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Retinitis pigmentosa (RP) ist eine vererbte Form der Erblindung, die durch eine progressive Degeneration von Photorezeptorzellen in der Retina verursacht wird. Neben „klassischen“ RP-Krankheitsgenen, die direkt oder indirekt mit dem Sehprozess und der Aufrechterhaltung der Photorezeptoren in Verbindung stehen, können auch Mutationen in Genen für konstitutive Spleißfaktoren zur Photorezeptordegeneration führen. RP kann daher als Paradebeispiel einer Erkrankung mit paradoxer Gewebespezifität angesehen werden: Defekte in essentiellen und ubiquitär exprimierten Genen führen zu einem Phänotyp, der nur wenige Zelltypen betrifft. Um Einblicke in diesen außergewöhnlichen Pathomechanismus zu erhalten, wurde im Rahmen der vorliegenden Arbeit ein Tiermodell für Spleißfaktor-vermittelte RP im Zebrafisch Danio rerio etabliert. Zunächst wurde gezeigt, dass eine RP verursachende Punktmutation des Spleißfaktors Prpf31 auch in dessen Zebrafisch-Homolog zu einem Verlust der physiologischen Aktivität führt. Als Modell für die Prpf31-Mangelsituation diente dann die durch ein Antisense-Morpholino induzierte partielle Reduktion der Prpf31-Expression in Zebrafischlarven. Konsistent mit einem RP-Phänotyp zeigte sich in diesen Larven eine starke Beeinträchtigung des Sehvermögens. Sie wurde – ebenfalls analog zu RP – durch defekte Photorezeptoren verursacht, die bei ansonsten normal entwickelter Retina eine deutlich veränderte Morphologie aufwiesen. Daraufhin konnten in einer genomweiten Transkriptomanalyse der Augen von Prpf31-defizienten Larven erstmals in vivo photorezeptorspezifische Gene identifiziert werden, deren Expression durch den Mangel an Prpf31 beeinträchtigt war. Im zweiten Teil der Arbeit wurde untersucht, ob es neben den bereits bekannten RP-Krankheitsgenen weitere Spleißfaktoren gibt, deren Defekt die Degeneration von Photorezeptoren auslösen kann. Dazu wurde in Zebrafischlarven ein Mangel an Prpf4 erzeugt, einem Spleißfaktor, der bislang nicht mit RP in Verbindung gebracht worden war. Der Phänotyp dieser Fische war nicht von dem des Prpf31 RP-Modells zu unterscheiden. Dies lieferte einen Hinweis darauf, dass auch Defekte in Prpf4 in der Lage sein könnten, RP auszulösen. Tatsächlich konnte durch genetisches Screening ein RP-Patient mit einer Punktmutation in Prpf4 identifiziert werden (Kollaboration mit Hanno Bolz, Universität Köln). Die biochemische Analyse dieser Mutation zeigte, dass sie zu einem Defekt der Integration von Prpf4 in spleißosomale Untereinheiten und zu dessen Funktionsverlust in vivo führt. Mit dem in dieser Arbeit etablierten Tiermodell konnte zum ersten Mal in vivo ein von Spleißfaktor-Mutationen verursachter Pathomechanismus von Retinitis pigmentosa nachvollzogen werden. Die vom Prpf31-Mangel betroffenen Photorezeptortranskripte stellen vielversprechende Kandidaten für die Vermittlung der Gewebespezifität dar und unterstützen die Hypothese, dass ihre ineffiziente Prozessierung den RP-Phänotyp auslöst. Die Entdeckung eines weiteren Spleißfaktors, dessen Defizienz ebenfalls zu defekten Photorezeptoren führt, zeigt, dass offenbar der Funktionsverlust des Spleißosoms generell in der Lage ist, die Degeneration dieser Zellen zu verursachen. Dies ist nicht zuletzt auch von klinischer Relevanz, da vermutet werden kann, dass sich unter den vielen bisher nicht identifizierten RP-Krankheitsgenen weitere Spleißfaktoren befinden.
