@phdthesis{Riemensperger2006, author = {Riemensperger, Thomas}, title = {Untersuchung pr{\"a}diktiver Eigenschaften des dopaminergen Systems von Drosophila melanogaster mittels genetisch kodierter Calcium Sensoren}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-19041}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2006}, abstract = {Die Technik des optischen Imaging unter Verwendung DNA-codierter Sensoren erm{\"o}glicht es, Messungen neuraler Aktivit{\"a}ten in genetisch definierten Populationen von Neuronen durchzuf{\"u}hren. In der Vielzahl der verschiedenen entwickelten Sensoren konnten die Calciumsensoren bisher das beste Verh{\"a}ltnis zwischen Signal und Rauschen und die beste zeitliche Aufl{\"o}sung aufzeigen. Hierbei handelt es sich in erster Linie um zwei Typen von Sensoren, zum einen ratiometrische Sensoren, deren Signal auf einem Fluoreszenz Resonanz Energie Transfer (FRET) basiert, und zum anderen um zirkul{\"a}r permutierte Sensoren, die auf einem modifizierten GFP-Molek{\"u}l basieren, wobei das Signal auf einer ver{\"a}nderten Protonierung des Chromophors beruht. Beide Arten dieser Sensoren wurden schon erfolgreich zum Messen neuraler Aktivit{\"a}ten in Nervensystemen verschiedener Tierarten verwendet. Ein Teil dieser Arbeit bestand darin, zu untersuchen, welche Sensoren sich f{\"u}r die Messung an einem lebenden Organismus am besten eignen. Hierf{\"u}r wurden die Eigenschaften von vier verschiedenen FRET basierten Sensoren und zwei der zyklisch permutierten Sensoren nach Expression im zentralen Nervensystem von Drosophila charakterisiert. Die Sensoren wurden in Neuronen zweiter und dritter Ordnung des olfaktorischen Signalwegs exprimiert und ihre Antworten auf physiologische Duftstimulation oder artifiziell induzierte Depolarisation des Gehirns untersucht. W{\"a}hrend die calciumabh{\"a}ngigen Signale der zyklisch permutierten Sensoren in der Regel gr{\"o}ßer waren als die der FRET basierten Sensoren, zeichneten sich letztere durch ein besseres Signal zu Rausch-Verh{\"a}ltnis aus, wenn Bewegungen der fluoreszierenden Strukturen nicht zu vermeiden waren. Dies war auch der ausschlaggebende Grund f{\"u}r die Verwendung eines FRET basierten Sensors im anschließenden Teil der Arbeit. Im zweiten Teil der Arbeit wurde der Effekt untersucht, den die Paarung eines neutralen Stimulus mit einem bestrafenden Stimulus auf dopaminerge Neurone hat. Eine solche Paarung kann zu einer klassischen Konditionierung f{\"u}hren, einer einfachen Form des Lernens, in welcher das Tier einem urspr{\"u}nglich neutralen Stimulus einen Wert zuordnet, und dadurch sein Verhalten dem Stimulus gegen{\"u}ber {\"a}ndert. Die olfaktorische klassische Konditionierung in Drosophila wird seit vielen Jahren intensiv untersucht, um die molekularen und neuronalen Grundlagen von Lernen und Ged{\"a}chtnis zu charakterisieren. Dabei hat sich gezeigt, dass besonders die Pilzk{\"o}rper von essentieller Bedeutung f{\"u}r die Ausbildung eines olfaktorischen Ged{\"a}chtnisses sind. W{\"a}hrend das olfactorische System bei Insekten bereits detailiert analysiert wurde, ist {\"u}ber die Neurone, die den bestrafenden Stimulus vermitteln, nur sehr wenig bekannt. Unter Anwendung des funktionellen optischen Calcium Imaging konnte im Rahmen der Arbeit gezeigt werden, dass die Projektionen von dopaminergen Neuronen im Bereich der Loben der Pilzk{\"o}rper schwach auf die Pr{\"a}sentation eines Duftes, jedoch sehr stark auf eine Stimulation durch einen Elektroschock antworten. Nach mehrmaliger Paarung eines Duftes mit einem Elektroschock w{\"a}hrend eines Trainings, verl{\"a}ngert sich die Aktivit{\"a}t dieser dopaminergen Neurone auf den bestraften Duft hin im Test ohne Elektroschock drastisch, w{\"a}hrend die Antwort auf den Kontrollduft keine signifikanten Ver{\"a}nderungen aufweist. W{\"a}hrend bei S{\"a}ugetieren belohnende Reize bei appetitiven Lernvorg{\"a}ngen {\"u}ber dopaminerge Neurone vermittelt werden, spielen bei Drosophila diese Neurone offensichtlich eine Rolle bei der aversiven Konditionierung. Jedoch blieb, auch wenn sich die Rolle des Dopamins im Laufe der Evolution ge{\"a}ndert zu haben scheint, die F{\"a}higkeit dieses Neuronentyps, nicht nur auf einen eintreffenden verst{\"a}rkenden Stimulus zu reagieren, sondern diesen auch vorhersagen zu k{\"o}nnen, zwischen S{\"a}ugern und Drosophila erhalten.}, subject = {Taufliege}, language = {de} } @phdthesis{Rister2008, author = {Rister, Jens}, title = {Genetic dissection of peripheral pathways in the visual system of Drosophila}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-25980}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2008}, abstract = {Die visuellen Systeme von Vertebraten und Invertebraten weisen {\"A}hnlichkeiten in den ersten Schritten visueller Informationsverarbeitung auf. Im menschlichen Gehirn werden zum Beispiel die Modalit{\"a}ten Farbe, Form und Bewegung separat in parallelen neuronalen Pfaden verarbeitet. Dieses grundlegende Merkmal findet sich auch bei der Fliege Drosophila melanogaster, welche eine {\"a}hnliche Trennung in farbsensitive und (farbenblinde) bewegungssensitive Pfade aufweist, die durch zwei verschiedene Gruppen von Photorezeptoren (dem R1-6 und dem R7/8 System) determiniert werden. Fliegen haben ein hoch organisiertes visuelles System, welches durch die repetitive, retinotope Organisation von vier Neuropilen charakterisiert ist: Dies sind die Lamina, die Medulla, die Lobula und die Lobulaplatte. Jedes einzelne besteht aus Kolumnen, die denselben Satz von Nervenzellen enthalten. In der Lamina formen Axonb{\"u}ndel von sechs Photorezeptoren R1-6, die auf denselben Bildpunkt blicken, S{\"a}ulen, die als Cartridges bezeichnet werden. Diese sind die funktionellen visuellen „sampling units" und sind mit vier Typen von Interneuronen erster Ordnung assoziiert, die von R1-6 den gleichen Input erhalten: L1, L2, L3 und die Amakrinzellen (amc, mit ihrem postsynaptischen Partner T1). Diese stellen parallele Pfade dar, die auf anatomischer Ebene im Detail untersucht wurden; jedoch ist wenig {\"u}ber ihre funktionelle Rolle bei der Verarbeitung f{\"u}r das Verhalten relevanter Information bekannt, z.B. hinsichtlich der Blickstabilisierung, der visuellen Kurskontrolle oder der Fixation von Objekten. Die Verf{\"u}gbarkeit einer Vielfalt von neurogenetischen Werkzeugen f{\"u}r die Struktur-Funktionsanalyse bei Drosophila erm{\"o}glicht es, erste Schritte in Richtung einer genetischen Zerlegung des visuellen Netzwerks zu unternehmen, das Bewegungs- und Positionssehen vermittelt. In diesem Zusammenhang erwies sich die Wahl des Effektors als entscheidend. {\"U}berraschenderweise wurde festgestellt, dass das clostridiale Tetanus-Neurotoxin die Photorezeptorsynapsen adulter Drosophila Fliegen nicht blockiert, hingegen irreversible Sch{\"a}den bei Expression w{\"a}hrend deren Entwicklung verursacht. Aus diesem Grund wurde das dominant-negative shibire Allel shits1, welches sich als geeigneter erwies, zur Blockierung der Lamina Interneurone verwendet, um die Notwendigkeit der jeweiligen Pfade zu analysieren. Um festzustellen, ob letztere auch hinreichend f{\"u}r das gleiche Verhalten waren, wurde f{\"u}r die umgekehrte Strategie die Tatsache ausgenutzt, daß die Lamina Interneurone Histaminrezeptoren exprimieren, die vom ort Gen kodiert werden. Die spezifische Rettung der ort Funktion in definierten Pfaden im mutanten Hintergrund erm{\"o}glichte festzustellen, ob sie f{\"u}r eine bestimmte Funktion hinreichend waren. Diese neurogenetischen Methoden wurden mit der optomotorischen Reaktion und dem objektinduzierten Orientierungsverhalten als Verhaltensmaß kombiniert, um folgende Fragen innerhalb dieser Doktorarbeit zu beantworten: (a) Welche Pfade stellen einen Eingang in elementare