak pathway is known to play an essential role in cell motility. VASP deficient cells showed compromised migration and reorientation in a wound healing assay, probably due to enhanced Rac activity. The spreading phenotype, compromised migration and the effect observed on the Rac and Pak activities were reverted in VASP-/- cells stably transfected with full lenght human VASP, indicating a VASP dependent modulation of the Rac/Pak pathway and Rac/Pak regulated processes. Moreover, adhesion and detachment of VASP-deficient cells were significantly slower when compared to wild type cells. Preincubation of VASP+/+ cells with a cGMP analog accelerated adhesion. This acceleration did not take place in the VASP-/- cells, suggesting a VASP dependent effect. The second part of this work focused on VASP function in platelets. On the one hand I investigated the possibility of VASP-dependent Rac regulation in mouse platelets. Murine platelets are a good model for studying Rac regulation since they express high levels of VASP but not Mena/Evl and since VASP-deficient platelets show an increased platelet activation. Rac was activated by platelet agonists which was inhibited by preincubation with cGMP and cAMP analogs. Initial results which need to be extended showed that the cGMPcaused inhibition of Rac activation was VASP-dependent. Finally, in vivo platelet adhesion (platelet-vessel wall interactions) was studied using VASP-deficient mice. These studies demonstrated in-vivo that VASP down regulates platelet adhesion to the vascular wall under both physiological and pathophysiological conditions.
In the work here presented four distinctly different problems were investigated. The first problem was an investigation into the degradation of Dichloroethylene (DCE) and 1,1-bis (p-Chlorophenyl)-2-dichloroethylene (DDE) utilising pure bacterial cultures. The second investigation dealt with the degradation of DDE and polychlorinated Biphenyl’s (PCB’s) utilising anaerobic sediments and soils from New Zealand. The third investigation worked on the Granulation of anaerobic River-sediments in Upflow Anaerobic Sludge Blanket (UASB) Reactors. The last investigation describes the commissioning of an industrial aerobic Wastewater Treatment Plant and the Implementation of biological Nitrogen- and Phosphate removal in this Wastewater Treatment Plant. Since the chemical Structure of DCE and DDE have certain similarities, Bacteria that were capable of degrading DCE, were tested here, whether they would also be able to degrade DDE utilising a co-metabolic pathway. In the experiments the aerobic bacteria Methylosinus trichosporium and Mycobacterium vaccae and the anaerobic bacteria Acetobacterium woodii and Clostridium butyricum were used. Approximately 60% of the added DCE was degraded by M. vaccae, while M. trichosporium degraded approximately 50%. A. woodii and C. butyricum degraded 40% and 30% respectively of the added DCE. Further experiments with these cultures and DDE lead to a microbial degradation of DDE to an extent of 34.6% for M. vaccae, 14.1% for C. butyricum, 2.2% for A. woodii and 10.5% for M. trichosporium. Additional experiments, utilising [14C]-DDE, showed that the DDE had not been degraded but were attached to the bacterial cells. The second investigation utilised anaerobic soils and sediments from New Zealand to study the anaerobic co-metabolic degradation of DDE and PCB’s. The soils and sediments originated from the River Waikato, from Wastewater Ponds in Kinleith, Marine-Sediments from Mapua, and a variety of soils comtaminated with Pentachlorophenyl (PCP). The cultures from these soils and sediments were raised on a variety of Carbon- and Energy-sources. Beside DDE, Aroclor 1260, and a mix of four pure PCB-Congeneres (one Tetra-, one Hexa, one Hepta- and one Deca-Chlorobiphenyl) were used to test for the reductive dechlorination. The cultivation process of the baceria lasted six months. Samples of the cultures were taken after zero, three and six months. These samples were tested for the increase of cell-protein, the degradation of carbon- and energy-sources, and the removal of the added polychlorinated chemicals. The organochlorines were analysed using reversed phase HPLC and FID-GC. When a change in the Chromatogram was detected the respective cultures were further analysed using ECD-GC and GC-MS. The results showed that the culutres grew under these conditions, but no degradation of DDE and the PCB-Mix could be detected, and only small changes in the composition/chromatograms of Aroclor 1260 were found. The third investigation worked on the Granulation of River-Sediments in UASB-Reactors. Sediments from the River Waikato in New Zealand and the River Saale in Germany were used. In both cases the Granulation process was successful, which