@phdthesis{Wagh2005,
  author    = {Wagh, Dhananjay Anil},
  title     = {"Bruchpilot" -molecular and functional characterization of a novel active zone protein at the Drosophila synapse},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-14989},
  school      = {Universit{\"a}t W{\"u}rzburg},
  year      = {2005},
  abstract  = {Chemical neurotransmission is a complex process of central importance for nervous system function. It is thought to be mediated by the orchestration of hundreds of proteins for its successful execution. Several synaptic proteins have been shown to be relevant for neurotransmission and many of them are highly conserved during evolution- suggesting a universal mechanism for neurotransmission. This process has checkpoints at various places like, neurotransmitter uptake into the vesicles, relocation of the vesicles to the vicinity of calcium channels in order to facilitate Ca2+ induced release thereby modulating the fusion probability, formation of a fusion pore to release the neurotransmitter and finally reuptake of the vesicles by endocytosis. Each of these checkpoints has now become a special area of study and maintains its own importance for the understanding of the overall process. Ca2+ induced release occurs at specialized membrane structures at the synapse known as the active zones. These are highly ordered electron dense grids and are composed of several proteins which assist the synaptic vesicles in relocating in the vicinity of Ca2+ channels thereby increasing their fusion probability and then bringing about the vesicular fusion itself. All the protein modules needed for these processes are thought to be held in tight arrays at the active zones, and the functions of a few have been characterized so far at the vertebrate active zones. Our group is primarily interested in characterizing the molecular architecture of the Drosophila synapse. Due to its powerful genetics and well-established behavioural assays Drosophila is an excellent system to investigate neuronal functioning. Monoclonal antibodies (MABs) from a hybridoma library against Drosophila brain are routinely used to detect novel proteins in the brain in a reverse genetic approach. Upon identification of the protein its encoding genetic locus is characterized and a detailed investigation of its function is initiated. This approach has been particularly useful to detect synaptic proteins, which may go undetected in a forward genetic approach due to lack of an observable phenotype. Proteins like CSP, Synapsin and Sap47 have been identified and characterized using this approach so far. MAB nc82 has been one of the shortlisted antibodies from the same library and is widely used as a general neuropil marker due to the relative transparency of immunohistochemical whole mount staining obtained with this antibody. A careful observation of double stainings at the larval neuromuscular junctions with MAB nc82 and other pre and post-synaptic markers strongly suggested an active zone localization of the nc82 antigen. Synaptic architecture is well characterized in Drosophila at the ultrastructural level. However, molecular details for many synaptic components and especially for the active zone are almost entirely unknown. A possible localization at the active zone for the nc82 antigen served as the motivation to initiate its biochemical characterization and the identification of the encoding gene. In the present thesis it is shown by 2-D gel analysis and mass spectrometry that the nc82 antigen is a novel active zone protein encoded by a complex genetic locus on chromosome 2R. By RT-PCR exons from three open reading frames previously annotated as separate genes are demonstrated to give rise to a transcript of at least 5.5 kb. Northern blots produce a prominent signal of 11 kb and a weak signal of 2 kb. The protein encoded by the 5.5 kb transcript is highly conserved amongst insects and has at its N-terminus significant homology to the previously described vertebrate active zone protein ELKS/ERC/CAST. Bioinformatic analysis predicts coiled-coil domains spread all over the sequence and strongly suggest a function involved in organizing or maintaining the structure of the active zone. The large C-terminal region is highly conserved amongst the insects but has no clear homologues in veretebrates. For a functional analysis of this protein transgenic flies expressing RNAi constructs under the control of the Gal4 regulated enhancer UAS were kindly provided by the collaborating group of S.Sigrist (G\&\#1616;ttingen). A strong pan-neuronal knockdown of the nc82 antigen by transgenic RNAi expression leads to embryonic lethality. A relatively weaker RNAi expression results in behavioural deficits