TY - THES A1 - Liu, Ruiqi T1 - Dynamic regulation of the melanocortin 4 receptor system in body weight homeostasis and reproductive maturation in fish T1 - Dynamische Regulation des Melanocortin-4-Rezeptor Systems bei der Körpergewichtshomöostase und der Fortpflanzungsreifung bei Fischen N2 - Puberty is an important period of life with physiological changes to enable animals to reproduce. Xiphophorus fish exhibit polymorphism in body size, puberty timing, and reproductive tactics. These phenotypical polymorphisms are controlled by the Puberty (P) locus. In X. nigrensis and X. multilineatus, the P locus encodes the melanocortin 4 receptor (Mc4r) with high genetic polymorphisms. Mc4r is a member of the melanocortin receptors, belonging to class A G-protein coupled receptors. The Mc4r signaling system consists of Mc4r, the agonist Pomc (precursor of various MSH and of ACTH), the antagonist Agrp and accessory protein Mrap2. In humans, MC4R has a role in energy homeostasis. MC4R and MRAP2 mutations are linked to human obesity but not to puberty. Mc4rs in X. nigrensis and X. multilineatus are present in three allele classes, A, B1 and B2, of which the X-linked A alleles express functional receptors and the male-specific Y-linked B alleles encode defective receptors. Male body sizes are correlated with B allele type and B allele copy numbers. Late-maturing large males carry B alleles in high copy number while early-maturing small males carry B alleles in low copy number or only A alleles. Cell culture co-expression experiments indicated that B alleles may act as dominant negative receptor mutants on A alleles. In this study, the main aim was to biochemically characterize the mechanism of puberty regulation by Mc4r in X. nigrensis and X. multilineatus, whether it is by Mc4r dimerization and/or Mrap2 interaction with Mc4r or other mechanisms. Furthermore, Mc4r in X. hellerii (another swordtail species) and medaka (a model organism phylogenetically close to Xiphophorus) were investigated to understand if the investigated mechanisms are conserved in other species. In medaka, the Mc4r signaling system genes (mc4r, mrap2, pomc, agrp1) are expressed before hatching, with agrp1 being highly upregulated during hatching and first feeding. These genes are mainly expressed in adult brain, and the transcripts of mrap2 co-localize with mc4r indicating a function in modulating Mc4r signaling. Functional comparison between wild-type and mc4r knockout medaka showed that Mc4r knockout does not affect puberty timing but significantly delays hatching due to the retarded embryonic development of knockout medaka. Hence, the Mc4r system in medaka is involved in regulation of growth rather than puberty. In Xiphophorus, expression co-localization of mc4r and mrap2 in X. nigrensis and X. hellerii fish adult brains was characterized by in situ hybridization. In both species, large males exhibit strikingly high expression of mc4r while mrap2 shows similar expression level in the large and small male and female. Differently, X. hellerii has only A-type alleles indicating that the puberty regulation mechanisms evolved independently in Xiphophorus genus. Functional analysis of Mrap2 and Mc4r A/B1/B2 alleles of X. multilineatus showed that increased Mrap2 amounts induce higher cAMP response but EC50 values do not change much upon Mrap2 co-expression with Mc4r (expressing only A allele or A and B1 alleles). A and B1 alleles were expressed higher in large male brains, while B2 alleles were only barely expressed. Mc4r A-B1 cells have lower cAMP production than Mc4r A cells. Together, this indicates a role of Mc4r alleles, but not Mrap2, in puberty onset regulation signaling. Interaction studies by FRET approach evidenced that Mc4r A and B alleles can form heterodimers and homodimers in vitro, but only for a certain fraction of the expressed receptors. Single-molecule colocalization study using super-resolution microscope dSTORM confirmed that only few Mc4r A and B1 receptors co-localized on the membrane. Altogether, the species-specific puberty onset regulation in X. nigrensis and X. multilineatus is linked to the presence of Mc4r B alleles and to some extent to its interaction with A allele gene products. This is reasoned to result in certain levels of cAMP signaling which reaches the dynamic or static threshold to permit late puberty in large males. In summary, puberty onset regulation by dominant negative effect of Mc4r mutant alleles is a special mechanism that is found so far only in X. nigrensis and X. multilineatus. Other Xiphophorus species obviously evolved the same function of the pathway by diverse mechanisms. Mc4r in other fish (medaka) has a role in regulation of growth, reminiscent of its role in energy homeostasis in humans. The results of this study will contribute to better understand the biochemical and physiological functions of the Mc4r system in vertebrates including human. N2 - Die Pubertät ist ein wichtiger Lebensabschnitt mit physiologischen Veränderungen, die die Fortpflanzung von Tieren ermöglichen. Xiphophorus Fische weisen einen Polymorphismus in Bezug auf Körpergröße, Pubertätszeit und Fortpflanzungstaktik auf. Diese phänotypischen Polymorphismen werden durch den Pubertäts (P) Locus gesteuert. In X. nigrensis und X. multilineatus kodiert der P Locus den Melanocortin-4-Rezeptor (Mc4r) mit hohen genetischen Polymorphismen. Mc4r gehört zu den Melanocortin-Rezeptoren, die zur Klasse A der G-Protein-gekoppelten Rezeptoren gehören. Das Mc4r-Signalsystem besteht aus Mc4r, dem Agonisten Pomc (Prohormon der verschiedenen MSH und des ACTH), dem Antagonisten Agrp und dem akzessorischen Protein