In mammals, the pituitary-derived neuropeptide adrenocorticotropic hormone (ACTH) is a major regulator of adrenocortical steroidogenesis and hormone secretion. However, the mechanism by which adrenal growth is governed by pituitary signals and the role of the pituitary in early adrenal development remain to be investigated. In this work the model organism zebrafish was used to elucidate pituitary adrenal interactions during early vertebrate development. The adrenal homologue in zebrafish is located in the head kidney and termed interrenal organ. The work deals with the analysis of pituitary-interrenal interactions by using pituitary mutants, gene-knockdown embryos and pharmacological interventions. As prerequisite to the main study, zebrafish pomc gene was cloned and characterized and the interrenal organogenesis in wild-type zebrafish was analysed.
Attention deficit hyperactivity disorder (ADHD) is one of the most prevalent developmental disorders, affecting 5.9% children and adolescents and 2.5% adults worldwide. The core characteristics are age-inappropriate levels of hyperactivity, impulsivity and inattention, often accompanied by co-morbidities such as mood and conduct disorders as wells as learning deficits. In the majority of cases, ADHD is caused by an interplay of accumulated genetic and environmental risk factors. Twin studies report a very high heritability of 70–80%, however, common genetic variants in the population only explain a third of the heritability. The rest of the genetic predisposition is composed of rare copy number variations (CNVs) and gene x environment interactions including epigenetic alterations. Through genome wide association (GWAS) and linkage studies a number of likely candidate genes were identified. A handful of them play a role in dopamine or noradrenaline neurotransmitter systems, simultaneously those systems are the main targets of common drug treatment approaches. However, for the majority of candidates the biological function in relation to ADHD is unknown. It is crucial to identify those functions in order to gain a deeper understanding of the pathomechanism and genetic networks potentially responsible for the disorder. This work focuses on the three candidate genes GFOD1, SLC2A3 and LBX1 and their role in the healthy organism as well as in case of ADHD. The neuroanatomy was regarded through expression analysis and various behavioural assays of activity were performed to link alterations on the transcript level to phenotypes associated with the neurodevelopmental disorder. Zebrafish orthologues of the human risk genes were identified and extensive temporal and spacial expression characterisation performed via RNA in situ hybridisation. Through morpholino derived knock-down and mRNA overexpression zebrafish models with subsequent behavioural analysis, both hyper- and hypoactive phenotypes were discovered. Additional expression analysis through double in situ hybridisation revealed a co-localisation during zebrafish neurodevelopment of each gfod1 and slc2a3a together with gad1b, a marker for GABAergic neurons. Interestingly, both risk genes have previously been associated with glucose homeostasis and energy metabolism, which when disrupted could lead to alterations in signal transduction and neuron survival. Likewise, Lbx1 plays a pivotal role in GABAergic versus glutamatergic neuron specification during spinal cord and hindbrain development in mice and chicken. Preliminary results of this work suggest a similar role in zebrafish. Taken together, those findings on the one hand represent a sturdy basis to con- tinue studies of the function of the genes and on the other hand open up the opportunity to investigate novel aspects of ADHD research by exploring the role of the GABAergic neurotransmitter system or the connection between energy metabolism and psychiatric disorders.
The vertebrate spinal cord is composed of billions of neurons and glia cells, which are formed in a highly coordinated manner during early neurogenesis. Specification of these cells at distinct positions along the dorsoventral (DV) axis of the developing spinal cord is controlled by a ventrally located signaling center, the medial floor plate (MFP). Currently, the origin and time frame of specification of this important organizer are not clear. During my PhD thesis, I have analyzed the function of the novel secreted growth factor Midkine-a (Mdka) in zebrafish. In higher vertebrates, mdk and the related factor pleiotrophin (ptn) are widely expressed during embryogenesis and are implicated in a variety of processes. The in-vivo function of both factors, however, is unclear, as knock-out mice show no embryonic phenotype. We have isolated two mdk co-orthologs, mdka and mdkb, and one single ptn gene in zebrafish. Molecular phylogenetic analyses have shown that these genes evolved after two large gene block duplications. In contrast to higher vertebrates, zebrafish mdk and ptn genes have undergone functional divergence, resulting in mostly non-redundant expression patterns and functions. I have shown by overexpression and knock-down analyses that Mdka is required for MFP formation during zebrafish neurulation. Unlike the previously known MFP inducing factors, mdka is not expressed within the embryonic shield or tailbud but is dynamically expressed in the paraxial mesoderm. I used epistatic and mutant analyses to show that Mdka acts independently from these factors. This indicates a novel mechanism of Mdka dependent MFP formation during zebrafish neurulation. To get insight into the signaling properties of zebrafish Mdka, the function of both Mdk proteins and the candidate receptor Anaplastic lymphoma kinase (Alk) have been compared. Knock-down of mdka and mdkb resulted in the same reduction of iridophores as in mutants deficient for Alk. This indicates that Alk could be a putative receptor of Mdks during zebrafish embryogenesis. In most vertebrate species a lateral floor plate (LFP) domain adjacent to the MFP has been defined. In higher vertebrates it has been shown that the LFP is located within the p3 domain, which forms V3 interneurons. It is unclear, how different cell types in this domain are organized during early embryogenesis. I have analyzed a novel homeobox gene in zebrafish, nkx2.2b, which is exclusively expressed in the LFP. Overexpression, mutant and inhibitor analyses showed that nkx2.2b is activated by Sonic hedgehog (Shh), but repressed by retinoids and the motoneuron-inducing factor Islet-1 (Isl1). I could show that in zebrafish LFP and p3 neuronal cells are located at the same level along the DV axis, but alternate along the anteroposterior (AP) axis. Moreover, these two different cell populations require different levels of HH signaling and nkx2.2 activities. This provides new insights into the structure of the vertebrate spinal cord and suggests a novel mechanism of neural patterning.
