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Intrinsic response properties of auditory thalamic neurons in the Gerbil (Meriones unguiculatus)
(2007)
Neurons in the medial geniculate body (MGB) have the complex task of processing the auditory ascending information from the periphery and a more extensive descending input from the cortex. Differences in the pattern of afferent and efferent neuronal connections suggest that neurons in the ventral and dorsal divisions of the MGB take different roles in this complex task. The ventral MGB (vMGB) is the primary, tonotopic, division and the dorsal MGB (dMGB) is one of the higher order, nontonotopic divisions. The vMGB neurons are arranged tonotopically, have sharp tuning properties, and a short response delay to acoustic stimuli. The dMGB neurons are not tonotopically arranged, have broad tuning properties, and a long response delay to acoustical stimuli. These two populations of neurons, with inherently different tasks, may display differences in intrinsic physiological properties, e.g. the capacity to integrate information on a single cell level. Neurons of the ventral and dorsal divisions of the MGB offer an ideal system to explore and compare the intrinsic neuronal properties related to auditory processing. Coronal slices of 200 μm thicknesses were prepared from the thalamus of 4 - 5 week old gerbils. The current-clamp configuration of the patch-clamp technique was used to do experiments on the dorsal and ventral divisions of the medial geniculate body. Slices were subsequently Nissl stained to verify the location of recording. Recordings from the dorsal and ventral divisions exhibited differences in response to depolarizing current injections. The ventral division responded with significantly shorter first spike latency (vMGB = 41.50 ± 7.7, dMGB = 128.43 ± 16.28; (p < 0.01)) and rise time constant (vMGB = 6.95 ± 0.90, dMGB = 116.67 ± 0.13; (p < 0.01)) than the dMGB. Neurons in the dorsal division possessed a larger proportion of slowly accommodating neurons (rapidly accommodating: vMGB: 89%, dMGB: 64%), including a subpopulation of neurons that fired at resting membrane potential. Neurons in the vMGB are primarily responsible for relaying primary auditory input. Dorsal MGB neurons relay converging multimodal input. A comparative analysis with the primary auditory neurons, the Type I and Type II spiral ganglion neurons, reveals a similar pattern. Type I neurons relay primary auditory input and exhibit short first spike latencies and rise time constants. The Type II neurons relay converging input from many sources, while possessing significantly slower response properties and a greater subpopulation of slowly accommodating neurons. Hence, accommodation, first spike latency, and rise time constant are suggested to be a reflection of the amount of input that must be integrated before an action potential can be fired. More converging input correlates to slower accommodation, a longer first spike latency and rise time. Conversely, a greater capacity to derive discrete input is associated with rapid accommodation, along with a short first spike latency and rise time.
The work presented in this thesis addresses a key issue of the CBM experiment at FAIR, which aims to study charm production in heavy ion collisions at energies ranging from 10 to 40 AGeV . For the first time in this kinematical range, open charm mesons will be used as a probe of the nuclear fireball. Despite of their short decay length, which is typically in the order of few 100 µm in the laboratory frame, those mesons will be identified by reconstructing their decay vertex.
This dissertation contains five independent chapters dealing with wage dispersion and unemployment. The first chapter deals with the explanation of international changes in wage inequality and unemployment in the 80s and 90s. Both theoretically and empirically, social benefits and its link to average income are blamed for the different experiences across countries. The second chapter discusses the search framework, to explain residual wage inequality and finds that institutional wage compression has ambiguous effects on employment. In the third chapter, we apply the theory to German data. We show that job-to-job transitions are important in explaining both frictions and career advances. In the fourth chapter, we empirically assess the relationship between wage dispersion and unemployment for homogeneous workers. We find that neither a frictional nor a neo-classical view in explaining this relationship are convincing. Unemployment within cells is not negatively correlated with wage dispersion. Finally, the last chapter builds a theoretical model which treats heterogeneous individuals in a production function framework and a frictional labor market. The model generates both wage dispersion within and between skill groups and both frictional and structural unemployment. In sum, the dissertation stresses the importance of modelling frictions to understand different types of wage inequality and unemployment.
Spatio-temporal dynamics of primary lymphoid follicles during organogenesis and lymphneogenesis
(2007)
Primary lymphoid follicles are structures which are important for adaptive immune responses in mammals. Within the follicles follicular dendritic cells (FDC) are maintained by constant stimuli provided by B cells. It is thought that the FDC are important for immune response. It is of interest to know how lymphoid follicles are regulated in order to understand their role in various autoimmune diseases in which these follicles are created ectopically. With the help of a tissue simulation relying on an agent-based cell model on top of a regular triangulation various scenarios suggested by the available experimental data have been investigated. In order to cope with the complexity in the simulation of immune tissue the regular triangulation has been implemented for the use on parallel computers. The algorithms for kinetic and dynamic regular triangulation have been created newly. Also the cell model underlying the simulation has been designed newly in many aspects. The simulations allowed to identify common factors that regulate the formation of lymphoid follicles normally during organogenesis in development and lymphneogenesis in the course of diseases. The generation of FDC from local stromal populations under the influence of B cell aggregates is shown to be possible with the given experimental parameters. The sequence of the organogenesis and lymphneogenesis can be described with regard to the morphology of the B and T zone. Tests for the stability of the primary lymphoid follicle system constraints the regulation of the B cell efflux. The required lymphatic vessels around the lymphoid follicle are shown to be negatively correlated with the FDC network. Moreover it is shown that the adjacent T zone consisting of its own stromal population and T cells has similar regulation principles. This easily explains the intermediate ring of B cells found around the T zone during development and certain signaling molecule deficiencies. A major result of this thesis is that the generation of FDC needs negative regulation while a number of other possible mechanisms is incompatible with the available experimental data. Moreover the observed microanatomy was brought into a functional relationship with data on the cellular level finally culminating in the proposal of new experiments that shed light on the dynamics of the primary lymphoid follicle. One conclusion is that the FDC directly or indirectly influence the angiogenesis and lymphangiogenesis processes in secondary lymphoid tissues. The work presented here may help to guide experiments with the help of computers in order to reduce the amount of experiments and design them in a way to maximize the amount of information about biological systems.
Rhythmic changes in environmental lighting conditions have ever been the most reliable environmental cue for life on earth. Nature has therefore selected a genetically encrypted endogenous clock very early in evolution, as it provided cells and subsequently organisms with the ability to anticipate persevering periods of light and darkness. Rhythm generation within the mammalian circadian system is achieved by clock genes and their protein products. The mammalian endogenous master clock, which synchronizes the body to environmental time, is located in the suprachiasmatic nucleus (SCN) of the hypothalamus. As an integral part of the time-coding system, the pineal gland serves the need to tune the body to the temporal environment by the rhythmic nocturnal synthesis and immediate release of the hormone melatonin. In contrast to the transcriptional regulation of melatonin synthesis in rodents, a post-translational shaping is indicated in the human pineal gland. Another important mediator of circadian time and seasonality to the body is the pituitary gland. The aim of this work was to elucidate regulation of melatonin synthesis in the human pineal gland. Furthermore, presence and regulation of clock genes in the human pineal and pituitary gland, and in the SCN were analyzed. Therefore, human tissue, taken from regular autopsies, was analyzed simultaneously for different parameters involved in melatonin biosynthesis and circadian rhythm generation. Presented data demonstrate that post-mortem brain tissue can be used to detect the remnant profile of pre-mortem adaptive changes in neuronal activity. In particular, our results give strong experimental support for the idea that transcriptional mechanisms are not dominant for the generation of rhythmic melatonin synthesis in the human pineal gland. Together with data obtained for clock genes and their protein products in the pituitary, data presented here offer 1) a new working hypothesis for post-translational regulation of melatonin biosynthesis in the human pineal gland, and 2) a novel twist in the molecular competence of clock gene proteins, achieved by nucleo-cytoplasmic shuttling in neuronal and neuroendocrine human tissue. Furthermore, in this study, oscillations in abundance of clock gene proteins were demonstrated for the first time in the human SCN.
The removal of apoptotic cells (AC) can be regarded as an integral component of the program to terminate inflammation. Clearance of AC by professional phagocytes such as macrophages induces an anti-inflammatory phenotype in the latter ones. Anti-inflammatory or M2 polarization is also observed in macrophages infiltrating certain human tumors. These tumor-associated macrophages (TAM) contribute actively to tumor progression by promoting immune evasion, angiogenesis and tumor cell survival. The aim of my Ph.D. thesis was to approach the mechanisms as well as the characteristics of macrophage phenotype alterations induced by AC, and to elucidate a possible connection between tumor cell apoptosis and TAM generation. In the first part of my studies, I investigated the impact of AC on macrophage viability. I could show that macrophage survival against pro-apoptotic agents increased after the interaction with AC. Protection of macrophages against cell death required activation of phosphatidylinositol-3 kinase (PI3K), extracellular signal-regulated kinase 1/2 (ERK1/2) and Ca2+ signaling, and correlated with Bcl-XL and Bcl-2 