Mrap2. Beim Menschen spielt MC4R eine Rolle bei der Energiehomöostase. MC4R und MRAP2 Mutationen stehen im Zusammenhang mit menschlicher Fettleibigkeit, jedoch nicht mit der Pubertät. Mc4rs in X. nigrensis und X. multilineatus sind in drei Allelklassen vorhanden, A, B1 und B2, von denen die X-chromosomalen A Allele funktionelle Rezeptoren exprimieren und die spezifischen männlichen Y-chromosomalen B Allele für defekte Rezeptoren kodieren. Die männliche Körpergröße korreliert mit dem B Alleltyp und der Kopienzahl des B Allels. Spätreife große Männchen tragen B Allele in hoher Kopienzahl, während frühreife kleine Männchen B Allele in niedriger Kopienzahl oder nur A Allele tragen. Koexpressions-Experimente in Zellkultur zeigten, dass B Allele als dominant negative Mutanten-Rezeptor auf A Allele wirken können. In dieser Studie war das Hauptziel die biochemische Charakterisierung des Mechanismus der Pubertätsregulation durch Mc4r in X. nigrensis und X. multilineatus. Dabei wurde untersucht, ob die Regulation durch eine Mc4r Dimerisierung und/oder Mrap2 Interaktion mit Mc4r oder durch andere Mechanismen erfolgt. Des Weiteren wurde Mc4r in X. hellerii (einer anderen Schwertträger Art) und Medaka (ein phylogenetisch naheliegender Modellorganismus von Xiphophorus) untersucht, um zu verstehen, ob die untersuchten Mechanismen in anderen Arten konserviert sind. In Medaka werden die Gene des Mc4r Signalsystems (mc4r, mrap2, pomc, agrp1) vor dem Schlüpfen exprimiert, wobei agrp1 während des Schlüpfens und der ersten Fütterung stark hochreguliert wird. Im adulten Medaka werden diese Gene hauptsächlich im Gehirn exprimiert und die Transkripte von mrap2 und mc4r kolokalisieren, was auf eine Funktion bei der Modulation der Mc4r-Signaltransduktion hinweist. Ein funktionaler Vergleich zwischen Wildtyp- und mc4r-Knockout Medaka zeigte, dass der Mc4r-Knockout das Pubertäts-Timing nicht beeinflusst, das Schlüpfen jedoch aufgrund der verzögerten embryonalen Entwicklung von Knockout-Medaka signifikant verzögert. Daher ist das Mc4r System in Medaka eher an der Regulation des Wachstums als an der Pubertät beteiligt. Bei Xiphophorus wurde die Lokalisierung von mc4r und mrap2 in erwachsenen Gehirnen von X. nigrensis und X. hellerii durch in situ Hybridisierung charakterisiert. Bei beiden Spezies zeigen große Männchen eine auffallend hohe Expression von mc4r, während mrap2 bei großen und kleinen Männchen und Weibchen ein ähnliches Expressionsniveau zeigt. Im Gegensatz dazu weist X. hellerii nur Allele vom A-Typ auf, was darauf hinweist, dass sich die Pubertätsregulationsmechanismen in dem Genus Xiphophorus unabhängig voneinander entwickelt haben. Die funktionelle Analyse der Mrap2 und Mc4r A/B1/B2 Allele von X. multilineatus zeigte, dass erhöhte Mrap2-Mengen eine höhere cAMP-Antwort induzieren, die EC50-Werte sich jedoch bei der Mrap2-Coexpression mit Mc4r nicht wesentlich ändern (nur A Allel oder A und B1 Allele). A und B1 Allele wurden in großen männlichen Gehirnen höher exprimiert, während B2 Allele kaum exprimiert wurden. Mc4r A-B1 Zellen haben eine geringere cAMP-Produktion als Mc4r A Zellen. Zusammengenommen deutet dies auf eine Rolle von Mc4r-Allelen, jedoch nicht von Mrap2, bei der Signalgebung zur Regulation des Pubertätsbeginns hin. Interaktionsstudien mit den FRET-Methoden zeigten, dass Mc4r A und B Allele in vitro Heterodimere und Homodimere bilden können, jedoch nur für einen bestimmten Anteil der exprimierten Rezeptoren. Die Einzelmolekül-co-lokalisierungsstudie unter Verwendung von der hochauflösenden Mikroskopiemethode dSTORM bestätigte, dass nur wenige Mc4r A und B1 Rezeptoren auf der Membran co-lokalisiert sind. Insgesamt ist die artspezifische Regulation des Pubertätsbeginns bei X. nigrensis und X. multilineatus auf das Vorhandensein von Mc4r B Allelen und teilweise auf deren Interaktion mit Genprodukten des A Allels zurückzuführen. Dies wird dadurch begründet, dass ein bestimmtes cAMP Niveau (statische oder dynamische Schwelle) erreicht werden muss, um die Pubertät einzuleiten. In großen Männchen wird dieses cAMP Niveau später erreicht und so die Pubertät später eingeleitet. Zusammenfassend ist die Regulation des Pubertätsbeginns durch die dominante negative Wirkung von mutierten Mc4r Allelen ein spezieller Mechanismus, der bisher nur bei X. nigrensis und X. multilineatus zu finden ist. Andere Xiphophorus Arten haben offensichtlich durch andere Mechanismen die gleiche Funktion des Signalwegs entwickelt. In anderen Fischen (Medaka) spielt Mc4r eine Rolle bei der Regulation des Wachstums und erinnert an seine Rolle bei der Energie-Homöostase beim Menschen. Die Ergebnisse dieser Studie werden dazu beitragen, die biochemischen und physiologischen Funktionen des Mc4r-Systems bei Wirbeltieren, einschließlich Menschen, besser zu verstehen. KW - Japankärpfling KW - Mc4r KW - Schwertkärpfling KW - Pubertät KW - Molekularbiologie KW - GPCR KW - Mrap2 KW - Medaka KW - Xiphophorus KW - Puberty KW - Growth Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-206536 ER - TY - JOUR A1 - Adam, Dieter A1 - Maueler, Winfried A1 - Schartl, Manfred T1 - Transcriptional activation of the melanoma inducing Xmrk oncogene in Xiphophorus N2 - The melanoma inducing locus of Xiphophorus encodes a tumorigenic version of a novel putative receptor tyrosine kinase (Xmrk). To elucidate the mechanism of oncogenic activation of Xmrk, we compared the structure and expression of two oncogenic loci with the corresponding proto-oncogene. Only minor structural alterations were found to be specific for the oncogenic Xmrk genes. Marked overexpression of the oncogene transcripts in melanoma, which are approximately 1 kb shorter