Investigation on Distinct Roles of Smad Proteins in Mediating Bone Morphogenetic Proteins Signals
(2011)
Bone morphogenetic proteins (BMPs) belong to the transforming growth factor-β (TGF-β) superfamily and play important roles in numerous biological events in the development of almost all multi-cellular organisms. Dysregulated BMP signaling is the underlying causes of numerous heritable and non-heritable human diseases including cancer. The vast range of biological responses induced by BMPs converges on three closely related Smad proteins that convey intracellular signals from BMP receptors to the nucleus. The specificity of BMP signaling has been intensively investigated at the level of ligand-receptor interactions, but how the different Smad proteins contribute to differential signals elicited by BMPs remains unclear. In this work, we investigated the BMP/Smad signaling in different aspects. In search for an appropriate fluorescence reporter in zebrafish, we compared different photo-switchable proteins and found EosFP the best candidate this model system for its fast maturation and fluorescence intensity. We modified and created appropriate vectors enabling Tol2-transposon based trangenesis in zebrafish, with which transgenic zebrafish lines were generated. We combined fluorescence protein tagging with high resolution microscopy and investigate the dynamics of Smad proteins in model system zebrafish. We observed that Smad5 undergoes nucleo-translocation as BMP signal transmitter during zebrafish gastrulation. We explored the Smad involvement during myogenic-to-osteogenic conversion of C2C12 cell line induced by BMP4. We created transient loss-of-function of Smads by siRNA-mediated knockdowns and analyzed the effects on these coupled yet distinct procedures by quantitative real-time PCR and terminal marker staining. We found that different Smad-complex stoichiometry might be responsible for distinct cellular signals elicited by BMPs.
Neural crest cells and sensory neurons are two prominent cell populations which are induced at the border between neural and non-neural ectoderm during early vertebrate development. The neural crest cells are multipotent and highly migratory precursors that give rise to face cartilage, peripheral neurons, glia cells, pigment cells and many other cell types unique to vertebrates. Sensory neurons are located dorsally in the neural tube and are essential for sensing and converting environmental stimuli into electrical motor reflexes. In my PhD thesis, I obtained novel insights into the complex processes of cell induction at the neural plate border by investigating the regulation and function of mdkb in zebrafish. First, it was possible to demonstrate that mdkb expression is spatiotemporally correlated with the induction of neural crest cells and primary sensory neurons at the neural plate border. Second, it became evident that the expression of mdkb is activated by known neural crest cell inducing signals, like Wnts, FGFs and RA, but that it is independent of Delta-Notch signals essential for lateral inhibition. Knockdown experiments showed that mdkb function is necessary for induction of neural crest cells and sensory neurons at the neural plate border, probably through determination of a common pool of progenitor cells during gastrulation. The present study also used the advantages of the zebrafish model system to investigate the in vivo function of all midkine gene family members during early brain development. In contrast to the situation in mouse, all three zebrafish genes show distinct expression patterns throughout CNS development. mdka, mdkb and ptn expression is detected in mostly non-overlapping patterns during embryonic brain development in the telencephalon, the mid-hindbrain boundary and the rhombencephalon. The possibility of simultaneously knocking down two or even three mRNAs by injection of morpholino mixtures allowed the investigation of functional redundancy of midkine factors during brain formation. Knockdown of Midkine proteins revealed characteristic defects in brain patterning indicating their association with the establishment of prominent signaling centers such as the mid-hindbrain boundary and rhombomere 4. Interestingly, combined knockdown of mdka, mdkb and ptn or single knockdown of ptn alone prevented correct formation of somites, either by interfering with the shifting of the somite maturation front or interferance with cell adhesion in the PSM. Thus, Ptn was identified as a novel secreted regulator of segmentation in zebrafish.
