TY - THES A1 - Zwettler, Fabian Ulrich T1 - Expansionsmikroskopie kombiniert mit hochauflösender Fluoreszenzmikroskopie T1 - Expansion Microscopy combined with Super-Resolution Fluorescence Microscopy N2 - Fluorescence microscopy is a form of light microscopy that has developed during the 20th century and is nowadays a standard tool in Molecular and Cell biology for studying the structure and function of biological molecules. High-resolution fluorescence microscopy techniques, such as dSTORM (direct Stochastic Optical Reconstruction Microscopy) allow the visualization of cellular structures at the nanometre scale (10−9 m). This has already made it possible to decipher the composition and function of various biopolymers, such as proteins, lipids and nucleic acids, up to the three-dimensional (3D) structure of entire organelles. In practice, however, it has been shown that these imaging methods and their further developments still face great challenges in order to achieve an effective resolution below ∼ 10 nm. This is mainly due to the nature of labelling biomolecules. For the detection of molecular structures, immunostaining is often performed as a standard method. Antibodies to which fluorescent molecules are coupled, recognize and bind specifcally and with high affnity to the molecular section of the target structure, also called epitope or antigen. The fluorescent molecules serve as reporter molecules which are imaged with the use of a fluorescence microscope. However, the size of these labels with a length of about 10-15 nm in the case of immunoglobulin G (IgG) antibodies, cause a detection of the fluorescent molecules shifted to the real position of the studied antigen. In dense regions where epitopes are located close to each other, steric hindrance between antibodies can also occur and leads to an insuffcient label density. Together with the shifted detection of fluorescent molecules, these factors can limit the achievable resolution of a microscopy technique. Expansion microscopy (ExM) is a recently developed technique that achieves a resolution improvement by physical expansion of an investigated object. Therefore, biological samples such as cultured cells, tissue sections, whole organs or isolated organelles are chemically anchored into a swellable polymer. By absorbing water, this so-called superabsorber increases its own volume and pulls the covalently bound biomolecules isotropically apart. Routinely, this method achieves a magnifcation of the sample by about four times its volume. But protocol variants have already been developed that result in higher expansion factors of up to 50-fold. Since the ExM technique includes in the frst instance only the sample treatment for anchoring and magnifcation of the sample, it can be combined with various standard methods of fluorescence microscopy. In theory, the resolution of the used imaging technique improves linearly with the expansion factor of the ExM treated sample. However, an insuffcient label density and the size of the antibodies can here again impair the effective achievable resolution. The combination of ExM with high-resolution fluorescence microscopy methods represents a promising strategy to increase the resolution of light microscopy. In this thesis, I will present several ExM variants I developed which show the combination of ExM with confocal microscopy, SIM (Structured Illumination Microscopy), STED (STimulated Emission Depletion) and dSTORM. I optimized existing ExM protocols and developed different expansion strategies, which allow the combination with the respective imaging technique. Thereby, I gained new structural insights of isolated centrioles from the green algae Chlamydomonas reinhardtii by combining ExM with STED and confocal microscopy. In another project, I combined 3D-SIM imaging with ExM and investigated the molecular structure of the so-called synaptonemal complex. This structure is formed during meiosis in eukaryotic cells and contributes to the exchange of genetic material between homologous chromosomes. Especially in combination with dSTORM, the ExM method showed its high potential to overcome the limitations of modern fluorescence microscopy techniques. In this project, I expanded microtubules in mammalian cells, a polymer of the cytoskeleton as well as isolated centrioles from C. reinhardtii. By labelling after expansion of the samples, I was able to signifcantly reduce the linkage error of the label and achieve an improved label density. In future, these advantages together with the single molecule sensitivity and high resolution obtained by the dSTORM