than the proto-oncogene transcript, correlates with the malignancy of the tumors. The tumor transcripts are derived from an alternative transcription start site that is used only in the oncogenic loci. Thus, oncogenic activation of the melanoma inducing Xmrk gene appears primarily to be due to novel transcriptional control and overexpression. KW - Schwertkärpfling KW - Onkogen KW - Melanom Y1 - 1991 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-87584 ER - TY - JOUR A1 - Schartl, Manfred A1 - Wittbrodt, J. A1 - Mäueler, W. A1 - Raulf, F. A1 - Adam, D. A1 - Hannig, G. A1 - Telling, A. A1 - Storch, F. A1 - Andexinger, S. A1 - Robertson, S. M. T1 - Oncogenes and melanoma formation in Xiphoporus (Teleostei: Poeciliidae) N2 - In Xiphophorus melanoma formation has been attributed by classical genetic findings to the overexpression of a cellular oncogene (Tu) due to elimination of the corresponding regulatory gene locus in hybrids. We have attempted to elucidate this phenomenon on the molecular biological level. Studies on the structure and expression of known proto-oncogenes revealed that several of these genes, especially the c-src gene of Xiphophorus, may act as effectors in establishing the neoplastic phenotype of the melanoma cells . However, these genes appear more to participate in secondary steps of tumorigenesis. Another gene, being termed Xmrk, which represents obviously a so far unknown proto-oncogene but with a cons iderably high similarity to the epidermal growth-factorreceptor gene, was mapped to the Tu-containing region of the chromosome. This gene shows features with respect to its structure and expression that seem to justify it to be regarded as a candidate for a gene involved in the primary processes leading to neoplastic transformation of pigment cells in Xiphophorus. KW - Schwertkärpfling KW - Onkogen KW - Melanom Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-87149 ER - TY - JOUR A1 - Meyer, Manfred K. A1 - Schartl, Manfred T1 - Eine neue Xiphophorus-Art aus Vera Cruz, Mexiko : (Pisces: Poeciliidae) N2 - Xiphophorus andersi n. sp. from the Rio Atoyac, Vera Cruz, Mexico is described: lang head, moderately slender body, large dark black spar at the basis of the anal fin; adult male with short sword-like caudal appendage; rip of ray 5a of gonopodium without a developed claw. Xiphophorus andersi n. sp. differs by the combination of distinct characters from all the other species of the genus known so far. The new species shows features of both the so-called platyfish species group and the so-called swordtail species group. KW - Schwertkärpfling KW - Veracruz Y1 - 1979 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-87124 ER - TY - JOUR A1 - Winkler, Christoph A1 - Hong, Yunhan A1 - Wittbrodt, Joachim A1 - Schartl, Manfred T1 - Analysis of heterologous and homologous promoters and enhancers in vitro and in vivo by gene transfer into Japanese medaka (Oryzias latipes) and Xiphophorus N2 - Efficient expression systems are required for analysis of gene regulation and function in teleost fish. To develop such systems, a nurober of inducible or constitutive promoter and enhancer sequences of fish or higher vertebrate origin were tested for activity in a variety of fish celllines andin embryos of the Japanese medaka fish (Oryzias latipes) and Xiphophorus. The activity of the different promoterenhancer combinations were quantitated. Considerable differences were found for some constructs if tested in vitro or in vivo. From the data obtained, a set of expression vectors for basic research as weH as for aquaculture purposes were established. KW - Schwertkärpfling KW - Japankärpfling KW - Gentransfer KW - Enhancer KW - Promotor KW - In vitro KW - In vivo Y1 - 1992 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-86796 ER - TY - JOUR A1 - Raulf, Friedrich A1 - Mäueler, Winfried A1 - Robertson, Scott M. A1 - Schartl, Manfred T1 - Localization of cellular src mRNA during development and in the differentiated bipolar neurons of the adult neural retina in Xiphophorus N2 - The expression of the c-src gene in embryonie and adult tissue of the teleost fish Xiphophorus helleri was analyzed by in-situ hybridization. The highly conserved fish c-src gene was found to be expressed at high levels in midterm embryos, where c-src mRNA was localized in developing neurons of the sensory layer of the differentiating retina and in the developing brain. In adult tissues the expression of c-src was found to persist in certain cell types of the brain and the neural retina, especially in the bipolar cells of the inner nuclear layer, which are postmitotic, fully differentiated mature neurons. Thus c-src in Xiphophorus appears to be a developmentally regulated proto-oncogene which is important for neuronal differentiation during organogenesis, but whose persistence of expression in certain terminally differentiated neurons strongly suggests a particular maintenance function for c-src in these cells as well. KW - Schwertkärpfling KW - Messenger-RNS Y1 - 1989 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-86703 ER - TY - JOUR A1 - Schartl, A. A1 - Schartl, Manfred A1 - Anders, F. T1 - Promotion and regression of neoplasia by testosterone-promoted cell differentiation in Xiphophorus and Girardinus N2 - No abstract available. KW - Schwertkärpfling KW - Lebendgebärende Zahnkarpfen Y1 - 1982 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-86684 ER - TY - CHAP A1 - Schartl, A. A1 - Schartl, Manfred A1 - Anders, F. T1 - Phenotypic conversion of malignant melanoma to benign melanoma and vice versa in Xiphophorus N2 - No abstract available. KW - Schwertkärpfling KW - Krebs