Formation oft the central nervous system (CNS) from multipotent neuronal stem cells (NSCs) requires a tightly controlled, step-wise activation of the neuronal gene expression program. Expression of neuronal genes at the transition from neural stem cell to mature neuron (i. e. neuronal cell differentiation) is controlled by the Repressor element 1 (RE1) silencing transcription factor (REST) complex. As a master transcriptional regulator, the REST-complex specifically inhibits expression of neuronal genes in non-neuronal tissues and neuronal progenitor cells. Differentiation of NSCs to mature neurons requires the activation of genes controlled by the REST-complex, but how abrogation of REST-complex mediated repression is achieved during neurogenesis is only poorly understood. MicroRNAs (miRNAs) are a class of small regulatory RNAs that posttranscriptionally control target gene expression. Binding of miRNAs to target sequences in the 3’UTR of mRNAs, leads either to degradation or translational inhibition of the mRNA. Distinct neuronal miRNAs (e.g. miR-124) were shown to modulate REST-complex activity by silencing expression of REST-complex components. Interestingly, these miRNAs are also under transcriptional control of the REST-complex and inactivation of the REST-complex precedes their expression. Hence, additional factors are required for derepression of neuronal genes at the onset of neurogenesis. In this study function of the miR-26 family during neurogenesis of the zebrafish (Danio rerio) was analyzed. Computational target prediction revealed a number of REST-complex components as putative miR-26 targets. One of these predicted target genes, the C-terminal domain small phosphatase 2 (Ctdsp2) was validated as an in vivo target for miR-26b. Ctdsps are important cofactors of REST and suppress neuronal gene expression by dephosphorylating the C-terminal domain (CTD) of RNA polymerase II (Pol II). Interestingly, miR-26b is encoded in an intron of the ctdsp2 primary transcript and is cotranscribed together with its host gene. Hence, miR-26b modulates expression of its host gene ctdsp2 in an intrinsic negative autoregulatory loop. This negative autoregulatory loop is inactive in NSCs because miR-26b biogenesis is inhibited at the precursor level. Generation of mature miR-26b is activated during neurogenesis, where it suppresses Ctdsp2 protein expression and is required for neuronal cell differentiation in vivo. Strikingly, miR-26b is expressed prior to miR-124 during neuronal cell differentiation. Thus, it is reasonable to speculate about a function of miR-26b in early events of neurogenesis. In line with this assumption, knockdown of miR-26b in zebrafish embryos results in downregulation of REST-complex controlled neuronal genes and a block in neuronal cell differentiation, most likely due to aberrant regulation of Ctdsp2 expression. This is evident by reduced numbers of secondary motor neurons compared to control siblings. In contrast, motor neuron progenitor cells and glia cells were not affected by depletion of miR-26b.This study identifies the ctdsp2/miR-26b autoregulatory loop as the first experimentally validated interaction between an intronic miRNA and its host gene transcript. Silencing of ctdsp2 by miR-26b in neurons is possible because biogenesis of the ctdsp2 mRNA and mature mir-26b is uncoupled at the posttranscriptional level. Furthermore the obtained data indicate a cell type specific role for miR-26b in vertebrate neurogenesis and CNS development.