was demonstrated by microscopic comparisons of the Sediments and the resulting Granules. The two main bacterial cultures detected were Methanosarcina- and Methanothrix-like cultures. The main carbon- and energy-source was Lactic Acid, which was used at a concentration of 21,8 g COD/L. The Granulation-Process was a combination of using high a COD-Concentration combined with a low Volumetric Loading-Rate. Comparisons of the specific degradation-rates of a variety of carbon- and energy-sources between the Sediments and the Granules, showed no increased degradation rates in regard to the same cell-mass, but the increased bio-mass in the Granules allowed for higher degradation-rates within the UASB-reactors. The fourth investigation describes the commissioning of an industrial Wastewater Treatment Plant for a Dairy-Site in Edendale, Southland, New Zealand. This Plant consists of a DAF-Unit (Dissolved Air Flotation), two Extended Aeration Lagoons with Activated Sludge and two Clarifiers, one for the Activated Sludge and the second for the dosing of Aluminium-Sulphate and the removal of Phosphat-Sulphate. Biological processes for the removal of carbon- and energy-sources were optimised and biological processes for the reduction of Nitrogen- and Phosphate-Concentrations within the wastewater were implemented and optimised. Bilogical removal rates for COD of 95% and above, for Nitrogen of 85-92% and Phosphate of 64-83% were achieved.
Fanconi anemia (FA) is a genetically and phenotypically heterogenous autoso- mal recessive disease associated with chromosomal instability, progressive bone marrow failure, typical birth defects and predisposition to neoplasia. The clinical phenotype is similar in all known complementation groups (FA-A, FA-B, FA-C,FA-D1, FA-D2, FA-E, FA-F and FA-G). The cellular phenotype is characterized by hypersensitivity to DNA crosslinking agents (MMC,DEB), which is exploited as a diagnostic tool. Alltogether, the FA proteins constitute a multiprotein pathway whose precise biochemical function(s) remain unknown. FANCA, FANCC, FANCE, FANCF and FANCG interact in a nuclear complex upstream of FANCD2. Complementation group FA-D1 was recently shown to be due to biallelic mutations in the human breast cancer gene 2 (BRCA2). After DNA damage, the nuclear complex regulates monoubiquitylation of FANCD2, result- ing in targeting of this protein into nuclear foci together with BRCA1 and other DNA damage response proteins. The close connection resp. identity of the FA genes and known players of the DSB repair pathways (BRCA1, BRCA2, Rad51) firmly establishs an important role of the FA gene family in the maintenance of genome integrity. The chapter 1 provides a general introduction to the thesis describing the current knowledge and unsolved problems of Fanconi anemia. The following chapters represent papers submitted or published in scientific literature. They are succeeded by a short general discussion (chapter 7). Mutation analysis in the Fanconi anemia genes revealed gene specific mutation spectra as well as different distributions throughout the genes. These results are described in chapter 1 and chapter 2 with main attention to the first genes identified, namely FANCC, FANCA and FANCG. In chapter 2 we provide general background on mutation analysis and we report all mutations published for FANCA, FANCC and FANCG as well as our own unpublished mutations until the year 2000. In chapter 3 we report a shift of the mutation spectrum previously reported for FANCC after examining ten FA-patients belonging to complementation group C. Seven of those patients carried at least one previously unknown mutation, whereas the other three patients carried five alleles with the Dutch founder mu- tation 65delG and one allele with the Ashkenazi founder mutation IVS4+4A>T, albeit without any known Ashkenazi ancestry. We also describe the first large deletion in FANCC. The newly detected alterations include two missense mu- tations (L423P and T529P) in the 3´-area of the FANCC gene. Since the only previously described missense mutation L554P is also located in this area, a case can be made for the existence of functional domain(s) in that region of the gene. In chapter 4 we report the spectrum of mutations found in the FANCG gene com- piled by several laboratories working on FA. As with other FA genes, most muta- tions have been found only once, however, the truncating mutation, E105X, was identified as a German founder mutation after haplotype analysis. Direct compar- ison of the murine and the human protein sequences revealed two leucine zipper motifs. In one of these the only identified missense mutation was located at a conserved residue, suggesting the leucine zipper providing an essential protein-protein interaction required for FANCG