in adult flies including unstable flight and impaired walking behavior. Due to this peculiar phenotype as observed in the first knockdown studies the gene was named "bruchpilot" (brp) encoding the protein "Bruchpilot (BRP)" (German for crash pilot). A pan-neuronal as well as retina specific downregulation of this protein results in loss of ON and OFF transients in ERG recordings indicating dysfunctional synapses. Retina specific downregulation also shows severely impaired optomotor behaviour. Finally, at an ultrastructural level BRP downregulation seems to impair the formation of the characteristic T-shaped synaptic ribbons at the active zones without significantly altering the overall synaptic architecture (in collaboration with E.Asan). Vertebrate active zone protein Bassoon is known to be involved in attaching the synaptic ribbons to the active zones as an adapter between active zone proteins RIBEYE and ERC/CAST. A mutation in Bassoon results in a floating synaptic ribbon phenotype. No protein homologous to Bassoon has been observed in Drosophila. BRP downregulation also results in absence of attached synaptic ribbons at the active zones. This invites the speculation of an adapter like function for BRP in Drosophila. However, while Bassoon mutant mice are viable, BRP deficit in addition to the structural phenotype also results in severe behavioural and physiological anomalies and even stronger downregulation causes embryonic lethality. This therefore suggests an additional and even more important role for BRP in development and normal functioning of synapses in Drosophila and also in other insects. However, how BRP regulates synaptic transmission and which other proteins are involved in this BRP dependant pathway remains to be investigated. Such studies certainly will attract prominent attention in the future.},
  subject      = {Taufliege},
  language  = {en}
}
@phdthesis{Raffelsbauer2001,
  author    = {Raffelsbauer, Diana},
  title     = {Identification and characterization of the inlGHE gene cluster of Listeria monocytogenes},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-1180595},
  school      = {Universit{\"a}t W{\"u}rzburg},
  year      = {2001},
  abstract  = {In the present study, a new gene cluster of Listeria monocytogenes EGD containing three internalin genes was identified and characterized. These genes, termed inlG, inlH and inlE, encode proteins of 490, 548 and 499 amino acids, respectively, which belong to the class of large, surface-bound internalins. Each of these proteins contains a signal peptide, two regions of repeats (Leucine-rich repeats and B repeats), an inter-repeat region and a putative cell wall anchor sequence containing the sorting motiv LPXTG. PCR analysis revealed the presence of the inlGHE gene cluster in most L. monocytogenes serotypes. A similar gene cluster termed inlC2DE localised to the same position on the chromosome was described in a different L. monocytogenes EGD isolate. Sequence comparison of the two clusters indicates that inlG is a new internalin gene, while inlH was generated by a site-specific recombination leading to an in-frame deletion which removed the 3'-terminal end of inlC2 and a 5'-portion of inlD. The genes inlG, inlH and inlE seem to be transcribed extracellularly and independent of PrfA. To study the function of the inlGHE gene cluster several in-frame deletion mutants were constructed which lack the genes of the inlGHE cluster individually or in combination with other inl genes. When tested in the mouse model, the inlGHE mutant showed a significant reduction of bacterial counts in liver and spleen in comparison to the wild type strain, indicating that the inlGHE gene cluster plays an important role in virulence of L. monocytogenes. The ability of this mutant to invade non-phagocytic cells in vitro was however two- to three-fold higher than that of the parental strain. To examine whether deletion of the single genes from the cluster has the same stimulatory effect on invasiveness as deletion of the complete gene cluster, the single in-frame deletion mutants inlG, inlH and inlE were constructed. These mutants were subsequently reverted to the wild type by introducing a copy of the corresponding intact gene into the chromosome by homologous recombination using knock-in plasmids. To determine a putative contribution of InlG, InlH and InlE in combination with other internalins to the entry of L. monocytogenes into mammalian cells, the combination mutants inlA/GHE, inlB/GHE, inlC/GHE, inlA/B/GHE, inlB/C/GHE, inlA/C and inlA/C/GHE were constructed. Transcription of the genes inlA, inlB and inlC in these mutants was studied by RT-PCR. Deletion of inlGHE enhances transcription of inlA and inlB, but not of inlC. This enhancement is not transient but can be observed at different time-points of the bacterial growth curve. Deletion of inlA also increases transcription of inlB and vice-versa. In contrast, the amounts of inlA and inlB transcripts in the single deletion mutants inlG, inlH and inlE were similar to those from the wild type.},