This thesis explores the development of monoaminergic systems in the central nervous system (CNS) of zebrafish. The serotonergic cells of the hypothalamus pose the main focus of the present work. Most vertebrates except for mammals possess serotonin (5-HT) synthesising cells in more than one region of the CNS. In zebrafish such regions are, e.g. the hypothalamus, the raphe nuclei and the spinal cord. Serotonin functions as a neurotransmitter and neuromodulator in the CNS. Presumably due to its neuromodulatory tasks hypothalamic serotonergic cells are in contact with the cerebrospinal fluid (CSF), which expands the field of potential serotonergic targets tremendously. This highlights that serotonergic CSF-contacting (CSF-c) cells are vital for the execution of many functions and behaviours. Further, the hypothalamic serotonergic clusters constitute the largest population of serotonergic cells in the CNS of zebrafish. Together, these facts emphasise the need to understand the development and function of serotonergic CSF-c cells in the hypothalamus. Few studies have dealt with this subject, hence, information about the development of these cells is scarce. The zinc-finger transcription factor fezf2, and Fibroblast growth factor (Fgf)-signalling via the ETS-domain transcription factor etv5b are known to regulate serotonergic cell development in the hypothalamus (Bosco et al., 2013; Rink and Guo, 2004). However, the main Fgf ligand responsible for this mediation has not been determined prior to this work. The present thesis identifies Fgf3 as a crucial Fgf ligand. To achieve this result three independent strategies to impair Fgf3 activity have been applied to zebrafish embryos: the fgf3t24152 mutant, an fgf3 morpholino-based knock-down and the CRISPR/Cas9 technique. The investigations show that Fgf3 regulates the development of monoaminergic CSF-c cells in the hypothalamus. Additionally, Fgf3 impacts on cells expressing the peptide hormone arginine vasopressin (avp). Most interestingly, the requirement for Fgf3 by these cells follows a caudo-rostral gradient with a higher dependence on Fgf3 by caudal cells. This also seems to be the case for dopaminergic CSF-c cells in the hypothalamus (Koch et al., 2014). Moreover, etv5b a downstream target of Fgf-signalling is demonstrated to be under the control of Fgf3. With regard to serotonergic CSF-c cell development, it is shown that fgf3 is expressed several hours before tph1a and 5-HT (Bellipanni et al., 2002; Bosco et al., 2013). Together with the result that the hypothalamus is already smaller before mature serotonergic CSF-c cells appear, this argues for an early impact of Fgf3 on serotonergic specification. This hypothesis is supported by several findings in this study: the universal decrease of proliferating cells in the hypothalamus and simultaneous increase of cell death after fgf3 impairment. Complementary cell fate experiments confirm that proliferating serotonergic progenitors need Fgf3 to commit serotonergic specification. Further, these results corroborate findings of an earlier study stating that hypothalamic serotonergic progenitors require Fgf-signalling via etv5b to maintain the progenitor pool (Bosco et al., 2013). Additionally, the transcriptome of the hypothalamus has been analysed and 13 previously overlooked transcripts of Fgf ligands are expressed at developmental stages. The transcriptome analysis provides evidence for a self-compensatory mechanism of fgf3 since expression of fgf3 is upregulated as a consequence of its own impairment. Moreover, the Fgf-signalling pathway appears to be mildly affected by fgf3 manipulation. Together, Fgf-signalling and especially Fgf3 are established to be of critical importance during hypothalamic development with effects on serotonergic, dopaminergic CSF-c and avp expressing cells. Furthermore, this thesis provides two strategies to impair the tph1a gene. Both strategies will facilitate investigations regarding the function of hypothalamic serotonergic CSF-c cells. Finally, the presented findings in this study provide insights into the emergence of the posterior recess region of the hypothalamus, thereby, contributing to the understanding of the evolution of the vertebrate hypothalamus.
Aufgrund mangelnder Aktivität der Gewebe-unspezifischen Phosphatase (tissue-nonspecific alkaline phosphatase, TNAP) kommt es zum Krankheitsbild der Hypophosphatasie (HPP). Neben skelettalen und neuronalen Symptomen leiden Patienten mit HPP häufig an einem vorzeitigen Verlust der Milchzähne und weiteren dentalen Manifestationen, wie Zahnhartsubstanzdefekten, Eruptionsstörungen, erweiterte Pulpenkammern oder einer verringerten alveolären Knochenhöhe.
Ziel der Arbeit war es, den Einfluss der TNAP auf die Zahnentwicklung von Zebrafischlarven zu untersuchen, um ein neues in-vivo Modell für die dentalen Auswirkungen bei Hypophosphatasie etablieren zu können. Um die sehr kleinen Zähne der Zebrafischlarven auch in frühen Entwicklungsstadien darzustellen, wurden mittels verschiedener histologischer Färbungen die Zahnstrukturen angefärbt und die Larven danach in JB4®, einen polymeren Kunststoff, eingebettet. Im Anschluss wurden histologische Schnitte angefertigt und am Fluoreszenzmikroskop ausgewertet.