function. With regard to genotype-phenotype correlations, two patients carrying a homozygous E105X mutation were seen to have an early onset of the hematological disorder, whereas the missense mutation seems to lead to a disease with later onset and milder clinical course. In chapter 5 we explore the phenomenon of revertant mosaicism which emerges quite frequently in peripheral blood cells of patients suffering from FA. We de- scribe the types of reversion found in five mosaic FA-patients belonging to com- plementation groups FA-A and FA-C. For our single FA-C-patient intragenic crossover could be proven as the mechanism of self-correction. In the remaining four patients (all of them being compound heterozygous in FANCA), either the paternal or maternal allele has reverted back to WT sequence. We also describe a first example of in vitro phenotypic reversion via the emergence of a compensat- ing missense mutation 15 amino acids downstream of the constitutional mutation explaining the MMC-resistance of the lymphoblastoid cell line of this patient. In chapter 6 we report two FA-A mosaic patients where it could be shown that the spontaneous reversion had taken place in a single hematopoietic stem cell. This has been done by separating blood cells from both patients and searching for the reverted mutation in their granulocytes, monocytes, T- and B-lymphocytes as well as in skin fibroblasts. In both patients, all hematopoietic lineages, but not the fibroblasts, carried the reversion, and comparison to their increase in erythrocyte and platelet counts over time demonstrated that reversion must have taken place in a single hematopoietic stem cell. This corrected stem cell then has been able to undergo self-renewal and also to create a corrected progeny, which over time repopulated all hematopoietic lineages. The pancytopenia of these patients has been cured due to the strong selective growth advantage of the corrected cells in vivo and the increased apoptosis of the mutant hematopoietic cells.
In vitro and in vivo studies on the activating platelet collagen receptor glycoprotein VI in mice
(2003)
The work summarized here focused on the characterization of the murine platelet collagen receptor glycoprotein (GP) VI and was performed to evaluate its potential as an antithrombotic target. The first mAb against (mouse) GPVI, JAQ1, was generated and used to demonstrate that GPVI requires the FcRgamma-chain for its expression and function and that this receptor is the central molecule in collagen-induced platelet activation. Blocking the major collagen binding site on GPVI with JAQ1 revealed the presence of a second activatory epitope within collagen. Additionally, the collagen receptor integrin alpha2beta1 was found to be required for activation via this second pathway but not to be essential for collagen-induced activation of normal platelets. In studies with mice expressing reduced levels of the GPVI-FcRgamma-complex, differential responses to GPVI ligands were observed. Most importantly, the striking difference between platelet responses to collagen and the GPVI specific synthetic collagen related peptide (CRP) confirmed the supportive role of other collagen receptor(s) on platelets. Irrespective of yet undefined additional receptors, studies with mice deficient in GPVI (FcRgamma-chain) or alpha2beta1 showed that GPVI, but not alpha2beta1 is essential for platelet-collagen interaction. Based on these results, the model of platelet attachment to collagen was revised establishing GPVI as the initial activating receptor which upregulates the activity of integrins, thus enabling firm attachment of platelets to the ECM. While the mAb JAQ1 had only limited inhibitory effects on collagen-induced activation in vitro, its in vivo application to mice resulted in completely abolished platelet responses to collagen and the GPVI specific agonists CRP and convulxin. This effect was found to be due to antibody-induced irreversible down-regulation of GPVI on circulating platelets for at least two weeks. Further studies revealed that GPVI depletion occurs independently of the targeted epitope on the receptor and does not require the divalent form of IgG as it was also induced by mAbs (JAQ2, JAQ3) or the respective Fab fragments directed against epitopes distinct from the major collagen binding site. The internalization of GPVI in vivo resulted in a long-term protection of the mice from lethal collagen-dependent thromboembolism whereas it had only moderate effects on the bleeding time, probably because the treatment did not affect other activation pathways. These results establish GPVI as a potential pharmacological target for the prevention of ischemic cardiovascular diseases and may open the way for a completely new generation of antithrombotics.