method could pave the way for achieving molecular resolution in fluorescence microscopy N2 - Die Fluoreszenzmikroskopie ist eine Form der Lichtmikroskopie, die sich im Laufe des 20. Jahrhunderts entwickelt hat und heutzutage standardmäßig in der Molekular-und Zellbiologie zur Erforschung von Aufbau und Funktion biologischer Moleküle eingesetzt wird. Hochauflösende Verfahren der Fluoreszenzmikroskopie, wie die dSTORM (direct Stochastic Optical Reconstruction Microscopy) Technik, ermöglichen die Visualisierung zellulärer Strukturen im Nanometer-Größenbereich (10−9 m). Dadurch konnte bereits die Zusammensetzung und Funktion unterschiedlicher Biopolymere, wie die von Proteinen, Lipiden und Nukleinsäuren, bis hin zum dreidimensionalen (3D) Aufbau ganzer Organellen entschlüsselt werden. In der Praxis zeigt sich jedoch, dass diese Bildgebungsverfahren und ihre Weiterentwicklungen immer noch vor großen Herausforderungen stehen, bevor eine effektive Auflösung von unter ∼10 nm erreicht werden kann. Die größte Hürde stellt die Art und Weise der Markierung von Biomolekülen dar. Bei dieser wird zum Nachweis molekularer Strukturen häufig die sogenannte Immunfärbung als Standardmethode eingesetzt. Antikörper, welche mit Fluoreszenzmolekülen gekoppelt werden, erkennen und binden hierbei spezifisch und mit hoher Affinität den Molekülabschnitt der Zielstruktur, auch Epitop oder Antigen genannt. Die Fluoreszenzmoleküle dienen als Reportermoleküle, welche mit Hilfe eines Fluoreszenzmikroskops abgebildet werden. Die Größe der Antikörper, mit einer Länge von etwa 10-15 nm im Falle von Immunglobulin G (IgG) Antikörpern, bewirkt jedoch eine Detektion der fluoreszierenden Moleküle verschoben zur eigentlichen Lage des untersuchten Antigens. In Regionen mit räumlich dicht nebeneinander liegenden Epitopen kann es zusätzlich zur sterischen Hinderung zwischen den Antikörpern kommen. Dies führt zu einer unzureichenden Markierungsdichte und stellt - zusammen mit der verschobenen Detektion der Fluoreszenzmoleküle - eine Limitierung der zu erreichenden Auflösung dar. Die Expansionsmikroskopie (ExM) ist ein neu entwickeltes Verfahren, welches eine Auflösungsverbesserung durch die physikalische Expansion eines untersuchten Objekts erreicht. Hierbei werden biologische Proben, wie beispielsweise kultivierte Zellen, Gewebeschnitte, ganze Organe oder isolierte Organellen, chemisch in ein quellbares Polymer verankert. Durch Absorption von Wasser vergrößert dieser sogenannte Superabsorber sein eigenes Volumen und zieht während der räumlichen Expansion die kovalent gebundenen Biomoleküle isotrop auseinander. Standardmäßig wird durch dieses Verfahren eine Vergrößerung der Proben um etwa das vierfache Volumen erreicht, wobei bereits Protokollvarianten entwickelt wurden, die eine bis zu 50-fache Expansion erzielt haben. Da die ExM-Technik zunächst nur die Probenbehandlung zur Verankerung und Vergrößerung der Probe selbst beinhaltet, kann sie mit unterschiedlichen Standardmethoden der Fluoreszenzmikroskopie kombiniert werden. Dadurch verbessert sich die Auflösung des verwendeten Bildgebungsverfahrens theoretisch linear um den Faktor der Volumenvergrößerung der ExM behandelten Probe. Eine unzureichende Markierungsdichte und die Größe der verwendeten Antikörper können auch hier die effektiv erreichbare Auflösung beeinträchtigen. Die Kombination der ExM mit hochauflösenden Verfahren der Fluoreszenzmikroskopie stellt eine vielversprechende Strategie zur Erhöhung der bisher erreichbaren Auflösung in der Lichtmikroskopie dar. In dieser Arbeit werde ich mehrere von mir entwickelte ExM Varianten vorstellen, welche die Kombination von ExM mit konfokaler Mikroskopie, SIM (Structured Illumination Microscopy), STED (STimulated Emission Depletion) und dSTORM zeigen. Um die Verbindung mit dem jeweiligen Bildgebungsverfahren zu ermöglichen, optimierte ich bestehende ExM-Protokolle und entwickelte unterschiedliche Expansionsstrategien. Dadurch konnte ich neue strukturelle Erkenntnisse von isolierten Zentriolen aus der Grünalge Chlamydomonas reinhardtii durch die Verbindung von ExM mit STED und konfokaler Mikroskopie gewinnen. In einem weiteren Projekt kombinierte ich 3D-SIM mit ExM und untersuchte den molekularen Aufbau des sogenannten synaptonemalen Komplexes. Diese Struktur bildet sich in eukaryotischen Zellen während der Reifeteilung (Meiose) aus und trägt zum Austausch des genetischen Materials zwischen homologen Chromosomen bei. Vor allem in Verbindung mit dSTORM zeigte sich das hohe Potential der ExM-Methode, die bisherigen Limitierungen moderner Techniken der Fluoreszenzmikroskopie zu überwinden. In