Einerseits konnte durch In-situ-Hybridisierung die Expression verschiedener Gene, wie z.B. alpl (welches für die Tnap im Zebrafisch kodiert), im Bereich von dentalen Strukturen in verschiedenen Entwicklungsstadien nachgewiesen werden. Außerdem zeigte die Analyse der dentalen Strukturen nach Inhibition der Tnap mittels Levamisol bei fünf Tage alten Zebrafischlarven eine Veränderung von Form, Größe und Struktur der ersten Zähne. Die TNAP-Inhibition führte auch zur quantitativ nachweisbaren Steigerung des Fluoreszenzsignals von ß-Catenin, welches eine zentrale Funktion im Wnt/ß-Catenin-Signalweg besitzt und essenziell in verschiedenen zellulären Prozessen während der Embryogenese ist.
Zusammenfassend zeigen die Ergebnisse der Arbeit, dass der Zebrafisch großes Potenzial als in-vivo Modell für die dentalen Symptome bei HPP bietet. Außerdem eröffnen sich neue interessante Fragen in Bezug auf den Einfluss von ß-Catenin bei den frühen pathophysiologischen Prozessen der Erkrankung.
Das Tuberoinfundibuläre Peptid von 39 Aminosäuren (TIP39), ein kurzes Oligopeptid mit einer N-terminalen und einer C-terminalen alpha-Helix, wurde ursprünglich bei der Suche nach einem Liganden für den neu beschriebenen PTH2-Rezeptor aus einem Hypothalamus-Hypophysen-Extrakt isoliert. Aus der bisherigen Charakterisierung von TIP39 ist am meisten bekannt bezüglich der Expressions-Muster und der Interaktion am PTH2-Rezeptor. TIP39 ist der stärkste bekannte Aktivator des PTH2-Rezeptors und wirkt am PTH1-Rezeptor als funktioneller Antagonist. Inzwischen wurde auch das TIP39 Gen des Menschen und der Maus charakterisiert. Die physiologische Rolle von TIP39 ist dennoch bisher weitgehend ungeklärt, diskutiert werden Einflüsse auf den Kalzium-Phosphat-Haushalt, die Hypothalamus-Hypophysen-Achse oder die Nozizeption. Der Schwerpunkt dieser Arbeit lag auf der Untersuchung des TIP39 kodierenden Gens des Zebrafischs danio rerio. Die komplette cDNA konnte amplifiziert werden und wurde unter der Accession No. AF486190 in der GenBank veröffentlicht. Der Genlocus konnte mittels Radiation Hybrid Mapping auf Chromosom 17 lokalisiert werden. Die 3 charakterisierten Exons und 2 Introns umfassen zusammen ca. 3750 bp. Daneben wurde die Prozessierung des Genprodukts aufgeklärt: TIP39 wird beim Zebrafisch als Preprohormon translatiert, am N-terminalen Ende findet sich eine 25 Aminosäuren lange Signalsequenz, die für sezernierte Peptide typisch ist und welche für die Aufnahme in das Endoplasmatische Retikulum verantwortlich ist. In diesem Bereich finden sich eine weitgehende Übereinstimmungen zwischen den analysierten Spezies. Gefolgt wird die Zielsequenz von einem 93 Aminosäuren langen Zwischenpeptid, das sich als wenig konserviert zwischen den Spezies zeigt. Die eigentliche Sequenz von TIP39 beim Zebrafisch zeigte eine Sequenzhomologie von 59% zur humanen Sequenz und wurde mittels Blast Suche als hochkonserviert in allen 12 untersuchten Spezies wiedergefunden. Im genomischen Southern-Blot zeigte sich, dass TIP39 beim Zebrafisch im einfachen Chromosomensatz ein „single-copy“ Gen ist. Mittels RT-PCR konnte eine sehr frühe erste Expression von TIP39 bereits ab 16 Stunden nach Fertilisation gezeigt werden. Im Bereich des supraoptischen Trakts des Zebrafischhirn konnte eine scharf umschriebene Zellpopulation mit starker TIP39-Expression detektiert werden. Durch Knockdown-Experimente konnte beim Zebrafisch gezeigt werden, dass ein Fehlen von TIP39 Expression während der Embryogenese zu einer Fehlentwicklung des Frontalhirns führt und zudem mit einer Funktionsbeeinträchtigung der Schwanzmotorik einhergeht. Hierfür wurden gerade befruchteten Zebrafischeiern im Zwei-Zell-Stadium sogenannte „Morpholinos“ injiiziert, welche als Antisense-Nukleotide spezifisch die Translation von TIP39 hemmen. Ergänzend konnte im Mäusehirn die Expression von TIP39 mittels in-situ Hybridisierung bestimmt werden. Es zeigte sich eine Expression von TIP39 in einer Vielzahl von klar umschriebenen Neuronengruppen, so im Hypothalamus, dem limbischen System und in sensorischen Neuronen, ohne dass sich im Einzelfall jeweils sicher eine Funktion hieraus ableiten lässt. In der vorliegenden Arbeit konnte somit erstmals gezeigt werden, dass TIP39 zur korrekten Neurogenese bei der Entwicklung des Frontalhirns des Zebrafisches unabdingbar ist und auch die frühe Entwicklung der Motoneurone durch TIP39 beeinflusst wird. Die ermittelten Daten unterstützen die Vorstellung von TIP39 als ein sezerniertes Neuropeptid, das als Transmitter in der Sensorik, insbesondere der Nozizeption, wirkt. Auch eine Beeinflussung der zentralnervösen Steuerung der Motorik durch TIP39 wird angenommen. Die gute Lokalisations-Übereinstimmung der Expressionen von TIP39 mit seinem zugeordneten Rezeptor, dem PTH2-Rezeptor, lässt eine systemische endokrine Wirkung von TIP39 wenig wahrscheinlich erscheinen, sondern stärkt die Hypothese von TIP39 als einem para-, bzw. autokrin wirkenden Neurotransmitter.
The Popeye domain containing (Popdc) gene family of membrane proteins is predominantly expressed in striated and smooth muscle tissues and has been shown to act as novel cAMP-binding proteins. In mice, loss of Popdc1 and Popdc2, respectively, affects sinus node function in the postnatal heart in an age and stress-dependent manner. In this thesis, I examined gene expression pattern and function of the Popdc gene family during zebrafish development with an emphasis on popdc2. Expression of the zebrafish popdc2 was exclusively present in cardiac and skeletal muscle during cardiac development, whereas popdc3 was expressed in striated muscle tissue and in distinct regions of the brain. In order to study the function of these genes, an antisense morpholino-based knockdown approach was used. Knockdown of popdc2 resulted in aberrant development of facial and tail musculature. In the heart, popdc2 morphants displayed irregular ventricular contractions with 2:1 and 3:1 ventricular pauses. Recordings of calcium transients using a transgenic indicator line Tg(cmlc2:gCaMP)s878 and selective plane illumination microscopy (SPIM) revealed the presence of an atrioventricular (AV) block in popdc2 morphants as well as a complete heart block. Interestingly, preliminary data revealed that popdc3 morphants developed a similar phenotype. In order to find a morphological correlate for the observed AV conduction defect, I studied the structure of the AV canal in popdc2 morphants using confocal analysis of hearts of the transgenic line Tg(cmlc2:eGFP-ras)s883, which outlines individual cardiac myocytes with the help of membrane-localized GFP. However, no evidence for morphological alterations was obtained. To ensure that the observed arrhythmia phenotype in the popdc2 morphant was based on a myocardial defect and not caused by defective valve development, live imaging was performed revealing properly formed valves. Thus, in agreement with the data obtained in knockout mice, popdc2 and popdc3 genes in zebrafish are involved in the regulation of cardiac electrical activity. However, both genes are not required for cardiac pacemaking, but they play essential roles in AV conduction. In order to elucidate the biological importance of cAMP-binding, wild type Popdc1 as well as mutants with a significant reduction in binding affinity for cAMP in vitro were overexpressed in zebrafish embryos. Expression of wild type Popdc1 led to a cardiac insufficiency phenotype characterized by pericardial edema and venous blood retention. Strikingly, the ability of the Popdc1 mutants to induce a cardiac phenotype correlated with the binding affinity for cAMP. These data suggest that cAMP-binding represents an important biological property of the Popdc protein family.