Bewegungsdetektoren dar und sind notwendig und/oder hinreichend f{\"u}r die Detektion gerichteter Bewegung? (b) Gibt es Pfade, die spezifisch Reaktionen auf unidirektionale Bewegung vermitteln? (c) Welche Pfade sind notwendig und/oder hinreichend f{\"u}r das objektinduzierte Orientierungsverhalten? Einige grundlegende Eigenschaften des visuellen Netzwerks konnten dabei aufgedeckt werden: Die zwei zentralen Cartridge Pfade, die von den großen Monopolarzellen L1 und L2 repr{\"a}sentiert werden, haben eine Schl{\"u}sselfunktion bei der Bewegungsdetektion. {\"U}ber ein breites Spektrum von Reizbedingungen hinweg sind die beiden Subsysteme redundant und k{\"o}nnen Bewegung unabh{\"a}ngig voneinander verarbeiten. Um eine Beeintr{\"a}chtigung des Systems festzustellen, wenn nur einer der beiden Pfade intakt ist, muß dieses an die Grenzen seiner Leistungsf{\"a}higkeit gebracht werden. Bei niedrigem Signal/Rauschverh{\"a}ltnis, d.h. bei geringem Musterkontrast oder geringer Hintergrundbeleuchtung, hat der L2 Pfad eine h{\"o}here Sensitivit{\"a}t. Bei mittlerem Musterkontrast sind beide Pfade auf die Verarbeitung unidirektionaler Bewegung in entgegengesetzten Reizrichtungen spezialisiert. Im Gegensatz dazu sind weder der L3, noch der amc/T1 Pfad notwendig oder hinreichend f{\"u}r die Detektion von Bewegungen. W{\"a}hrend der erstere Positionsinformation f{\"u}r Orientierungsverhalten zu verarbeiten scheint, nimmt der letztere eine modulatorische Rolle bei mittlerem Kontrast ein. Es stellte sich heraus, daß das Orientierungsverhalten noch robuster als das Bewegungssehen ist und m{\"o}glicherweise auf einem weniger komplizierten Mechanismus beruht, da dieser keinen nichtlinearen Vergleich der Signale benachbarter visueller „sampling units" ben{\"o}tigt. Die Fixation von Objekten setzt nicht grunds{\"a}tzlich das Bewegungssehen voraus, allerdings verbessert die Detektion von Bewegung die Fixation von Landmarken, im besonderen, wenn diese schmal sind oder einen geringen Kontrast aufweisen.}, subject = {Genetik}, language = {en} } @phdthesis{Roth2003, author = {Roth, Martin}, title = {Functional and developmental characterisation of matrix binding sites in decapentaplegic}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-7542}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2003}, abstract = {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.}, subject = {Taufliege}, language = {en} } @phdthesis{Ruf2016, author = {Ruf, Franziska}, title = {The circadian regulation of eclosion in \(Drosophila\) \(melanogaster\)}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-146265}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2016}, abstract = {Eclosion is the emergence of an adult insect from the pupal case at the end of development. In the fruit fly Drosophila melanogaster, eclosion is a circadian clock-gated event and is regulated by various peptides. When studied on the population level, eclosion reveals a clear rhythmicity with a peak at the beginning of the light-phase that persists also under constant conditions. It is a long standing hypothesis that eclosion gating to the morning hours with more humid conditions is an adaption to reduce water loss and increase the survival. Eclosion behavior, including the motor pattern required for the fly to hatch out of the puparium, is orchestrated by a well-characterized cascade of peptides. The main components are ecdysis-triggering hormone (ETH), eclosion hormone (EH) and crustacean cardioactive peptide (CCAP). The molt is initiated by a peak level and pupal ecdysis by a subsequent decline of the ecdysteroid ecdysone. Ecdysteroids are produced by the prothoracic gland (PG), an endocrine tissue that contains a peripheral clock and degenerates shortly after eclosion. Production and release of ecdysteroids are regulated by the prothoracicotropic hormone (PTTH). Although many aspects of the circadian clock and the peptidergic control of the eclosion behavior are known, it still remains unclear how both systems are interconnected. The aim of this dissertation research was to dissect this connection and evaluate the importance of different Zeitgebers on eclosion rhythmicity under natural conditions. Potential interactions between the central clock and the peptides regulating ecdysis motor behavior were evaluated by analyzing the influence of CCAP on eclosion rhythmicity. Ablation and silencing of CCAP neurons, as well as CCAP null-mutation did not affect eclosion rhythmicity under either light or temperature entrainment nor under natural conditions. To dissect the connection between the central and the peripheral clock, PTTH neurons were ablated. Monitoring eclosion under light and temperature entrainment revealed that eclosion became arrhythmic under constant conditions. However, qPCR expression analysis revealed no evidence for cycling of Ptth mRNA in pharate flies. To test for a connection with pigment-dispersing factor (PDF)-expressing neurons, the PDF receptor (PDFR) and short neuropeptide F receptor (sNPFR) were knocked down in the PTTH neurons. Knockdown of sNPFR, but not PDFR, resulted in arrhythmic eclosion under constant darkness conditions. PCR analysis of the PTTH receptor, Torso, revealed its expression in the PG and the gonads, but not in the brain or eyes, of pharate flies. Knockdown of torso in the PG lead to arrhythmicity under constant conditions, which provides strong evidence for the specific effect of PTTH on the PG. These results suggest connections from the PDF positive lateral neurons to the PTTH neurons via sNPF signaling, and to the PG via PTTH and Torso. This interaction presumably couples the period of the peripheral clock in the PG to that of the central clock in the brain. To identify a starting signal for eclosion and possible further candidates in the regulation of eclosion behavior, chemically defined peptidergic and aminergic neurons were optogenetically activated in pharate pupae via ChR2-XXL. This screen approach revealed two candidates for the regulation of eclosion behavior: Dromyosuppressin (DMS) and myo-inhibitory peptides (MIP). However, ablation of DMS neurons did not affect eclosion rhythmicity or success and the exact function of MIP must be evaluated in future studies. To assess the importance of the clock and of possible Zeitgebers in nature, eclosion of the wildtype Canton S and the clock mutant per01 and the PDF signaling mutants pdf01 and han5304 was monitored under natural conditions. For this purpose, the W{\"u}rzburg eclosion monitor (WEclMon) was developed, which is a new open monitoring system that allows direct exposure of pupae to the environment. A general decline of rhythmicity under natural conditions compared to laboratory conditions was observed in all tested strains. While the wildtype and the pdf01 and han5304 mutants stayed weakly rhythmic, the per01 mutant flies eclosed mostly arrhythmic. PDF and its receptor (PDFR encoded by han) are required for the synchronization of the clock network and functional loss can obviously be compensated by a persisting synchronization to external Zeitgebers. The loss of the central clock protein PER, however, lead to a non-functional clock and revealed the absolute importance of the clock for eclosion rhythmicity. To quantitatively analyze the effect of the clock and abiotic factors on eclosion rhythmicity, a statistical model was developed in cooperation with Oliver Mitesser and Thomas Hovestadt. The modelling results confirmed the clock as the most important factor for eclosion rhythmicity. Moreover, temperature was found to have the strongest effect on the actual shape of the daily emergence pattern, while light has only minor effects. Relative humidity could be excluded as Zeitgeber for eclosion and therefore was not further analyzed. Taken together, the present dissertation identified the so far unknown connection between the central and peripheral clock regulating eclosion. Furthermore, a new method for the analysis of eclosion rhythms under natural conditions was established and the necessity of a functional clock for rhythmic eclosion even in the presence of multiple Zeitgebers was shown.