  subject      = {Listeria monocytogenes},
  language  = {en}
}
@phdthesis{Pietsch2005,
  author    = {Pietsch, Christof},
  title     = {The genetics of species differences within the genus Nasonia ASHMEAD 1904 (Hymenoptera: Pteromalidae)},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-14348},
  school      = {Universit{\"a}t W{\"u}rzburg},
  year      = {2005},
  abstract  = {The genetics of species differences is an outstanding question in evolutionary biology. How do species evolve to become phenotypically distinct and how is the genetic architecture organized that underlie species differences? Phenotypic diverged traits are supposed to be frequently involved in prezygotic isolation, i.e. they prevent the formation of hybrids, whereas postzygotic isolation occurs when hybrids experience a fitness reduction. The parasitic wasp genus Nasonia represents an appropriate model system to investigate the genetics of species differences as well as the genetics of postzygotic isolation. The genus consists of three species N. vitripennis, N. longicornis and N. giraulti that differ particularly in male traits that are assumed to posses an adaptive significance: courtship behaviour and wing size differences. The courtship behaviour consists of cyclically repeated series of head nods that are separated by pauses. The stereotypic performance allowed to split up the display into distinct courtship components. Males of N. vitripennis bear vestigial forewings and are incapable of flight, whereas N. longicornis wear intermediate sized wings and N. giraulti is fully capable of flying. Nasonia species can produce interspecific hybrids after removing Wolbachia bacteria induced hybrid incompatibilities with antibiotics. Postzygotic isolation occurs to different extent and is asymmetric among reciprocal crosses, e.g. inviability is stronger in the N. vitripennis (\&\#9792;) x N. longicornis (\&\#9794;) cross than in the N. longicornis (\&\#9792;) x N. vitripennis (\&\#9794;) cross. The formation of hybrids allow to study the genetic of species differences in QTL (quantitative trait locus) analyses as well as the genetics of postzygotic isolation causing hybrid inviability. The aim of the study was to investigate the genetic architecture of differences in courtship behaviour and wing size between N. vitripennis and N. longicornis and to assess the genetics of postzygotic isolation to gain clues about the evolutionary processes underlying trait divergence and establishment of reproductive isolation between taxa. In a QTL analysis based on 94 F2-hybrid individuals of an LV cross only few QTL for wing size differences have been found with relatively large effects, although a large proportion of the phenotypic variance remained unexplained. The QTL on courtship behaviour analysis based on 94-F2 hybrid males revealed a complex genetic architecture of courtship behaviour with QTL of large phenotypic effects that explained more than 40 \% of the phenotypic variance in one case. Additionally, an epistatic analysis (non-additive interlocus interaction) of courtship QTL revealed frequent genetic interchromsomal relations leading in some instances to hybrid specific effects, e.g. reversion of phenotypic effects or the transgression of phenotypes. A QTL analysis based on a threefold sample size revealed, however, an overestimation of QTL effects in the analysis based on smaller sample size pointing towards a genetic architecture of many loci with small effects governing the phenotypic differences in courtship behaviour. Furthermore, the the study comprised the analysis of postzygotic isolation in the reciprocal crosses N. vitripennis (\&\#9792;) x N. longicornis (\&\#9794;) versus N. longicornis (\&\#9792;) x N. vitripennis (\&\#9794;) located several loci distributed over different chromosomes that are involved in hybrid incompatibility. The mapping of hybrid incompatibility regions reproduced for the first time the observed asymmetries in the strength of postzygotic isolation in reciprocal crosses of between the more distant related taxa within the genus Nasonia. Stronger postzygotic incompatibilities in the VL cross are supposed to result from the superposition of nuclear-nuclear incompatibilities with nuclear-cytoplasmic incompatibilities, whereas the coincidences of these to types of incompatibilities were found to be much weaker in the reciprocal LV cross.},