Y1 - 1981 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-86662 ER - TY - CHAP A1 - Anders, F. A1 - Scholl, E. A1 - Schartl, Manfred T1 - Environmental and hereditary factors in the causation of neoplasia, based on studies of the Xiphophorus fish melanoma system N2 - Neoplasia in Xiphophorus can be classified into: a) a Jarge group triggered by carcinogens; b) a large group triggered by promoters; and c) a small group that develops "spontaneously" according to Mendelian Jaw. The process leading to susceptibility for neoplasia is represented by the disintegration of gene systems that normally protect the fish from neoplasia. Interpopulational arid interracial hybridization is the most effective process that Ieads to disintegration of the protective gene systems. Environmental factors may complete disintegration in somatic cells and thus may trigger neoplasia. The applications of the findings on Xiphophorus to humans are discussed. KW - Schwertkärpfling KW - Gen KW - Umweltfaktor KW - Tumor Y1 - 1981 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-86402 ER - TY - CHAP A1 - Anders, Fritz A1 - Schartl, Manfred A1 - Barnekow, Angelika T1 - Xiphophorus as an in vivo model for studies on oncogenes N2 - The capacity of Xiphophorus to develop neoplasia can be formally assigned to a "tumor gene" (Tu), which appears to be a normal part of the genome of all individuals. The wild fish have evolved population-specific and cell type-specific systems of regulatory genes (R) for Tu that protect the fish from neoplasia. Hybridization of members of different wild populations in the laborstory followed by treatment of the hybrids with carcinogens led to disintegration of the R systems permitting excessive expression of Tu and thus resulting in neoplasia. Certain hybrids developed neoplasia even spontaneously. Observations on the genuine phenotypic effect of the derepressed Tu in the early embryo indicated an essential normal function of this oncogene in cell differentiation, proliferation and cell-cell communication. Tu appeared to be indispensable in the genome but may also be present in accessory copics. Recently, c-src, the cellular homolog of the Rous sarcoma virus oncogene v-src, was detected in Xiphophorus. The protein product of c-src, pp60c-src, was identified and then examined by its associated kinase activity. This pp60c-src was found in all individuals tested, but, depending on the genotype, its kinase activity was different. The genetic characters of c-src, such as linkage relations, dosage relations, expression, etc., correspond to those of Tu. From a systematic study which showed that pp60c-src was present in all metazoa tested ranging from mammals down to sponges, we concluded that c-src has evolved with the multicellular organization of animals. Neoplasia of animals and humans is a characteristic closely related to this evolution. Our data showed that small aquariurn fish, besides being used successfully because they are time-, space-, and money-saving systems for carcinogenicity testing, are also highly suitable for basic studies on neoplasia at the populational, morphological, developmental, cell biological, and molecular levels. KW - Schwertkärpfling KW - In vivo KW - Onkogen Y1 - 1984 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-86398 ER - TY - JOUR A1 - Maueler, W. A1 - Barnekow, A. A1 - Eigenbrodt, E. A1 - Raulf, F. A1 - Falk, H. F. A1 - Telling, A. A1 - Schartl, Manfred T1 - Different regulation of oncogene expression in tumor and embryonal cells of Xiphophorus N2 - Melanoma formation in the poeciliid fish Xiphophorus is mediated primarily by a cellular oncogene, designated Tu. Elimination of Tu-specific genes releases the transforming function of Tu and leads to melanoma formation. Southern blot analyses revealed a tight linkage of a v-erb B related gene to the Tu-locus and Northern blot analyses of RNA of solid melanomas indicated a coordinated deregulation and for mutational activation of several oncogenes. In order to get a better insight into the regulation of oncogene expression in normal and transformed cells of Xiphophorus, we studied the expression of Xsrc, Xras, Xmyc, Xerb A, Xsis, and the v-erb B related gene in a melanoma derived cell line (PSM) and an embryonic cell line (A2) under conditions of low growth factor supply. Both celllines express the Xsrc, Xmyc, and Xras genes, while PSM cells in addition express the v-erb B related gene and A2 cells the Xsis gene. In PSM cells serum deprivation leads to an accumulation of most of the oncogene mRNAs analysed. This is most apparent for a 5.0 kb transcript of the v-erb B related gene, probably due to an increase in transcript stability. The levels of these mRNAs returned to normal within 2h after stimulation with 10% fetal calf serum. At the protein level we observed an initial decrease followed by an increase of the n-p60c-src kinase (the protein product of tbe Xsrc gene) activity in cells deprived of serum. Serum stimulation restored a normal pp60"-src kinase activity. In contrast serum deprivation of A2 cells reduced the transcript amounts of each of the oncogenes analysed. The same holds true for one beta-tubulin transcript, while the level of a second beta-tubulin transcript was unaffected. Serum stimulation led to a reactivation of Xras and Xsrc after a delay of approximately 48b. The pp60(c-src) kinase activity was found to be 6-10 times lower as compared to the PSM cells and did not differ between serum deprived and serum stimulated cells. Enzyme activities and isoenzyme patterns of several glycolytic enzymes were found to be not affected by serum deprivation and stimulation in both