}, subject = {Taufliege}, language = {en} } @phdthesis{Saumweber2011, author = {Saumweber, Timo}, title = {Mechanism of Learning and Plasticity in Larval Drosophila}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-66354}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2011}, abstract = {According to a changing environment it is crucial for animals to make experience and learn about it. Sensing, integrating and learning to associate different kinds of modalities enables animals to expect future events and to adjust behavior in the way, expected as the most profitable. Complex processes as memory formation and storage make it necessary to investigate learning and memory on different levels. In this context Drosophila melanogaster represents a powerful model organism. As the adult brain of the fly is still quite complex, I chose the third instar larva as model - the more simple the system, the easier to isolate single, fundamental principles of learning. In this thesis I addressed several kinds of questions on different mechanism of olfactory associative and synaptic plasiticity in Drosophila larvae. I focused on short-term memory throughout my thesis. First, investigating larval learning on behavioral level, I developed a one-odor paradigm for olfactory associative conditioning. This enables to estimate the learnability of single odors, reduces the complexity of the task and simplify analyses of "learning mutants". It further allows to balance learnability of odors for generalization-type experiments to describe the olfactory "coding space". Furthermore I could show that innate attractiveness and learnability can be dissociated and found finally that paired presentation of a given odor with reward increase performance, whereas unpaired presentations of these two stimuli decrease performance, indicating that larva are able to learn about the presence as well as about the absence of a reward. Second, on behavioral level, together with Thomas Niewalda and colleagues we focussed on salt processing in the context of choice, feeding and learning. Salt is required in several physiological processes, but can neither be synthesized nor stored. Various salt concentrations shift the valence from attraction to repulsion in reflexive behaviour. Interestingly, the reinforcing effect of salt in learning is shifted by more than one order of magnitude toward higher concentrations. Thus, the input pathways for gustatory behavior appear to be more sensitive than the ones supporting gustatory reinforcement, which is may be due to the dissociation of the reflexive and the reinforcing signalling pathways of salt. Third, in cooperation with Michael Schleyer we performed a series of behavioral gustatory, olfactory preference tests and larval learning experiments. Based on the available neuroanatomical and behavioral data we propose a model regarding chemosensory processing, odor-tastant memory trace formation and the 'decision' like process. It incorporates putative sites of interaction between olfactory and gustatory pathways during the establishment as well as behavioral expression of odor-tastant memory. We claim that innate olfactory behavior is responsive in nature and suggest that associative conditioned behavior is not a simple substitution like process, but driven more likely by the expectation of its outcome. Fourth, together with Birgit Michels and colleagues we investigated the cellular site and molecular mode of Synapsin, an evolutionarily conserved, presynaptic vesicular phosphoprotein and its action in larval learning. We confirmed a previously described learning impairment upon loss of Synapsin. We localized this Synapsin dependent memory trace in the mushroom bodies, a third-order "cortical" brain region, and could further show on molecular level, that Synapsin is as a downstream element of the AC-cAMP-PKA signalling cascade. This study provides a comprehensive chain of explanation from the molecular level to an associative behavioral change. Fifth, in the main part of my thesis I focused on molecular level on another synaptic protein, the Synapse associated protein of 47kDa (Sap47) and its role in larval behavior. As a member of a phylogenetically conserved gene family of hitherto unknown function. It is localized throughout the whole neuropil of larval brains and associated with presynaptic vesicles. Upon loss of Sap47 larvae exhibit normal sensory detection of the to-be-associated stimuli as well as normal motor performance and basic synaptic transmission. Interestingly, short-term plasticity is distorted and odorant-tastant associative learning ability is reduced. This defect in associative function could be rescued by restoring Sap47 expression. Therefore, this report is the first to suggest a function for Sap47 and specifically argues that Sap47 is required for synaptic as well as for behavioral plasticity in Drosophila larva. This prompts the question whether its homologs are required for synaptic and behavioral plasticity also in other species. Further in the last part of my thesis I contributed to the study of Ayse Yarali. Her central topic was the role of the White protein in punishment and relief learning in adult flies. Whereas stimuli that precede shock during training are subsequently avoided as predictors for punishment, stimuli that follow shock during training are later on approached, as they predict relief. Concerning the loss of White we report that pain-relief learning as well as punishment learning is changed. My contribution was a comparison between wild type and the white1118 mutant larvae in odor-reward learning. It turned out that a loss of White has no effect on larval odorant-tastant learning. This study, regarding painrelief learning provides the very first hints concerning the genetic determinants of this form of learning.}, subject = {Taufliege}, language = {en} } @phdthesis{Schindelin2005, author = {Schindelin, Johannes}, title = {The standard brain of Drosophila melanogaster and its automatic segmentation}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-15518}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2005}, abstract = {In this thesis, I introduce the Virtual Brain Protocol, which facilitates applications of the Standard Brain of Drosophila melanogaster. By providing reliable and extensible tools for the handling of neuroanatomical data, this protocol simplifies and organizes the recurring tasks involved in these applications. It is demonstrated that this protocol can also be used to generate average brains, i.e. to combine recordings of several brains with the same features such that the common features are emphasized. One of the most important steps of the Virtual Insect Protocol is the aligning of newly recorded data sets with the Standard Brain. After presenting methods commonly applied in a biological or medical context to align two different recordings, it is evaluated to what extent this alignment can be automated. To that end, existing Image Processing techniques are assessed. I demonstrate that these techniques do not satisfy the requirements needed to guarantee sensible alignments between two brains. Then, I analyze what needs to be taken into account in order to formulate an algorithm which satisfies the needs of the protocol. In the last chapter, I derive such an algorithm using methods from Information Theory, which bases the technique on a solid mathematical foundation. I show how Bayesian Inference can be applied to enhance the results further. It is demonstrated that this approach yields good results on very noisy images, detecting apparent boundaries between structures. The same approach can be extended to take additional knowledge into account, e.g. the relative position of the anatomical structures and their shape. It is shown how this extension can be utilized to segment a newly recorded brain automatically.