  subject      = {Pteromalidae},
  language  = {en}
}
@phdthesis{Niewalda2010,
  author    = {Niewalda, Thomas},
  title     = {Neurogenetic analyses of pain-relief learning in the fruit fly},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-65035},
  school      = {Universit{\"a}t W{\"u}rzburg},
  year      = {2010},
  abstract  = {All animals learn in order to cope with challenges imposed on them by their environment. This is true also for both larval and adult fruit flies as exemplified in pavlovian conditioning. The focus of this Thesis is on various aspects of the fruit flies learning ability. My main project deals with two types of learning which we call punishment-learning and pain-relief learning. Punishment learning happens when fruit flies are exposed to an odour which is followed by electric shock. After such training, flies have learned that that odour signals pain and consequently will avoid it in the future. If the sequence of the two stimuli is reversed such that odour follows shock, flies learn the odour as a signal for relief and will later on approach it. I first report a series of experiments investigating qualitative and parametric features of relief-learning; I find that (i) relief learning does result from true associative conditioning, (ii) it requires a relatively high number of training trials, (iii) context-shock training is ineffective for subsequent shock-odour learning. A further question is whether punishment-learning and pain-relief learning share genetic determinants. In terms of genetics, I test a synapsin mutant strain, which lacks all Synapsin protein, in punishment and relief-learning. Punishment learning is significantly reduced, and relief-learning is abolished. Pan-neuronal RNAi-mediated knock-down of Synapsin results in mutant-like phenotypes, confirming the attribution of the phenotype to lack of Synapsin. Also, a rescue of Synapsin in the mushroom body of syn97 mutants restores both punishment- and relief-learning fully, suggesting the sufficiency of Synapsin in the mushroom body for both these kinds of learning. I also elucidate the relationship between perception and physiology in adult fruit flies. I use odour-shock conditioning experiments to identify degrees of similarity between odours; I find that those similarity measures are consistent across generalization and discrimination tasks of diverse difficulty. Then, as collaborator of T. V{\"o}ller and A. Fiala, I investigate how such behavioural similarity/dissimilarity is reflected at the physiological level. I combine the behaviour data with calcium imaging data obtained by measuring the activity patterns of those odours in either the sensory neurons or the projection neurons at the antennal lobe. Our interpretation of the results is that the odours perceptual similarity is organized by antennal lobe interneurons. In another project I investigate the effect of gustatory stimuli on reflexive behaviour as well as their role as reinforcer in larval learning. Drosophila larvae greatly alter their behaviour in presence of sodium chloride. Increasing salt concentration modulates choice behaviour from weakly appetitive to strongly aversive. A similar concentration-behaviour function is also found for feeding: larval feeding is slightly enhanced in presence of low salt concentrations, and strongly decreased in the presence of high salt concentrations. Regarding learning, relatively weak salt concentrations function as appetitive reinforcer, whereas high salt concentrations function as aversive reinforcer. Interestingly, the behaviour-concentration curves are shifted towards higher concentrations from reflexive behaviour (choice behaviour, feeding) as compared to associative learning. This dissociation may reflect a different sensitivity in the respective sensory-motor circuitry.},
  subject      = {Taufliege},
  language  = {en}
}
@phdthesis{Ng2001,
  author    = {Ng, Eva Yee Wah},
  title     = {How did Listeria monocytogenes become pathogenic?},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-1752},
  school      = {Universit{\"a}t W{\"u}rzburg},
  year      = {2001},