celllines. KW - Schwertkärpfling KW - Tumorzelle Y1 - 1988 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-86240 ER - TY - JOUR A1 - Mäueler, Winfried A1 - Raulf, Friedrich A1 - Schartl, Manfred T1 - Expression of proto-oncogenes in embryonic, adult, and transformed tissue of Xiphophorus (Teleostei: Poeciliidae) N2 - In Xiphophorus the causative, primary cellular oncogene for melanoma formation has been assigned by classical genetics to a sex-chromosomal locus, designated Tu. Activation of Tu was proposed to be the result of the elimination of Tu-specific regulatory genes which normally suppress the transforming function in the nontumorous state. In order to understand the role which known proto-oncogenes migbt play in this process, we have analysed the expression of src, erb A, erb B, ras, abl, sis and mil related genes from Xiphophorus during embryogenesis, in non-tumorous organs and in melanoma cells. For src, ras, erb B and sis a differential expression during embryogenesis and/or in normal organs was detected, with preferential expression of src in neural tissues, a high abundance of sis transcripts in an embryonal epitheloid cellline and of erbB transcripts in the head nephros. In melanoma cells ras, src and a v-erb B related gene were found to be expressed. The src gene most likely is more involved in secondary processes during tumor progression, while the expression of the v-erb B related gene might be transformation-specific because recently such a sequence was found to map to the close vicinity of the Tu-locus. KW - Schwertkärpfling KW - Protoonkogen KW - Gewebe Y1 - 1988 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-86233 ER - TY - JOUR A1 - Schartl, Angelika A1 - Schartl, Manfred T1 - Genes and cancer: Molecular biology of the melanoma oncogene of Xiphophorus N2 - No abstract available. KW - Schwertkärpfling KW - Krebs Y1 - 1990 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-72670 ER - TY - CHAP A1 - Altschmied, Joachim A1 - Schartl, Manfred T1 - Genetics and molecular biology of tumour formation in Xiphophorus N2 - No abstract available. KW - Schwertkärpfling KW - Tumor KW - Entstehung KW - Molekularbiologie KW - Genetik Y1 - 1994 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-69752 ER - TY - CHAP A1 - Peter, R. U. A1 - Schartl, Manfred A1 - Anders, F. A1 - Duncker, H.-R. T1 - Pigment pattern formation during embryogenesis in Xiphophorus N2 - No abstract available. KW - Schwertkärpfling KW - Embryonalentwicklung KW - Pigmentmuster Y1 - 1985 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-69370 ER - TY - CHAP A1 - Riehl, Rüdiger A1 - Schartl, Manfred A1 - Anders, Fritz T1 - An ultrastructural study of melanoma in Xiphophorus N2 - Melanotic melanoma (MM) of Xiphophorus (Teleostei: Poeciliidae) was studied by conventional preparations and freeze-etch preparations for electron microscopy. MM of Xiphophorus exhibits tightly packed pigment cells with prominent dendritic processes and interdigitations of their plasma membranes. The most impressive feature of MM cells is the occurrence of Iarge lobulated nuclei with numerous nuclear pores and some nuclear pockets. Abundant spheroidal or ellipsoidal melanosomes (diameter 200-650 nm) and vesicular structures are distributed throughout the cellular dendrites, whereas the perinucJear cytoplasm is free of melanosomes. A further characteristic feature of melanoma cells in fish is the occurrence of melanosome complexes (i.e., "compound melanosomes"). These melanosome complexes consist of a few to numerous melanosomes, which are enveloped by a separate rnembrane. Pinocytotic vesicles couJd be demonstrated with distinct differences in frequency and distribution patterns, indicating differences in the metabolic activities of the cells in the same melanoma. Intercellular junctions are lacking in the MM cells. The conventional TEM technique showed clear advantages in the demonstration of intemal architecture of organelles, whereas FE bad considerable potential in respect to the visualization of membrane surface specializations. KW - Schwertkärpfling KW - Krebs KW - Ultrastruktur Y1 - 1985 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-70978 ER - TY - CHAP A1 - Schartl, Manfred A1 - Mäueler, Winfried A1 - Raulf, Friedrich A1 - Robertson, Scott M. T1 - Molecular aspects of melanoma formation in Xiphophorus N2 - No abstract available. KW - Schwertkärpfling KW - Krebs Y1 - 1988 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-72689 ER - TY - CHAP A1 - Anders, F. A1 - Schartl, Manfred A1 - Scholl, E. T1 - Evaluation of environmental and hereditary factors in carcinogenesis, based on studies in Xiphophorus N2 - Neoplasia in Xiphophorus can be classified into a) a large group that is triggered by carcinogens; b) a large group triggered by promoters; c) a small group that develops "spontaneously" following interpopulational and interracial hybridizations; and d) a small group that develops "spontaneously" following germ line mutation. The process leading to susceptibility for neoplasia is represented by the disintegration of gene systems that normally protect the fish from neoplasia. Hybridization is the most effective process that leads to disintegration of the protection gene systems. Environmental factors may complete disintegration and thus may trigger neoplasia. It is discussed whether the findings on Xiphophorus may also apply to humans. KW - Schwertkärpfling KW - Gen KW - Umweltfaktor KW - Carcinogenese Y1 - 1981 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-72741 ER - TY - THES A1 - Regneri, Janine T1 - Transcriptional regulation of cancer genes in the Xiphophorus melanoma system