}, subject = {Taufliege}, language = {en} } @phdthesis{Schleyer2012, author = {Schleyer, Michael}, title = {Integrating past, present and future: mechanisms of a simple decision in larval Drosophila}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-78923}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2012}, abstract = {Is behaviour response or action? In this Thesis I study this question regarding a rather simple organism, the larva of the fruit fly Drosophila melanogaster. Despite its numerically simple brain and limited behavioural repertoire, it is nevertheless capable to accomplish surprisingly complex tasks. After association of an odour and a rewarding or punishing reinforcement signal, the learnt odour is able to retrieve the formed memory trace. However, the activated memory trace is not automatically turned into learned behaviour: Appetitive memory traces are behaviourally expressed only in absence of the rewarding tastant whereas aversive memory traces are behaviourally expressed in the presence of the punishing tastant. The 'decision' whether to behaviourally express a memory trace or not relies on a quantitive comparison between memory trace and current situation: only if the memory trace (after odour-sugar training) predicts a stronger sugar reward than currently present, animals show appetitive conditioned behaviour. Learned appetitive behaviour is best seen as active search for food - being pointless in the presence of (enough) food. Learned aversive behaviour, in turn, can be seen as escape from a punishment - being pointless in absence of punishment. Importantly, appetitive and aversive memory traces can be formed and retrieved independent from each other but also can, under appriate circumstances, summate to jointly organise conditioned behaviour. In contrast to learned behaviour, innate olfactory behaviour is not influenced by gustatory processing and vice versa. Thus, innate olfactory and gustatory behaviour is rather rigid and reflexive in nature, being executed almost regardless of other environmental cues. I suggest a behavioural circuit-model of chemosensory behaviour and the 'decision' process whether to behaviourally express a memory trace or not. This model reflects known components of the larval chemobehavioural circuit and provides clear hypotheses about the kinds of architecture to look for in the currently unknown parts of this circuit. The second chapter deals with gustatory perception and processing (especially of bitter substances). Quinine, the bitter tastant in tonic water and bitter lemon, is aversive for larvae, suppresses feeding behaviour and can act as aversive reinforcer in learning experiments. However, all three examined behaviours differ in their dose-effect dynamics, suggesting different molecular and cellular processing streams at some level. Innate choice behaviour, thought to be relatively reflexive and hard-wired, nevertheless can be influenced by the gustatory context. That is, attraction toward sweet tastants is decreased in presence of bitter tastants. The extent of this inhibitory effect depends on the concentration of both sweet and bitter tastant. Importantly, sweet tastants differ in their sensitivity to bitter interference, indicating a stimulus-specific mechanism. The molecular and cellular processes underlying the inhibitory effect of bitter tastants are unknown, but the behavioural results presented here provide a framework to further investigate interactions of gustatory processing streams.}, subject = {Lernen}, language = {en} } @phdthesis{Schmid2010, author = {Schmid, Benjamin}, title = {Computational tools for the segmentation and registration of confocal brain images of Drosophila melanogaster}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-51490}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2010}, abstract = {Neuroanatomical data in fly brain research are mostly available as spatial gene expression patterns of genetically distinct fly strains. The Drosophila standard brain, which was developed in the past to provide a reference coordinate system, can be used to integrate these data. Working with the standard brain requires advanced image processing methods, including visualisation, segmentation and registration. The previously published VIB Protocol addressed the problem of image registration. Unfortunately, its usage was severely limited by the necessity of manually labelling a predefined set of neuropils in the brain images at hand. In this work I present novel tools to facilitate the work with the Drosophila standard brain. These tools are integrated in a well-known open-source image processing framework which can potentially serve as a common platform for image analysis in the neuroanatomical research community: ImageJ. In particular, a hardware-accelerated 3D visualisation framework was developed for ImageJ which extends its limited 3D visualisation capabilities. It is used for the development of a novel semi-automatic segmentation method, which implements automatic surface growing based on user-provided seed points. Template surfaces, incorporated with a modified variant of an active surface model, complement the segmentation. An automatic nonrigid warping algorithm is applied, based on point correspondences established through the extracted surfaces. Finally, I show how the individual steps can be fully automated, and demonstrate its application for the successful registration of fly brain images. The new tools are freely available as ImageJ plugins. I compare the results obtained by the introduced methods with the output of the VIB Protocol and conclude that our methods reduce the required effort five to ten fold. Furthermore, reproducibility and accuracy are enhanced using the proposed tools.}, subject = {Taufliege}, language = {en} } @phdthesis{Schubert2010, author = {Schubert, Alice}, title = {Immunhistochemische und funktionelle Charakterisierung der Serin/Arginin-Proteinkinase SRPK79D mit Identifizierung von Interaktionspartnern in Drosophila melanogaster}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-53841}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2010}, abstract = {Auf der Suche nach Mutanten mit einer vom Wildtyp abweichenden Verteilung des Aktive Zone-Proteins Bruchpilot wurde die Serin/Arginin-Proteinkinase SRPK79D identifiziert. Hier zeigte sich, dass die Mutation im Srpk79D-Gen zu einer Agglomeration von Bruchpilot in den larvalen segmentalen und intersegmentalen Nerven f{\"u}hrt. In der vorliegenden Arbeit sollte die SRPK79D genauer charakterisiert werden. Nach Pr{\"a}adsorptionen und Affinit{\"a}tsreinigungen von in einer fr{\"u}heren Arbeit erzeugten Antiseren, gelang es die Lokalisation der {\"u}berexprimierten SRPK79D-GFP-Isoformen zu bestimmen. Dabei zeigte sich, dass keines der Antiseren die endogene Kinase im Western Blot oder immunhistocheimisch detektieren konnte. Dies legt den Schluss nahe, dass die Expression der SRPK79D in einer geringen Konzentration erfolgt. Es war jedoch m{\"o}glich die endogene SRPK79D-PC-Isoform mittels einer Immunpr{\"a}zipitation soweit anzureichern, dass sie im Western Blot nachweisbar war. F{\"u}r die SRPK79D-PB-Isoform gelang dies allerdings