  abstract  = {Listeriae are Gram positive, facultative, saprophytic bacteria capable of causing opportunistic infections in humans and animals. This thesis presents three separate lines of inquiries that can lead to the eventual convergence of a global view of Listeria as pathogen in the light of evolution, genomics, and function. First, we undertook to resolve the phylogeny of the genus Listeria with the goal of ascertaining insights into the evolution of pathogenic capability of its members. The phylogeny of Listeriae had not yet been clearly resolved due to a scarcity of phylogenetically informative characters within the 16S and 23S rRNA molecules. The genus Listeria contains six species: L. monocytogenes, L. ivanovii, L. innocua, L. seeligeri, L. welshimeri, and L. grayi; of these, L. monocytogenes and L. ivanovii are pathogenic. Pathogenicity is enabled by a 10-15Kb virulence gene cluster found in L. seeligeri, L. monocytogenes and L. ivanovii. The genetic contents of the virulence gene cluster loci, as well as some virulence-associated internalin loci were compared among the six species. Phylogenetic analysis based on a data set of nucleic acid sequences from prs, ldh, vclA, vclB, iap, 16S and 23S rRNA genes identified L. grayi as the ancestral branch of the genus. This is consistent with previous 16S and 23S rRNA findings. The remainder 5 species formed two groupings. One lineage represents L. monocytogenes and L. innocua, while the other contains L. welshimeri, L. ivanovii and L. seeligeri, with L. welshimeri forming the deepest branch within this group. Deletion breakpoints of the virulence gene cluster within L. innocua and L. welshimeri support the proposed tree. This implies that the virulence gene cluster was present in the common ancestor of L. monocytogenes, L. innocua, L. ivanovii, L. seeligeri and L. welshimeri; and that pathogenic capability has been lost in two separate events represented by L. innocua and L. welshimeri. Second, we attempted to reconstitute L. innocua of its deleted virulence gene cluster, in its original chromosomal location, from the L. monocytogenes 12 Kb virulence gene cluster. This turned out particularly difficult because of the limits of genetic tools presently available for the organism. The reconstitution was partially successful. The methods and approaches are presented, and all the components necessary to complete the constructs are at hand for both L. innocua and the parallel, positive control of L. monocytogenes mutant deleted of its virulence gene cluster. Third, the sequencing of the entire genome of L. monocytogenes EGDe was undertaken as part of an EU Consortium. Our lab was responsible for 10 per cent of the labor intensive gap-closure and annotation efforts, which I helped coordinate. General information and comparisons with sister species L. innocua and a close Gram positive relative Bacillus subtilis are presented in context. The areas I personally investigated, namely, sigma factors and stationary phase functions, are also presented. L. monocytogenes and L. innocua both possess surprisingly few sigma factors: SigA, SigB, SigH, SigL, and an extra-cytoplasmic function type sigma factor (SigECF). The stationary phase genes of L. monocytogenes is compared to the well-studied, complex, stationary phase networks of B. subtilis. This showed that while genetic competence functions may be operative in unknown circumstances, non-sporulating Listeria opted for very different approaches of regulation from B. subtilis. There is virtually no overlap of known, stationary phase genes between Listeria and Gram negative model organism E. coli.},
  subject      = {Listeria monocytogenes},
  language  = {en}
}
@phdthesis{Motsch2005,
  author    = {Motsch, Isabell},
  title     = {Lamin A and lamin C are differentially dysfunctional in autosomal dominant Emery-Dreifuss muscular dystrophy},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-15360},
  school      = {Universit{\"a}t W{\"u}rzburg},
  year      = {2005},
  abstract  = {Emery-Dreifuss muscular dystrophy (EDMD) is a rare genetic disorder characterised by early contractures of the elbows, Achilles tendons and spine, slowly progressive muscle wasting and cardiomyopathy associated with cardiac conduction defect. The autosomal dominant form is caused by mutations in the LMNA gene which gives rise to lamin A and lamin C proteins by alternative splicing. These A-type lamins, together with B-type lamins, form the nuclear lamina, a network of intermediate filament proteins underlining the nuclear envelope. In order to ascertain the role lamin A and C separately contribute to the molecular phenotype, we analysed ten LMNA mutations and one single nucleotide polymorphism (SNP) in transfection studies in COS7 fibroblasts and, partially, in C2C12 myoblasts. The EGFP or DsRed2 tagged lamins were exogenously expressed either individually or both A-types together and examined by light and electron microscopy. The protein mobility of lamin A mutants was determined by FRAP analysis. Additionally, a co-immunoprecipitation binding assay of in vitro synthesised A-type lamins and emerin was performed.Eight of the LMNA mutations (R50S, R133P, E358K, E358K+C<T1698, E361K, R527P, L530P, R541S and G602S) and the SNP C<T1698, when expressed in lamin A, exhibited