up-regulation as well as Ser136-Bad phosphorylation. Unexpectedly, neither phagocytosis nor binding of apoptotic debris to the phagocyte was necessary to induce protection. AC released the bioactive lipid sphingosine-1-phosphate (S1P), dependent on sphingosine kinase (SphK) 2, as a survival messenger. These data indicated an active role of AC in preventing cell destruction in their neighborhood. My next aim was to elucidate the mechanism of S1P production by AC. During cell death, SphK 2 was cleaved at its N-terminus by caspase-1. Thereupon, the truncated but enzymatically active fragment of SphK 2 was released from cells. This release was coupled to phosphatidylserine exposure, a hallmark of apoptosis and a crucial signal for the phagocyte/apoptotic cell interaction. Thus, I observed a link between common signaling events during apoptosis and the extracellular production of S1P, which is known to affect immune cell attraction and polarization as well as angiogenesis in cancer. In the next part of my studies, I asked for a correlation between tumor cell apoptosis and TAM polarization. During co-culture of human macrophages with human breast cancer carcinoma cells (MCF-7), the latter ones were killed, while macrophages acquired an alternatively activated phenotype. This was characterized by decreased tumor necrosis factor (TNF)-α; and interleukin (IL)-12-p70 production, but increased formation of IL-8 and IL-10. Alternative macrophage activation required tumor cell death, because a co-culture with apoptosis-resistant colon carcinoma cells (RKO) or Bcl-2-overexpressing MCF-7 cells failed to induce phenotype alterations. These phenotype alterations were also achieved with conditioned media from apoptotic tumor cells, which again argued for a soluble factor being involved. Knock-down of SphK2, but not SphK1, to attenuate S1P formation in MCF-7 cells, repressed the otherwise observed alternative macrophage polarization during co-culture. Furthermore, macrophage polarization achieved by tumor cell apoptosis or substitution of authentic S1P was characterized by suppression of pro-inflammatory nuclear factor (NF)-κB DNA binding. These findings suggested that tumor cell apoptosis-derived S1P contributes to the macrophage polarization present in human tumors. To validate these in vitro data, I used an in vivo tumor model to clarify the relevance of SphK2 and S1P in tumor development. The growth of, as well as blood vessel infiltration into SphK2 knock-down MCF-7 (MCF-7-siSphK2) xenografts in nude mice was markedly decreased in comparison to control MCF-7 xenografts. In contrast, macrophage infiltration was similar or even more pronounced. These data provided a first hint for an in vivo role of SphK2-derived S1P in macrophage polarization associated with tumor promotion. In summary, these data indicate a new mechanism how AC themselves shape macrophage polarization, which results in the termination of inflammatory responses and macrophage survival. Furthermore, my studies present evidence that human tumors may utilize this mechanism to foster growth via increased angiogenesis.
The high energy loss of heavy ions in matter as well as the small angular scattering makes heavy ion beams an excellent tool to produce almost cylindrical and homogeneously excited volumes in matter. This aspect can be used to pump short wavelength lasers. In an experiment performed at the GSI (Gesellschaft für Schwerionenforschung, Darmstadt, Germany) ion accelerator facility in December 2005 the well-known KrF* excimer laser was pumped with an intense high energy uranium beam. Pulses of an uranium beam with initial particle energy of 250 MeV per nucleon, provided by heavy-ion-synchrotron SIS-18, were delivered to the HHT-target station and then stopped inside a gas laser cell. The maximum beam intensity reached in the experiment was 2,5·109 particles per pulse, which resulted in 34 J/g specific energy deposited in the laser gas. By applying electron cooling and a bunch compression technique at SIS-18, the beam pulses were compressed down to 110 ns (FWHM). A mixture of an excimer laser premix gas (95,5% Kr + 0,5% F2) and a buffer gas (Ar 4.8) was used as the laser gas in proportions of 35/65 and 60/40, respectively. The gas pressure inside the laser cell was varied in the range of 1,2÷2 bar in continues flow mode. The experimental setup consisted of a 1 m long stainless steel tube with a number of diagnostic viewports and two mirror adjustment units. The optical cavity was formed by a flat, Alcoated mirror at the beam entrance and a second dielectrically coated, highly reflective mirror with 3 m radius of curvature at a distance of 1,3 m. A beam of heavy ions has been used to pump a short wavelength gas laser for the first time. Laser effect on the KrF* laser transition (λ = 248 nm) has been successfully demonstrated. Laser threshold for this specific setup was reached with a beam intensity of 1,2·109 particles per pulse. Laser action has been clearly proofed by the following methods: appearance of the laser line, spectral narrowing of the laser line, temporal narrowing of the laser signal, non-linear response of the laser output intensity on the pumping power, and cavity disalignment effect. An energy of the laser pulse of about 2 mJ was measured for an ion beam intensity of 2·109 particles per pulse. The time delay of the onset of the laser emission with respect to the pumping pulse was measured as a function of ion beam intensity. The dependence of spontaneous emission spectra on the gas pressure in a range of 1,3÷2 bar was observed and the optimal gas pressure for laser experiments in the sense of laser efficiency was concluded. As a next step in studying short wavelength lasers pumped with heavy ion beams it is planned to reduce the laser wavelength down to the VUV region of the spectrum, and to proceed to the excimer lasers of the pure rare gases: Xe2 * (λ = 172 nm), Kr2 * (λ = 146 nm), Ar2 * (λ = 126 nm), Ne2 * (λ = 83 nm) and He2 * (λ = 80 nm). We believe that the use of heavy ion beams as a pumping source may lead to new pumping schemes on the higher lying level transitions and considerably shorter wavelengths (XUV and X-ray spectral region), which rely on the high cross sections for multiple ionization of the target species.