nicht. Anhand von larvalen Nerv-Muskel-Pr{\"a}paraten konnte gezeigt werden, dass die panneural {\"u}berexprimierte SRPK79D-PC-GFP-Isoform an die Aktiven Zone transportiert wird und dort mit Bruchpilot, sowie den Interaktionspartnern von Bruchpilot Liprin-α und Rab3 kolokalisiert. Außerdem liegt sie diffus im Zytoplasma von neuronalen Zellk{\"o}rpern vor. In adulten Gehirnen lokalisiert die transgen {\"u}berexprimierte SRPK79D-PC-GFP im Fanshaped body, Ringkomplex und in neuronalen Zellk{\"o}rpern. Die panneural {\"u}berexprimierte SRPK79D-PB-GFP-Isoform liegt im larvalen und adulten Gehirn lokal im Zytoplasma der Perikaryen akkumuliert vor und wird nicht an die Aktive Zone transportiert. Das PB-Antiserum erkennt im adulten Gehirn neuronale Zellk{\"o}rper und das Neuropil in der Calyxregion der Pilzk{\"o}rper. Immunhistochemische F{\"a}rbungen von larvalen Nerv-Muskel-Pr{\"a}paraten mit verschiedenen Antik{\"o}rpern gegen neuronale Proteine belegen, dass die Agglomerate in der Srpk79D-Mutante f{\"u}r Bruchpilot spezifisch sind. Es konnten bisher keine weiteren Komponenten der Agglomerate detektiert werden. Auch ein genereller axonaler Defekt konnte durch F{\"a}rbungen gegen CSP, Synaptotagmin und Experimenten mit dem Mitochondrienfarbstoff MitoTracker® FM Green ausgeschlossen werden. Die quantitative Auswertung der Pr{\"a}parate zeigte, dass die Morphologie der synaptischen Boutons und die Zahl der Aktiven Zonen durch die Mutation im Srpk79D-Gen nicht beeinflusst werden. Um gesicherte Kenntnis dar{\"u}ber zu erlangen, ob die Mutation im Srpk79D-Gen die beobachteten Ph{\"a}notypen verursacht, wurden Rettungsexperimente durchgef{\"u}hrt. Es konnte sowohl f{\"u}r das hypomorphe Srpk79DP1-Allel, als auch f{\"u}r die Nullmutante Srpk79DVN eine nahezu vollst{\"a}ndige Rettung des Agglomerat-Ph{\"a}notyps mit der panneural exprimierten SRPK79D-PF- oder der SRPK79D-PB-Isoform erreicht werden. Aus diesen Ergebnissen folgt, dass beide Isoformen der SRPK79D in der Lage sind den Bruchpilot-Agglomerat-Ph{\"a}notyp zu retten, die Rettung der Verhaltensdefizite jedoch alle Isoformgruppen ben{\"o}tigen. Um zu untersuchen, ob der Agglomerations-Ph{\"a}notyp der Srpk79D-Mutanten auf einer {\"U}berexpression des Bruchpilotgens oder auf Fehlspleißen seiner pr{\"a}-mRNA beruht, wurden Immunpr{\"a}zipitationen, semiquantitative RT-PCRs und Real Time-PCRs durchgef{\"u}hrt. Ausgehend von den Ergebnissen kann eine m{\"o}gliche {\"U}berexpression bzw. Spleißdefekte von Bruchpilot weitgehend ausgeschlossen werden. Die simultane {\"U}berexpression von SRPK79D und Bruchpilot konnte den Ph{\"a}notyp der Bruchpilot-{\"U}berexpression nicht retten. Anhand der stimulated emission depletion-Mikroskopie konnte gezeigt werden, dass die gebildeten Agglomerate das charakteristische Donut-f{\"o}rmige Muster der T-bars zeigen und wahrscheinlich als fusionierte Ketten von T-bars in den larvalen Nerven vorliegen. Beim in vivo Imaging Versuch konnte demonstriert werden, dass das verk{\"u}rzte Bruchpilot-D3-Strawberry in die Bruchpilot-Agglomerate der Srpk79D-Nullmutante eingebaut wird und dass gr{\"o}ßere Agglomerate unbewegt im Nerv verharren. Der anterograde und retrograde Transport kleinerer Agglomerate konnte verzeichnet werden. Bei CytoTrap-Yeast-two-hybrid-Experimenten konnten f{\"u}r die SRPK79D-PB Isoform vier potentielle Interaktionspartner identifiziert werden: das Hitzeschockprotein Hsp70Bbb, die mitochondriale NADH-Dehydrogenase mt:ND5, das large ribosomal RNA Gen in Mitochondrien und das am Spleißen beteiligte Protein 1.3CC/Caper. Die Sequenzierung zeigte, dass nur das letzte Exon von Caper im pMyr-Vektor vorliegt. Der f{\"u}r die PC-Isoform durchgef{\"u}hrte CytoTrap-Versuch ergab nur Temperatur-Revertanten. SR-Proteinkinasen phosphorylieren die RS-Dom{\"a}ne von SR-Proteinen und sind dadurch an der Regulation des konstitutiven und alternativen Spleißens beteiligt. Somit stellen die acht identifizierten SR-Proteine in Drosophila potentielle Interaktionspartner der SRPK79D dar. Die durch RNAi-vermittelte Reduktion von sieben SR-Proteinen f{\"u}hrte zu keiner Agglomeration von Bruchpilot. Jedoch f{\"u}hrte die RNAi-vermittelte Reduktion des SR-Proteins Spleißfaktor 2 (SF2) zu kleineren Bruchpilot-Agglomeraten in den axonalen Nerven. SF2 ist selbst kein Bestandteil der Agglomerate der Srpk79D-Nullmutante. Die {\"U}berexpression von SF2 f{\"u}hrt wahrscheinlich zu einem axonalen Transportdefekt, wie die F{\"a}rbung gegen das Cysteine string protein zeigte. Weiterhin f{\"u}hrt die {\"U}berexpression zu einer Akkumulation von SF2 in larvalen Axonen und im adulten Gehirn der Fliegen. SF2 ist nicht nur in Zellkernen s{\"a}mtlicher Zellen nachweisbar, sondern es konnte auch ein spezifisches Signal im subsynaptischen Retikulum der Postsynapse detektiert werden, wie die F{\"a}rbungen gegen Disc large best{\"a}tigten.}, subject = {Taufliege}, language = {de} } @phdthesis{Schubert2019, author = {Schubert, Frank Klaus}, title = {The circadian clock network of \(Drosophila\) \(melanogaster\)}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-157136}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2019}, abstract = {All living organisms need timekeeping mechanisms to track and anticipate cyclic changes in their environment. The ability to prepare for and respond to daily and seasonal changes is endowed by circadian clocks. The systemic features and molecular mechanisms that drive circadian rhythmicity are highly conserved across kingdoms. Therefore, Drosophila melanogaster with its relatively small brain (ca. 135.000 neurons) and the outstanding genetic tools that are available, is a perfect model to investigate the properties and relevance of the circadian system in a complex, but yet comprehensible organism. The last 50 years of chronobiological research in the fruit fly resulted in a deep understanding of the molecular machinery that drives circadian rhythmicity, and various histological studies revealed the neural substrate of the circadian system. However, a detailed neuroanatomical and physiological description on the single-cell level has still to be acquired. Thus, I employed a multicolor labeling approach to characterize the clock network of Drosophila melanogaster with single-cell resolution and additionally investigated the putative in- and output sites of selected neurons. To further study the functional hierarchy within the clock network and to monitor the "ticking clock" over the course of several circadian cycles, I established a method, which allows us to follow the accumulation and degradation of the core clock genes in living brain explants by the means of bioluminescence imaging of single-cells.