a range of nuclear mis-localisation patterns from a wild type phenotype to the formation of nuclear aggregates. Two mutations (T150P and delQ355) led to the severe mis-localisation of the exogenous protein and additionally affected nuclear envelope reassembly and mid-body protein composition after mitosis. Exogenously expressed DsRed2 tagged wild type and mutant lamin C was only inserted into the nuclear lamina if co-expressed with the equivalent EGFP tagged lamin A construct, except for the T150P mutation which prevented either lamin from reaching the nuclear lamina. The T150P, R527P and L530P mutations reduced the ability of lamin A, but not lamin C from binding to emerin. These data indicate that mutations in the rod domain of lamin A mainly impair its function as a structural protein, whereas mutations of the globular tail domain appear to disrupt protein-protein interactions important for gene regulation and signal transduction processes. In addition, our results suggest specific functional roles for the emerin-lamin A and emerin-lamin C containing protein complexes; this is the first report to propose that the A-type lamin mutations may be differentially dysfunctional for the same LMNA mutation.},
  subject      = {Muskeldystrophie},
  language  = {en}
}
@phdthesis{Mao2006,
  author    = {Mao, Zhengrong},
  title     = {Clonality analysis in B-Cell Chronic Lymphocytic Leukemia (B-CLL) associated with Richter's syndrome},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-20596},
  school      = {Universit{\"a}t W{\"u}rzburg},
  year      = {2006},
  abstract  = {Die chronische lymphatische Leuk{\"a}mie vom B-Zell-Typ (B-CLL) macht ca. 90\% der chronischen lymphatischen Leuk{\"a}mien aus. Der klinische Verlauf der B-CLL ist heterogen, und bei 3-5\% der Patienten kommt es im Verlauf der Erkrankung zu einer Transformation in ein aggressives Lymphom, meist in ein diffuses großzelliges B-Zell-Lymphom (DLBCL) oder in ein Hodgkin-Lymphom (HL). Eine solche Transformation wird als Richter-Syndrom bezeichnet und ist mit einer ung{\"u}nstigen klinischen Prognose assoziiert. In B-Zell-Lymphomen (B-NHL) erm{\"o}glicht der Mutationsstatus der variablen Anteile der Immunglobulinschwerkettengene (IgVH) eine Aussage {\"u}ber das Entwicklungsstadium der B-Zelle, in dem sich die Transformation zu einem B-Zell-Lymphom ereignet hat. In der B-CLL stellt der Mutationsstatus auch einen bedeutenden prognostischen Faktor dar, wobei die Erkrankung bei Patienten mit unmutierten IgVH Genen meist einen ung{\"u}nstigen klinischen Verlauf zeigt. Die wenigen bisher durchgef{\"u}hrten molekularen Analysen an F{\"a}llen von Richter-Syndromen deuten darauf hin, dass ein Transformationsereignis sowohl bei B-CLL-Patienten mit mutierten als auch mit unmutierten IgVH Genen vorkommen kann, und dass die Tumorzellen des DLBCL oder HL sowohl klonal identisch mit dem B-CLL-Klon sein k{\"o}nnen als auch unabh{\"a}ngig als sekund{\"a}res Lymphom entstehen k{\"o}nnen. Um die klonale Beziehung zwischen DLBCL- bzw. Hodgkin/Reed-Sternberg (HRS)-Zellen und den Zellen der vorbestehenden B-CLL zu analysieren, den Mutationsstatus des IgVH Gens sowie m{\"o}gliche prognostische Faktoren in B-CLL-F{\"a}llen mit Richter-Transformation zu identifizieren, wurde eine gr{\"o}ßere Fallserie mit Hilfe eines PCR-basierten GeneScan Ansatzes mit anschließender Sequenzierung der IgVH-Gene untersucht. In F{\"a}llen mit HRS bzw. HRS-{\"a}hnlichen Zellen wurden die CD30-positiven Tumorzellen mittels Laser-Capture Mikrodissektion (LCM) isoliert. Weiterhin erfolgte eine morphologische und immunhistochemische Analyse der F{\"a}lle. Insgesamt wurden 48 Patientenproben untersucht, darunter 40 F{\"a}lle mit Richter-Syndrom sowie weitere 8 B-CLL-F{\"a}lle mit CD30-positiven HRS-{\"a}hnlichen Zellen. Unter den 40 Proben mit Richter-Syndrom zeigten 34 B-CLL-F{\"a}lle eine Transformation in ein DLBCL, in 6 F{\"a}llen erfolgte eine Transformation in ein HL. In 23 F{\"a}llen mit B-CLL und DLBCL wurde eine Sequenzierung der IgVH Gene durchgef{\"u}hrt. In 18 F{\"a}llen waren B-CLL und DLBCL klonal identisch, in 5 F{\"a}llen war das DLBCL als klonal unabh{\"a}ngige Neoplasie entstanden. Unter den klonal verwandten Paaren zeigten 11 von 15 Paaren unmutierte IgVH-Gene sowohl in der B-CLL als auch im DLBCL, wohingegen 5 von 6 F{\"a}lle mit Transformation einer B-CLL in ein HL mutierte IgVH Gene trugen. HRS-Zellen in 2 F{\"a}llen und HRS-{\"a}hnliche Zellen in einem Fall waren klonal verschieden vom B-CLL-Zellklon. Die VH-Gene VH3-23, VH3-74, VH1-2 und VH3-9 waren {\"u}berproportional h{\"a}ufig in B-CLL F{\"a}llen mit einer sp{\"a}teren Transformation in ein DLBCL vertreten, wohingegen VH4-34 und VH3-48 in mehr als der H{\"a}lfte der F{\"a}lle