T1 - Transkriptionelle Regulation von Krebsgenen im Xiphophorus-Melanommodell N2 - The Xiphophorus melanoma system is a useful animal model for the study of the genetic basis of tumor formation. The development of hereditary melanomas in interspecific hybrids of Xiphophorus is connected to pigment cell specific overexpression of the mutationally activated receptor tyrosine kinase Xmrk. In purebred fish the oncogenic function of xmrk is suppressed by the molecularly still unidentified locus R. The xmrk oncogene was generated by a gene duplication event from the Xiphophorus egfrb gene and thereby has acquired a new 5’ regulatory sequence, which has probably altered the transcriptional control of the oncogene. So far, the xmrk promoter region was still poorly characterized and the molecular mechanism by which R controls xmrk-induced melanoma formation in Xiphophorus still remained to be elucidated. To test the hypothesis that R controls melanoma development in Xiphophorus on the transcriptional level, the first aim of the thesis was to gain a deeper insight into the transcriptional regulation of the xmrk oncogene. To this end, a quantitative analysis of xmrk transcript levels in different Xiphophorus genotypes carrying either the highly tumorigenic xmrkB or the non-tumorigenic xmrkA allele was performed. I was able to demonstrate that expression of the tumorigenic xmrkB allele is strongly increased in malignant melanomas of R-free backcross hybrids compared to benign lesions, macromelanophore spots, and healthy skin. The expression level of the non-tumorigenic xmrkA allele, in contrast, is not influenced by the presence or absence of R. These findings strongly indicate that differential transcriptional regulation of the xmrk promoter triggers the tumorigenic potential of these xmrk alleles. To functionally characterize the xmrk promoter region, I established a luciferase assay using BAC clones containing the genomic regions where xmrk and egfrb are located for generation of reporter constructs. This approach showed for the first time a melanoma cell specific transcriptional activation of xmrkB by its flanking regions, thereby providing the first functional evidence that the xmrk oncogene is controlled by a pigment cell specific promoter region. Subsequent analysis of different deletion constructs of the xmrkB BAC reporter construct strongly indicated that the regulatory elements responsible for the tumor-inducing overexpression of xmrkB in melanoma cells are located within 67 kb upstream of the xmrk oncogene. Taken together, these data indicate that melanoma formation in Xiphophorus is regulated by a tight transcriptional control of the xmrk oncogene and that the R locus acts through this mechanism. As the identification of the R-encoded gene(s) is necessary to fully understand how melanoma formation in Xiphophorus is regulated, I furthermore searched for alternative R candidate genes in this study. To this end, three genes, which are located in the genomic region where R has been mapped, were evaluated for their potential to be a crucial constituent of the regulator locus R. Among these genes, I identified pdcd4a, the ortholog of the human tumor suppressor gene PDCD4, as promising new candidate, because this gene showed the expression pattern expected from the crucial tumor suppressor gene encoded at the R locus. N2 - Fische der Gattung Xiphophorus sind ein gut etabliertes Modellsystem zur Analyse der genetischen Grundlagen der Tumorentwicklung. Die Entwicklung hereditärer Melanome in bestimmten interspezifischen Xiphophorus-Hybriden wird durch die pigmentzellspezifische Überexpression des Onkogens xmrk ausgelöst. Dieses Gen codiert für eine durch Mutationen aktivierte Rezeptortyrosinkinase. In den reinerbigen Elterntieren wird die onkogene Funktion von xmrk durch den Regulator-Locus R unterdrückt, welcher jedoch auf molekularer Ebene noch nicht identifiziert wurde. Das Onkogen xmrk ist durch eine Genduplikation aus dem Protoonkogen egfrb entstanden und hat dabei eine neue regulatorische 5‘ Region erhalten, welche mit hoher Wahrscheinlichkeit die transkriptionelle Regulation des Onkogens verändert hat. Die Promotorregion von xmrk war allerdings bisher nur unzureichend charakterisiert und der molekulare Mechanismus, durch den der R-Locus die xmrk-induzierte Melanomentwicklung kontrolliert, war noch weitgehend unbekannt. Um zu analysieren, ob der R-Locus die Melanomentwicklung in Xiphophorus auf transkriptioneller Ebene kontrolliert, war das erste Ziel dieser Arbeit die transkriptionelle Regulation des xmrk Onkogens genauer zu untersuchen. Zu diesem Zweck habe ich eine quantitative Analyse der xmrk Expressionslevel in Geweben verschiedener Xiphophorus-Genotypen durchgeführt, welche entweder das stark tumorigene xmrkB oder das nicht tumorigene xmrkA Allel besitzen. Ich konnte zeigen, dass im Vergleich zu benignen Läsionen, Macromelanophoren und gesunder Haut, die Expression des tumorigenen xmrkB Allels in den malignen Melanomen der R-defizienten Rückkreuzungshybride stark erhöht ist. Das Expressionslevel des xmrkA Allels wird hingegen nicht durch den R-Locus beeinflusst. Dieses Ergebnis deutet darauf hin, dass eine differenzielle transkriptionelle Regulierung des xmrk Promotors für die Unterschiede im onkogenen Potential dieser Allele verantwortlich ist. Um die xmrk Promotorregion funktional zu charakterisieren, habe ich in der hier vorliegenden Studie einen Luciferase-Assay etabliert, für den BAC-Klone, welche die xmrk- oder egfrb-Region enthalten, zur Herstellung von Reporterkonstrukten verwendet wurden. Mit Hilfe dieses Ansatzes konnte ich zum ersten Mal eine melanomzellspezifische