}, subject = {Taufliege}, language = {en} } @phdthesis{Schwenkert2005, author = {Schwenkert, Isabell}, title = {Phenotypic characterization of hangover at the neuromuscular junction}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-14977}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2005}, abstract = {Ethanoltoleranz beruht vermutlich auf Ver{\"a}nderung in synaptischer Plastizit{\"a}t; da die Mechanismen, die zu dieser Anpassung der Synapsen f{\"u}hren, in hang-Mutanten offensichtlich defekt sind, war es Ziel dieser Arbeit zu erkl{\"a}ren, wie HANG zu synaptischer Plastizit{\"a}t beitr{\"a}gt. In diesem Zusammenhang war es besonders wichtig herauszufinden, in welchem neuronalen Prozeß HANG eine Rolle spielt. Antik{\"o}rperfarbungen gegen HANG zeigten, da das Protein in allen neuronalen Zellkernen larvaler und adulter Gehirne vorhanden ist. Gehirne der hangAE10 Mutante zeigen keine F{\"a}rbung, was best{\"a}tigt, da diese Tiere Nullmutanten f{\"u}r HANG sind. Eine genauere Analyse der Verteilung von HANG im Zellkern ergab, daß HANG in einem punktartigen Muster an bestimmten Stellen im Kern angereichert ist; diese HANG-Aggregate sind an der Innenseite der Kernmembran lokalisiert und colokalisieren nicht mit dem Chromatin. Auf der Basis dieser Ergebnissen wurde postuliert, daß HANG vermutlich an der Stabilisierung, Prozessierung oder dem Export von mRNAs beteiligt ist. Da synaptische Plastizit{\"a}t gut an den einzelnen Neuronen der neuromuskul{\"a}ren Synapse von Drosophila-Larven studiert werden kann, wurde die Morphologie der Motorneurone dritter Larven am Muskelpaar 6/7 des Segments A4 untersucht. Diese Untersuchungen zeigten, da Boutonanzahl und Axonl{\"a}nge in hangAE10-Larven um 40 \% erh{\"o}ht sind. Außerdem zeigen einige Boutons der hang-Mutanten eine abnormale, sanduhrf{\"o}rmige Form, was darauf hinweist, daß sie nach Initiation der Bouton-Teilung m{\"o}glicherweise in einem halb-separierten Zustand geblieben sind. Die Zunahme an Boutons in den Mutanten ist im wesentlichen auf eine Zunahme der Anzahl der Typ Ib-Boutons zur{\"u}ckzuf{\"u}hren. Die Analyse der Verteilung verschiedener synaptischer Marker in hangover-Mutanten ergab keine Hinweise auf Abnormalit{\"a}ten im Zytoskelett oder in der Ausbildung der pr{\"a}-und postsynaptischen Strukturen. Des weiteren ist die Anzahl der aktiven Zonen relativ zur Boutonoberfl{\"a}che nicht ver{\"a}ndert; da hang-Mutanten aber mehr synaptische Boutons pro synaptischem Terminal besitzen, kann man insgesamt von einer Zunahme der Anzahl der aktiven Zonen ausgehen. Die pr{\"a}synaptische Expression von HANG in den Mutanten rettet die erh{\"o}hte Boutonanzahl und die verl{\"a}ngerten Axone, was ebenfalls beweist, daß die beobachteten synaptischen Defekte auf das Fehlen von HANG und nicht auf Sekund{\"a}rmutationen zur{\"u}ckzuf{\"u}hren sind. Eine postsynaptische Expression der hangover cDNA in den Mutanten dagegen rettet den Ph{\"a}notyp nicht. Die Anzahl der synaptischen Boutons wird unter anderem durch cAMP-Levels bestimmt, welche somit synaptische Plastizit{\"a}t regeln. Da hang-Mutanten eine erh{\"o}hte Boutonanzahl aufweisen, f{\"u}hrte dies zu der Spekulation, daß der Ph{\"a}notyp dieser Mutanten m{\"o}glicherweise auf ver{\"a}nderte cAMPlevels zur{\"u}ckzuf{\"u}hren ist. Um dies zu {\"u}berpr{\"u}fen, wurde die Morphologie der neuromuskul{\"a}ren Synapsen von hangAE10-Larven mit denen von dnc1 verglichen, welche Defekte in der cAMP-Kaskade aufweisen. Einige Aspekte des Ph{\"a}notyps (z. B. die Zunahme der Boutonanzahl und das Verhaltnis von aktiven Zonen pro Boutonfl{\"a}che) sind sehr ¨ahnlich; jedoch unterscheiden sich die beiden Mutanten in anderen morphologischen Aspekten. Die Expression eines UAS-dnc-Transgens in hangover-Mutanten modifizierte den hang-Ph{\"a}notyp ebenfalls nicht. Auf der Basis der Ergebnisse dieser Arbeit wurde ein Modell f{\"u}r die Funktion von HANG erstellt, nach dem dieses Protein vermutlich am Isoform-spezifischen Spleißen bestimmter Transkripte beteiligt ist, deren Produkte f{\"u}r die synaptische Plastizit{\"a}t an der neuromuskul{\"a}ren Synapse ben{\"o}tigt werden.}, subject = {Taufliege}, language = {en} } @phdthesis{Schwaerzel2003, author = {Schw{\"a}rzel, Martin}, title = {Localizing engrams of olfactory memories in Drosophila}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-5065}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2003}, abstract = {Zars and co-workers were able to localize an engram of aversive olfactory memory to the mushroom bodies of Drosophila (Zars et al., 2000). In this thesis, I followed up on this finding in two ways. Inspired by Zars et al. (2000), I first focused on the whether it would also be possible to localize memory extinction.While memory extinction is well established behaviorally, little is known about the underlying circuitry and molecular mechanisms. In extension to the findings by Zars et al (2000), I show that aversive olfactory memories remain localized to a subset of mushroom body Kenyon cells for up to 3 hours. Extinction localizes to the same set of Kenyon cells. This common localization suggests a model in which unreinforced presentations of a previously learned odorant intracellularly antagonizes the signaling cascades underlying memory formation. The second part also targets memory localization, but addresses appetitive memory. I show that memories for the same olfactory cue can be established through either sugar or electric shock reinforcement. Importantly, these memories localize to the same set of neurons within the mushroom body. Thus, the question becomes apparent how the same signal can be associated with different events. It is shown that two different monoamines are specificaly necessary for formation of either of these memories, dopamine in case of electric shock and octopamine in case of sugar memory, respectively. Taking the representation of the olfactory cue within the mushroom bodies into account, the data suggest that the two memory traces are located in the same Kenyon cells, but in separate subcellular domains, one modulated by dopamine, the other by octopamine. Taken together, this study takes two further steps in the search for the engram. (1) The result that in Drosophila olfactory learning several memories are organized within the same set of Kenyon cells is in contrast to the pessimism expressed by Lashley that is might not be possible to localize an engram. (2) Beyond localization, a possibible mechanism how several engrams about the same stimulus can be localized within the same neurons might be suggested by the models of subcellular organisation, as postulated in case of appetitive and aversive memory on the one hand and acquisition and extinction of aversive memory on the other hand.}, subject = {Taufliege}, language = {en} } @phdthesis{Thum2006, author = {Thum, Andreas Stephan}, title = {Sugar reward learning in Drosophila : neuronal circuits in Drosophila associative olfactory learning}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-17930}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2006}, abstract = {Genetic intervention in the fly Drosophila melanogaster has provided strong evidence that the mushroom bodies of the insect brain act as the seat of memory traces for aversive and appetitive olfactory learning (reviewed in Heisenberg, 2003). In flies, electroshock is mainly used as negative reinforcer. Unfortunately this fact complicates a comparative consideration with other inscets as most studies use sugar as positive reinforcer. For example, several lines of evidence from honeybee and moth have suggested another site, the antennal lobe, to house neuronal plasticity underlying appetitive olfactory memory (reviewed in Menzel, 2001; Daly et al., 2004). Because of this I focused my work mainly on appetitive olfactory learning. In the first part of my thesis, I used a novel genetic tool, the TARGET system (McGuire et al., 2003), which allows the temporally controlled expression of a given effector gene in a defined set of cells. Comparing effector genes which either block neurotransmission or ablate cells showed important differences, revealing that selection of the appropriate effector gene is critical for evaluating the function of neural circuits. In the second part, a new engram of olfactory memory in the Drosophila projection neurons is described by restoring Rutabaga adenlylate cyclase (rut-AC) activity specifically in these cells. Expression of wild-type rutabaga in the projection neurons fully rescued the defect in sugar reward memory, but not in aversive electric shock memory. No difference was found in the stability of the appetitive memories rescued either in projection neurons or Kenyon cells. In the third part of the thesis I tried to understand how the reinforcing signals for sugar reward are