mit Transformation zu einem HL nachgewiesen werden konnten. Der immunhistochemische Nachweis von ZAP70 zeigte eine signifikante Assoziation mit unmutierten IgVH-Genen in B-CLL mit nachfolgender Richter-Transformation. Bei 24 Patienten konnte der klinische Verlauf eruiert werden. Die mediane {\"U}berlebenszeit von Patienten mit B-CLL mit stattgehabter Transformation in ein DLBCL oder ein HL betrug 7 beziehungsweise 21 Monate. Es fanden sich weder signifikante Unterschiede der {\"U}berlebenszeit zwischen klonal verwandten und nicht verwandten F{\"a}llen, noch zwischen IgVH-mutierten und -unmutierten F{\"a}llen. Zusammenfassend kann festgestellt werden, dass bei der Richter-Transformation einer B-CLL in ein DLBCL dieses einerseits aus dem pr{\"a}existenten B-CLL-Klon entstehen kann, andererseits aber auch als unabh{\"a}ngige, klonal nicht verwandte Neoplasie auftreten kann. In der Mehrzahl der F{\"a}lle (78\% in dieser Serie) sind B-CLL und DLBCL jedoch klonal identisch und nur gelegentlich entsteht ein DLBCL ohne klonale Beziehung zur B-CLL als unabh{\"a}ngige, sekund{\"a}re Neoplasie. Eine klonale Transformation in ein DLBCL tritt vorwiegend bei B-CLL-Patienten mit unmutierten IgVH-Genen auf, wohingegen die Mehrzahl der B-CLL-Patienten mit einer Transformation in ein HL oder CD30-positive HRS-{\"a}hnliche Zellen mutierte IgVH-Gene aufweist. Dieser Befund l{\"a}sst auf unterschiedliche Transformationswege der beiden Subtypen des Richter-Syndroms schließen. Weiterhin existieren vermutlich wesentliche Unterschiede in der Pathogenese zwischen DLBCL-F{\"a}llen, die sich aus einer vorbestehenden B-CLL entwickelt haben, und de novo DLBCL-F{\"a}llen, da de novo DLBCL zumeist durch mutierte IgVH-Gene charakterisiert sind.},
  subject      = {B-Zell-Leuk{\"a}mie},
  language  = {en}
}
@phdthesis{FadlElMola2003,
  author    = {Fadl El Mola, Faisal Mohamed},
  title     = {Bioinformatic and molecular approaches for the analysis of the retinal pigment epithelium (RPE) transcriptome},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-6877},
  school      = {Universit{\"a}t W{\"u}rzburg},
  year      = {2003},
  abstract  = {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.},
  subject      = {Senile Makuladegeneration},
  language  = {en}
}
@phdthesis{Fackler2014,
  author    = {Fackler, Marc},
  title     = {Biochemical characterization of GAS2L3, a target gene of the DREAM complex},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-103394},
  school      = {Universit{\"a}t W{\"u}rzburg},
  year      = {2014},
  abstract  = {GAS2L3 was identified recently as a target gene of the DREAM complex (Reichert et al., 2010; Wolter et al., 2012). It was shown that GAS2L3 is expressed in a cell cycle specific manner and that depletion of the protein leads to defects in cytokinesis and genomic instability (Wolter et al., 2012). Major aim of this thesis was, to further characterize the biochemical properties and physiological function of GAS2L3. By in vitro co-sedimentation and bundling assays, GAS2L3 was identified as a cytoskeleton associated protein which bundles, binds and crosslinks F-actin and MTs. GST pulldown assays and co-immunoprecipitation experiments revealed that GAS2L3 interacts in vitro and in vivo with the chromosomal passenger complex (CPC), a very important regulator of mitosis and cytokinesis, and that the interaction is mediated by the GAR domain of GAS2L3 and the C-terminal part of Borealin and the N-terminal part of Survivin. Kinase assays showed that GAS2L3 is not a substrate of the CPC but is strongly phosphorylated by CDK1 in vitro. Depletion of GAS2L3 by shRNA influenced protein stability and activity of the CPC. However pharmacological studies showed that the decreased CPC activity is not responsible for the observed cytokinesis defects upon GAS2L3 depletion. Immunofluorescence experiments revealed that GAS2L3 is localized to the constriction zone by the CPC in a GAR dependent manner and that the GAR domain is important for proper protein function. New interacting proteins of GAS2L3 were identified by stable isotope labelling by amino acids in cell culture (SILAC) in combination with tandem affinity purification and subsequent mass spectrometrical analysis. Co-immunoprecipitation experiments further confirmed the obtained mass spectrometrical data. To address the physiological function of GAS2L3 in vivo, a conditional and a non-conditional knockout mouse strain was established. The non-conditional mouse strain showed a highly increased mortality rate before weaning age probably due to heart failure. The physiological function of GAS2L3 in vivo as well as the exact reason for the observed heart phenotype is not known at the moment.},