Aktivierung des xmrkB Gens durch seine regulatorischen Regionen zeigen. Dies liefert den ersten funktionalen Beweis, dass das xmrk Onkogen tatsächlich durch einen pigmentzellspezifischen Promotor kontrolliert wird. Durch die nachfolgende Analyse einer Deletionsserie des xmrkB Reporterkonstrukts konnte gezeigt werden, dass die regulatorischen Elemente, welche die starke Überexpression von xmrk in Melanomzellen steuern, in den proximalen 67 kb der xmrk 5‘ Region lokalisiert sind. Zusammengefasst deuten diese Ergebnisse darauf hin, dass die Melanomentwicklung in Xiphophorus durch eine strikte transkriptionelle Kontrolle des xmrk Onkogens reguliert wird und dass der Regulator-Locus R seine tumorsuppressive Funktion über diesen Mechanismus ausübt. Da die Identifizierung des R-Locus-Gens entscheidend ist, um die Melanomentwicklung in Xiphophorus vollständig zu verstehen, habe ich im zweiten Teil dieser Arbeit drei Gene, welche in derselben genomischen Region liegen in der R lokalisiert wurde, genauer untersucht, um zu testen, ob es sich bei einem dieser Gene um eine entscheidende tumorsuppressive Komponente des R-Locus handelt. Von diesen Genen wurde pdcd4a, welches das Ortholog zum humanen Tumorsuppressorgen PDCD4 ist, als vielversprechendes neues Kandidatengen identifiziert, da das Expressionsmuster von pdcd4a mit dem zu erwartenden Expressionsmuster des am R-Locus codierten Tumorsuppressorgens übereinstimmt. KW - Melanom KW - Schwertkärpfling KW - Chromatophor KW - Epidermaler Wachstumsfaktor KW - Onkogen KW - Tumorsuppressorgen KW - Hybrid KW - transkriptionelle Regulation KW - melanoma KW - Xiphophorus KW - xmrk KW - transcriptional control KW - pigment cell KW - Hautkrebs KW - Epidermaler Wachstumsfaktor-Rezeptor Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-82319 ER - TY - THES A1 - Laisney, Juliette Agnès Geneviève Claire T1 - Characterisation and regulation of the Egfr/Egfr ligand system in fish models for melanoma N2 - Fish of the genus Xiphophorus belong to the oldest animal models in cancer research. The oncogene responsible for the generation of spontaneous aggressive melanoma encodes for a mutated epidermal growth factor receptor (Egfr) and is called xmrk for Xiphophorus melanoma receptor kinase. Xmrk constitutive activation mechanisms and subsequent signaling pathways have already been investigated and charaterized but it is still unknown if Egfr ligands may also play a role in Xmrk-driven melanoma formation. To investigate the potential role of Egfr ligands in Xmrk-driven melanoma, I firstly analyzed the evolution of teleost and tetrapod Egfr/Egfr ligand systems. I especially focused on the analysis on the medaka fish, a closely related species to Xiphophorus, for which the whole genome has been sequenced. I could identify all seven Egfr ligands in medaka and could show that the two teleost-specific Egfr copies of medaka display dissimilar expression patterns in adult tissues together with differential expression of Egfr ligand subsets, arguing for subfunctionalization of receptor functions in this fish. Our phylogenetic and synteny analyses supported the hypothesis that only one gene in the chordate ancestor gave rise to the diversity of Egfr ligands found in vertebrate genomes today. I also could show that the Egfr extracellular subdomains implicated in ligand binding are not evolutionary conserved between tetrapods and teleosts, making the use of heterologous ligands in experiments with fish cells debatable. Despite its well understood and straight-forward process, Xmrk-driven melanomagenesis in Xiphophorus is problematic to further investigate in vivo. Our laboratory recently established a new melanoma animal model by generating transgenic mitf::xmrk medaka fishes, a Xiphophorus closely related species offering many more advantages. These fishes express xmrk under the control of the pigment-cell specific Mitf promoter. During my PhD thesis, I participated in the molecular analysis of the stably transgenic medaka and could show that the Xmrk-induced signaling pathways are similar when comparing Xiphophorus with transgenic mitf::xmrk medaka. These data together with additional RNA expression, protein, and histology analyses showed that Xmrk expression under the control of a pigment cell-specific promoter is sufficient to induce melanoma in the transgenic medaka, which develop very stereotyped tumors, including uveal and extracutaneous melanoma, with early onset during larval stages. To further investigate the potential role of Egfr ligands in Xmrk-driven melanoma, I made use of two model systems. One of them was the above mentioned mitf::xmrk medaka, the other was an in-vitro cell culture system, where the EGF-inducible Xmrk chimera HERmrk is stably expressed in murine melanocytes. Here I could show that HERmrk activation strongly induced expression of amphiregulin (Areg) and heparin-binding EGF-like growth factor (Hbegf) in melanocytes. This regulation was dependent on the MAPK and SRC signaling pathways. Moreover, upregulation of Adam10 and Adam17, the two major sheddases of Egfr ligands, was observed. I also could demonstrate the functionality of the growth factors by invitro analyses. Using the mitf::xmrk medaka model I could also show the upregulation of a subset of ligand genes, namely egf, areg, betacellulin (btc) and epigen (epgn) as well as upregulation of medaka egfrb in tumors from fish with metastatic melanoma. All these results converge to support an Xmrk-induced autocrine Egfr ligand loop. Interestingly, my in-vitro experiments with conditioned supernatant from medaka Egf- and Hbegf-producing cells revealed that not only Xiphophorus