internally represented. In the bee Hammer (1993) described a single octopaminergic neuron - called VUMmx1 - that mediates the sugar stimulus in associative olfactory reward learning. Analysis of single VUM neurons in the fly (Selcho, 2006) identified a neuron with a similar morphology as the VUMmx1 neuron. As there is a mutant in Drosophila lacking the last enzymatic step in octopamine synthesis (Monastirioti et al., 1996), Tyramine beta Hydroxylase, I was able to show that local Tyramine beta Hydroxylase expression successfully rescued sugar reward learning. This allows to conclude that about 250 cells including the VUM cluster are sufficient for mediating the sugar reinforcement signal in the fly. The description of a VUMmx1 similar neuron and the involvement of the VUM cluster in mediating the octopaminergic sugar stimulus are the first steps in establishing a neuronal map for US processing in Drosophila. Based on this work several experiments are contrivable to reach this ultimate goal in the fly. Taken together, the described similiarities between Drosophila and honeybee regarding the memory organisation in MBs and PNs and the proposed internal representation of the sugar reward suggest an evolutionarily conserved mechanism for appetitive olfactory learning in insects.}, subject = {Taufliege}, language = {en} } @phdthesis{Triphan2009, author = {Triphan, Tilman}, title = {The Central Control of Gap Climbing Behaviour in Drosophila melanogaster}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-43666}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2009}, abstract = {In this work, a behavioural analysis of different mutants of the fruit fly Drosophila melanogaster has been carried out. Primarily, the gap climbing behaviour (Pick \& Strauss, 2005) has been assayed as it lends itself for the investigation of decision making processes and the neuronal basis of adaptive behaviour. Furthermore it shows how basic motor actions can be combined into a complex motor behaviour. Thanks to the neurogenetic methods, Drosophila melanogaster has become an ideal study object for neurobiological questions. Two different modules of climbing control have been examined in detail. For the decision making, the mutant climbing sisyphus was analysed. While wild-type flies adapt the initiation of climbing behaviour to the width of the gap and the probability for a successful transition. climbing sisyphus flies initiate climbing behaviour even at clearly insurmountable gap widths. The climbing success itself is not improved in comparison to the wild-type siblings. The mutant climbing sisyphus is a rare example of a hyperactive mutant besides many mutants that show a reduced activity. Basic capabilities in vision have been tested in an optomotor and a distance-estimation paradigm. Since they are not affected, a defect in decision making is most probably the cause of this behavioural aberration. A second module of climbing control is keeping up orientation towards the opposite side of the gap during the execution of climbing behaviour. Mutants with a structural defect in the protocerebral bridge show abnormal climbing behaviour. During the climbing attempt, the longitudinal body axis does not necessarily point into the direction of the opposite side. Instead, many climbing events are initiated at the side edge of the walking block into the void and have no chance to ever succeed. The analysed mutants are not blind. In one of the mutants, tay bridge1 (tay1) a partial rescue attempt used to map the function in the brain succeeded such that the state of the bridge was restored. That way, a visual targeting mechanism has been activated, allowing the flies to target the opposite side. When the visibility of the opposing side was reduced, the rescued flies went back to a tay1 level of directional scatter. The results are in accord with the idea that the bridge is a central constituent of the visual targeting mechanism. The tay1 mutant was also analysed in other behavioural paradigms. A reduction in walking speed and walking activity in this mutant could be rescued by the expression of UAS-tay under the control of the 007Y-GAL4 driver line, which concomitantly restores the structure of the protocerebral bridge. The separation of bridge functions from functions of other parts of the brain of tay1 was accomplished by rescuing the reduced optomotor compensation in tay1 by the mb247-GAL4>UAS-tay driver. While still having a tay1-like protocerebral bridge, mb247-GAL4 rescue flies are able to compensate at wild-type levels. An intact compensation is not depended on the tay expression in the mushroom bodies, as mushroom body ablated flies with a tay1 background and expression of UAS-tay under the control of mb247-GAL4 show wild-type behaviour as well. The most likely substrate for the function are currently unidentified neurons in the fan-shaped body, that can be stained with 007Y-GAL4 and mb247-GAL4 as well.}, subject = {Taufliege}, language = {en} } @phdthesis{Tschaepe2002, author = {Tsch{\"a}pe, Jakob-Andreas}, title = {Molekulare und funktionelle Analyse der Drosophila-Mutante l{\"o}chrig}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-2963}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2002}, abstract = {Neurodegenerative Erkrankungen des Menschen sind eines der Hauptfelder molekularer neurobiologischer Grundlagenforschung. Um generell molekulare, komplizierte Vorg{\"a}nge in vivo untersuchen zu k{\"o}nnen, nutzt man seit geraumer Zeit Modellorganismen wie Caenorhabditis elegans oder Drosophila melanogaster. In der vorliegenden Arbeit wird die Drosophila-Neurodegenerationsmutante loe (l{\"o}chrig) beschrieben, die als Modell f{\"u}r die Rolle des Cholesterinhaushalts im Bezug auf Neurodegeneration herangezogen werden kann. Die Fliegen dieser Mutante zeigen stark progressive, altersabh{\"a}ngige Degeneration von Neuronen, dabei unterlaufen diese Nervenzellen einen nekrotischenZelltod. Verantwortlich f{\"u}r diese Mutation ist die Insertion eines P-Elementes in einem Intron des Drosophila-g-5'-AMP-aktivierten Proteinkinase- (AMPK)-Gens. Die verschiedenen Spleißprodukte des loe Gens kodieren f{\"u}r die regulatorische g-Untereinheit des AMPK-Komplexes, der , aktiviert durch 5'AMP, energieintensive Prozesse negativ reguliert. Die Spleißform loeI ist durch die P-Element-Insertion betroffen, Anteile des P-Elementes werden in das loeI-Transkript hineingespleißt. Eine neuronale Expression von loeI im loe-Hintergrund f{\"u}hrt zur Revertierung des loe-Ph{\"a}notypes. Mit der Expression anderer Spleißformen kann dieser Effekt nicht erzielt werden. Das LOE I-Protein birgt in seinem N-Terminus eine Reihe m{\"o}glicher Interaktionstellen mit anderen Proteinen, die den AMPK-Komplex in einen Kontext mit den Proteinen der APP (Amyloid Precursor Proteins) ?Familie stellen oder z. B. Interaktionen mit dem Cytoskelett herstellen k{\"o}nnen. Eine molekulare Interaktion mit NiPSNAP, einem Protein, dass vermutlich eine Rolle im Vesikelverkehr spielt, konnte nachgewiesen werden. Ein direktes humanes Homolog von LOE I ist nicht bekannt, wohlgleich es im Menschen drei AMPK-g-Untereinheiten gibt, von denen zwei {\"a}hnliche Funktionen {\"u}bernehmen k{\"o}nnten wie LOE I. Die loe-Mutante interagiert genetisch mit der Mutante clb ? columbus, die einen Defekt im Gen der HMG-CoA-Reduktase tr{\"a}gt. Dieses Emzym ist das Schl{\"u}sselenzym der Cholesterinbiosynthese. Die Art der Interaktion belegt eine negative Regulierung der HMG-CoA-Reduktase durch die AMPK. So schw{\"a}cht die clb-Mutation den neurodegenerativen loe-Ph{\"a}notyp ab, eine {\"U}berexpression von clb verst{\"a}rkt diesen. Eine Verminderung der Neurodegeneration kann auch mit Medikamenten erreicht werden: Statine, potente