  subject      = {Zellzyklus},
  language  = {en}
}
@phdthesis{Cruz2006,
  author    = {Cruz, Alexandre Bettencourt da},
  title     = {Molecular and functional characterization of the swiss-cheese and olk mutants in Drosophila melanogaster : two approaches to killing neurons},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-17734},
  school      = {Universit{\"a}t W{\"u}rzburg},
  year      = {2006},
  abstract  = {In this thesis two genes involved in causing neurodegenerative phenotypes in Drosophila are described. olk (omb-like), a futsch allele, is a micotubule associated protein (MAP) which is homologous to MAP1B and sws (swiss cheese) a serine esterase of yet unknown function within the nervous system. The lack of either one of these genes causes progressive neurodegeneration in two different ways. The sws mutant is characterized by general degeneration of the adult nervous system, glial hyperwrapping and neuronal apoptosis. Deletion of NTE (neuropathy target esterase), the SWS homolog in vertebrates, has been shown to cause a similar pattern of progressive neural degeneration in mice. NTE reacts with organophosphates causing axonal degeneration in humans. Inhibition of vertebrate NTE is insufficient to induce paralyzing axonal degeneration, a reaction called "aging reaction" is necessary for the disease to set in. It is hypothesized that a second "non-esterase" function of NTE is responsible for this phenomenon. The biological function of SWS within the nervous system is still unknown. To characterize the function of this protein several transgenic fly lines expressing different mutated forms of SWS were established. The controlled expression of altered SWS protein with the GAL4/UAS system allowed the analysis of isolated parts of the protein that were altered in the respective constructs. The characterization of a possible non-esterase function was of particular interest in these experiments. One previously described aberrant SWS construct lacking the first 80 amino acids (SWS\&\#916;1-80) showed a deleterious, dominant effect when overexpressed and was used as a model for organophosphate (OP) intoxication. This construct retains part of its detrimental effect even without catalytically active serine esterase function. This strongly suggests that there is another characteristic to SWS that is not defined solely by its serine esterase activity. Experiments analyzing the lipid contents of sws mutant, wildtype (wt) and SWS overexpressing flies gave valuable insights into a possible biological function of SWS. Phosphatidylcholine, a major component of cell membranes, accumulates in sws mutants whereas it is depleted in SWS overexpressing flies. This suggests that SWS is involved in phosphatidylcholine regulation. The produced \&\#945;-SWS antibody made it possible to study the intracellular localization of SWS. Images of double stainings with ER (endoplasmic reticulum) markers show that SWS is in great part localized to the ER. This is consistent with findings of SWS/ NTE localization in yeast and mouse cells. The olk mutant also shows progressive neurodegeneration but it is more localized to the olfactory system and mushroom bodies. Regarding specific cell types it seemed that specifically the projection neurons (PNs) are affected. A behavioral phenotype consisting of poor olfactory memory compared to wt is also observed even before histologically visible neurodegeneration sets in. Considering that the projection neurons connect the antennal lobes to the mushroom bodies, widely regarded as the "learning center", this impairment was expected. Three mutants where identified (olk1-3) by complementation analysis with the previously known futschN94 allele and sequencing of the coding sequence of olk1 revealed a nonsense mutation early in the protein. Consistent with the predicted function of Futsch as a microtubule associated protein (MAP), abnormalities are most likely due to a defective microtubule network and defects in axonal transport. In histological sections a modified cytoskeletal network is observed and western blots confirm a difference in the amount of tubulin present in the olk1 mutant versus the wt. The elaboration of neuronal axons and dendrites is dependent on a functional cytoskeleton. Observation of transport processes in primary neural cultures derived from olk1 mutant flies also showed a reduction of mitochondrial transport. Interaction with the fragile X mental retardation gene (dfmr1) was observed with the olk mutant. A dfmr1/ olk1 double mutant shows an ameliorated phenotype compared to the olk1 single mutant. tau, another MAP gene, was also shown to be able to partially rescue the olk1 mutant.},
  subject      = {Taufliege},
  language  = {en}
}