Egfrb, but also the pre-activated Xmrk could be further stimulated by the ligands. Altogether, I could show with in-vitro and in-vivo experiments that Xmrk is capable of inducing a functional autocrine Egfr ligand loop. These data confirm the importance of autocrine loops in receptor tyrosine kinase (RTK)-dependent cancer development and show the possibility for a constitutively active RTK to strengthen its oncogenic signaling by ligand binding. N2 - Fische der Gattung Xiphophorus gehören zu den ältesten Tiermodellen für die Krebsforschung. Das im Xiphophorus-System für die Melanomentstehung verantwortliche Onkogen codiert für eine mutierte Version des epidermalen Wachstumsfaktorrezeptors (Egfr) und wird xmrk (für “Xiphophorus melanoma receptor kinase”) genannt. Die konstitutiven Aktivierungsmechanismen dieses Rezeptors und die daraus resultierenden aktivierten Signalwege sind bereits gut untersucht und charakterisiert. Dennoch war bisher unbekannt, ob Egfr-Liganden auch eine Rolle bei der Xmrk-vermittelten Melanomentstehung spielen. Um eine potenzielle Rolle dieser Egfr-Liganden im Xmrk-induzierten Melanom zu erforschen, habe ich zunächst die Evolution des Egfr/Egfr-Liganden-Systems in Teleostiern und Tetrapoden untersucht. Hierfür fokussierte ich mich im besonderen auf den Medaka- Fisch, der zum einen eine nahe evolutionäre Verwandtschaft zu Xiphophorus aufweist und zum anderen – im Gegensatz zu Xiphophorus - ein komplett sequenziertes und gut annotiertes Genom besitzt. Ich konnte alle sieben Egfr-Liganden in Medaka identifizieren und konnte weiterhin zeigen, dass die zwei Teleost-spezifischen Egfr-Kopien dieses Fisches ein unterschiedliches Expressionsmuster in adulten Geweben aufweisen, welches außerdem mit unterschiedlicher Egfr-Liganden-Expression einherging. Diese Daten sprechen für eine Subfunktionalisierung der Egfr-Funktionen in Medaka. Unsere phylogenetischen und Syntenie-Analysen unterstützen die Hypothese, dass nur ein einziges Egfr-Liganden-Gen des Chordaten-Vorfahren der genetische Ursprung für die zahlreichen Egfr-Liganden-Gene, die in heutigen Vertrebraten zu finden sind, darstellt. Ich konnte weiterhin zeigen, dass die an der Ligandenbindung beteiligten Domänen des Egfr nicht zwischen Tetrapoden und Teleostiern konserviert sind. Diese Daten sprechen somit gegen die Verwendung heterologer Liganden in Zellkulturexperimenten mit Fischzellen. Trotz der gut verstandenen Konsequenzen einer Xmrk-Expression auf die Pigmentzelle lässt sich die Xmrk-vermittelte Melanomentstehung in Xiphophorus relativ schwer in vivo untersuchen. In unserem Labor wurde daher kürzlich ein neues Tiermodell für Melanome entwickelt. Dabei handelt es sich um einen mitf::xmrk-transgenen Medaka. Diese Fische exprimieren xmrk unter der Kontrolle des Pigmentzell-spezifischen Mitf-Promoters. Während meiner Doktorarbeit trug ich zur molekularen Analyse der stabil transgenen Tiere bei und konnte zeigen, dass die Xmrk-vermittelte Signalgebung in mitf::xmrk-Medakas der von Xmrk-exprimierenden Xiphophorus-Fischen gleicht. Diese Daten, zusammen mit weiteren RNA-Expressions-, Protein- und histologischen Analysen, zeigten, dass die Expression von xmrk unter der Kontrolle eines Pigmentzellspezifischen Promoters ausreichend für die Melanomentstehung in Medaka ist. Eine Besonderheit dieses Melanommodelles ist die auffallend stereotype Tumorentstehung. Der Beginn der Hyperpigmentierung wird bereits in frühen Larvenstadien sichtbar und führt – je nach Fischlinie – anschließend zuverlässig zu extrakutanen Pigmentzelltumoren oder invasiven bzw. uvealen Melanomen. Um eine potenzielle Funktion der Egfr-Liganden für Xmrk-induzierte Melanome zu untersuchen, machte ich mir zwei Modellsysteme zunutze. Eines der beiden Modelle war der bereits oben erwähnte mitf::xmrk-transgene Medaka, das andere war ein in-vitro- Zellkultursystem, bei dem die EGF-induzierbare Xmrk-Chimäre HERmrk stabil in murinen Melanozyten exprimiert wird. Hier konnte ich zeigen, dass HERmrk-Aktivierung zu einer starken Genexpression der EGFR-Liganden Amphiregulin (Areg) und Heparin-binding EGFlike growth factor (Hbegf) in Melanozyten führte. Diese Regulierung war abhängig von den MAPK- und SRC-Signalwegen. Weiterhin wurde eine Induktion von Adam10 und Adam17, den zwei bedeutsamsten Proteasen zur Freisetzung von EGFR-Liganden (“Sheddasen”), festgestellt. Ich konnte die Funktionalität der so sezernierten Liganden durch in-vitro- Experimente nachweisen. Anhand des mitf::xmrk Medaka-Modelles konnte ich ebenfalls zeigen, dass sowohl mehrere Egfr-Ligandengene, nämlich egf, areg, betacellulin (btc) und epigen (epgn), als auch egfrb in Tumoren von Medaka-Fischen mit metastatischen Melanomen heraufreguliert wurden. All diese Daten lassen auf einen durch Xmrk induzierten autokrinen EGFR-Liganden-Loop schließen. Interessanterweise zeigte sich durch in-vitro- Experimente mit konditioniertem Überstand von Medaka Egf- und Hbegf-produzierenden Zellen, dass nicht nur Xiphophorus Egfrb, sondern auch das bereits aktivierte Xmrk durch beide Liganden weiter stimuliert werden konnte. Zusammengefasst zeigen meine in-vitro- und in-vivo-Daten, dass Xmrk in der Lage ist, einen funktionalen autokrinen Egfr-Liganden-Loop zu induzieren. Dieses Ergebnis unterstreicht die Bedeutung autokriner Loops in Rezeptortyrosinkinasen (RTK)-abhängiger Tumorentstehung und zeigt auf, dass selbst die onkogene Signalgebung prädimerisierter RTKs durch Ligandenbindung verstärkt werden kann. KW - Schwertkärpfling KW - Melanom KW - Epidermaler Wachstumsfaktor-Rezeptor KW - cancer KW - melanoma KW - fish model KW - EGFR Y1 - 2010 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-51369 ER -