Hemmer der HMG-COA-Reduktase, reprimieren deutlich den loe-Ph{\"a}notyp. In loe ist der Cholesterinester-Spiegel auf 40\% abgesenkt. Eine weitere genetische Interaktion von loe konnte nachgewiesen werden: Die Mutante f{\"u}r das Drosophila-Homolog von APP (Appl) verst{\"a}rkt den neurodegenerativen Ph{\"a}notyp in loe stark, wogegen die Appl-Mutante selbst keine neurodegenerativen Defekte aufweist. Dar{\"u}berhinaus zeigt die Doppelmutante Defekte, die keine der Einzelmutanten aufweist: Sterilit{\"a}t oder eine extrem kurze Lebensdauer von nur 3-4 Tagen. Diese Interaktion ließ sich auf molekularer Ebene charakterisieren. Die proteolytische Prozessierung von APPL durch Sekretasen ist in loe alteriert. In der vorliegenden Arbeit konnte gezeigt werden, dass durch die loe-Mutation die b-Sekretase aus Vertebraten (BACE) und eine bisher noch nicht beschriebene endogene Sekretase aus Drosophila negativ beeiflusst werden. Ein AMPK-Komplex mit LOE I als g-Untereinheit scheint {\"u}ber den Cholesterinester-Spiegel die Aktivit{\"a}t einer speziellen Untergruppe der Sekretasen zu beeinflussen. Die Missfunktion dieser Sekretasen ist ein kritischer Punkt in der Pathogenese der Alzheimer-Krankheit. Die loe-Mutation wirft neues Licht auf die bekannten Verbindungen zwischen Cholesterin-Stoffwechsel, Vesikelverkehr und Prozessierung von APP(L). Mit den großen M{\"o}glichkeiten, die die Drosophila-Genetik bietet, stellt diese neue Mutante ein weiteres Werkzeug zur Charakterisierung von Therapie-Ans{\"a}tzen f{\"u}r die Alzheimer-Kankheit dar. Die vorliegende Arbeit belegt um ein weiteres Mal, dass Drosophila ein potentes Modellsystem zur Untersuchung humaner, neurodegenerativer Erkrankungen wie Chorea Huntington, Parkinson oder der Alzheimer Krankheit ist.}, subject = {Taufliege}, language = {de} } @phdthesis{Tyagi2012, author = {Tyagi, Anu}, title = {Role of SWI/SNF in regulating pre-mRNA processing in Drosophila melanogaster}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-72253}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2012}, abstract = {ATP dependent chromatin remodeling complexes are multifactorial complexes that utilize the energy of ATP to rearrange the chromatin structure. The changes in chromatin structure lead to either increased or decreased DNA accessibility. SWI/SNF is one of such complex. The SWI/SNF complex is involved in both transcription activation and transcription repression. The ATPase subunit of SWI/SNF is called SWI2/SNF2 in yeast and Brahma, Brm, in Drosophila melanogaster. In mammals there are two paralogs of the ATPase subunit, Brm and Brg1. Recent studies have shown that the human Brm is involved in the regulation of alternative splicing. The aim of this study was to investigate the role of Brm in pre-mRNA processing. The model systems used were Chironomus tentans, well suited for in situ studies and D. melanogaster, known for its full genome information. Immunofluorescent staining of the polytene chromosome indicated that Brm protein of C. tentans, ctBrm, is associated with several gene loci including the Balbiani ring (BR) puffs. Mapping the distribution of ctBrm along the BR genes by both immuno-electron microscopy and chromatin immunoprecipitation showed that ctBrm is widely distributed along the BR genes. The results also show that a fraction of ctBrm is associated with the nascent BR pre-mRNP. Biochemical fractionation experiments confirmed the association of Brm with the RNP fractions, not only in C. tentans but also in D. melanogaster and in HeLa cells. Microarray hybridization experiments performed on S2 cells depleted of either dBrm or other SWI/SNF subunits show that Brm affects alternative splicing and 3´ end formation. These results indicated that BRM affects pre-mRNA processing as a component of SWI/SNF complexes. 1}, subject = {Taufliege}, language = {en} } @phdthesis{Voeller2009, author = {V{\"o}ller, Thomas}, title = {Visualisierung und Manipulation neuronaler Aktivit{\"a}ten im Gehirn von Drosophila melanogaster}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-35589}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2009}, abstract = {In dieser Arbeit wurden zwei Techniken zur Analyse der Funktion diverser Neuronen in Drosophila melanogaster angewendet. Im ersten Teil wurde mittels in-vivo Calcium Imaging Technik unter Verwendung des Calciumsensors Cameleon neuronale Aktivit{\"a}t entlang des olfaktorischen Signalweges registriert. Hierbei wurde die neuronale Repr{\"a}sentation der Duftidentit{\"a}t und der Duftintensit{\"a}t untersucht. In Bezug auf diese Fragestellung wurde die Datenverarbeitung und Datenanalyse weiterentwickelt und standardisiert. Die Experimente f{\"u}hrten zu dem Ergebnis, dass duftspezifische Aktivit{\"a}tsmuster auf der Ebene des Antennallobus sehr gut unterscheidbar sind. Manche Aktivit{\"a}tsmuster der pr{\"a}sentierten D{\"u}fte zeigten interessanterweise einen hohen {\"A}hnlichkeitsgrad, wohingegen andere un{\"a}hnlich waren. In h{\"o}heren Gehirnzentren wie den Orten der terminalen Aborisationen der Projektionsneurone oder den Pilzk{\"o}rper Kenyonzellen liegt eine starke Variabilit{\"a}t der duftevozierten Aktivit{\"a}tsmuster vor, was generelle Interpretationen unm{\"o}glich macht und h{\"o}chstens Vergleiche innerhalb eines Individuums zul{\"a}sst. Des Weiteren konnte gezeigt werden, dass die Calciumsignale in den Rezeptorneuronen sowie pr{\"a}- und postsynaptisch in den Projektionsneuronen bei Erh{\"o}hung der Konzentration der verschiedenen pr{\"a}sentierten D{\"u}fte {\"u}ber einen Bereich von mindestens drei Gr{\"o}ßenordnungen ansteigen. In den Kenyonzellen des Pilzk{\"o}rper-Calyx und der Pilzk{\"o}rper-Loben ist diese Konzentrationsabh{\"a}ngigkeit weniger deutlich ausgepr{\"a}gt und im Falle der Loben nur f{\"u}r bestimmte D{\"u}fte detektierbar. Eine Best{\"a}tigung des postulierten „sparsed code" der Duftpr{\"a}sentation in den Pilzk{\"o}rpern konnte in dieser Arbeit nicht erbracht werden, was m{\"o}glicherweise daran liegt, dass eine Einzelzellaufl{\"o}sung mit der verwendeten Technik nicht erreicht werden kann. Im zweiten Teil dieser Arbeit sollte durch die Nutzung des lichtabh{\"a}ngigen Kationenkanals Channelrhodopsin-2 der Frage nachgegangen werden, ob bestimmte modulatorische Neurone die verst{\"a}rkenden Eigenschaften eines bestrafenden oder belohnenden Stimulus vermitteln. Die lichtinduzierte Aktivierung von Channelrhodopsin-2 exprimierenden dopaminergen Neuronen als Ersatz f{\"u}r einen aversiven Reiz f{\"u}hrte bei einer olfaktorischen Konditionierung bei Larven zur Bildung eines aversiven assoziativen Ged{\"a}chtnisses. Im Gegensatz dazu induzierte die Aktivierung von Channelrhodopsin-2 in oktopaminergen/tyraminergen Neuronen als Ersatz f{\"u}r einen appetitiven Reiz ein appetitives assoziatives Ged{\"a}chtnis. Diese Ergebnisse zeigen, dass dopaminerge Neurone bei Larven aversives Duftlernen, oktopaminerge/tyraminerge Neurone dagegen appetitives Duftlernen induzieren.}, subject = {Taufliege}, language = {de} } @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{Wagner2003, author = {Wagner, Nicole}, title = {Charakterisierung der Kernmembranproteine Lamin-B-Rezeptor und Bocksbeutel von Drosophila melanogaster}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-7245}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2003}, abstract = {Funktionelle Charakterisierung neuer Proteine der inneren Kernmembran von Drosophila melanogaster: Drosophila Lamin B Rezeptor (dLBR), ein integrales Membranprotein der inneren Kernmembran; Bocksbeutel alpha und Bocksbeutel beta, LEM-Dom{\"a}nen Proteine sowie deren potentiellen Interaktionspartner Drosophila Barrier-to-Autointegration Factor (dBAF).}, subject = {Taufliege}, language = {de} }