diesem Projekt expandierte ich Mikrotubuli in Säugetierzellen, ein Polymer des Zytoskeletts, sowie isolierte Zentriolen aus C. reinhardtii. Dadurch, dass die Markierung erst nach dem Expandieren der Proben erfolgte, gelang es, den Abstandsfehler der Markierung deutlich zu verringern und eine verbesserte Markierungsdichte zu erreichen. Diese Vorteile könnten in Verbindung mit der Einzelmolekülsensititvität und hohen Auflösung der dSTORM Methode Wegbereiter zur Erreichung einer molekularen Auflösung sein KW - Fluoreszenzmikroskopie KW - Expansionsmikroskopie KW - Einzelmolekül-Lokalisationsmikroskopie KW - Zentriolen KW - Synaptonemaler Komplex Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-212362 ER - TY - JOUR A1 - Zupanc, Günther K. H. A1 - Rössler, Wolfgang T1 - Government funding of research beyond biomedicine: challenges and opportunities for neuroethology JF - Journal of Comparative Physiology A N2 - Curiosity-driven research is fundamental for neuroethology and depends crucially on governmental funding. Here, we highlight similarities and differences in funding of curiosity-driven research across countries by comparing two major funding agencies—the National Science Foundation (NSF) in the United States and the German Research Foundation (Deutsche Forschungsgemeinschaft, DFG). We interviewed representatives from each of the two agencies, focusing on general funding trends, levels of young investigator support, career-life balance, and international collaborations. While our analysis revealed a negative trend in NSF funding of biological research, including curiosity-driven research, German researchers in these areas have benefited from a robust positive trend in DFG funding. The main reason for the decrease in curiosity-driven research in the US is that the NSF has only partially been able to compensate for the funding gap resulting from the National Institutes of Health restricting their support to biomedical research using select model organisms. Notwithstanding some differences in funding programs, particularly those relevant for scientists in the postdoctoral phase, both the NSF and DFG clearly support curiosity-driven research. KW - German Research Foundation KW - Government research funding KW - National Science Foundation KW - Deutsche Forschungsgemeinschaft KW - neuroethology Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-325113 VL - 208 IS - 3 ER - TY - THES A1 - Zube, Christina T1 - Neuronal representation and processing of chemosensory communication signals in the ant brain N2 - Ants heavily rely on olfaction for communication and orientation and ant societies are characterized by caste- and sex-specific division of labor. Olfaction plays a key role in mediating caste-specific behaviours. I investigated whether caste- and sex-specific differences in odor driven behavior are reflected in specific differences and/or adaptations in the ant olfactory system. In particular, I asked the question whether in the carpenter ant, Camponotus floridanus, the olfactory pathway exhibits structural and/or functional adaptations to processing of pheromonal and general odors. To analyze neuroanatomical specializations, the central olfactory pathway in the brain of large (major) workers, small (minor) workers, virgin queens, and males of the carpenter ant C. floridanus was investigated using fluorescent tracing, immunocytochemistry, confocal microscopy and 3D-analyzes. For physiological analyzes of processing of pheromonal and non-pheromonal odors in the first odor processing neuropil , the antennal lobe (AL), calcium imaging of olfactory projection neurons (PNs) was applied. Although different in total glomerular volumes, the numbers of olfactory glomeruli in the ALs were similar across the female worker caste and in virgin queens. Here the AL contains up to ~460 olfactory glomeruli organized in 7 distinct clusters innervated via 7 antennal sensory tracts. The AL is divided into two hemispheres regarding innervations of glomeruli by PNs with axons leaving via a dual output pathway. This pathway consists of the medial (m) and lateral (l) antenno-cerebral tract (ACT) and connects the AL with the higher integration areas in the mushroom bodies (MB) and the lateral horn (LH). M- and l-ACT PNs differ in their target areas in the MB calyx and the LH. Three additional ACTs (mediolateral - ml) project to the lateral protocerebrum only. Males had ~45% fewer glomeruli compared to females and one of the seven sensory tracts was absent. Despite a substantially smaller number of glomeruli, males possess a dual PN output pathway to the MBs. In contrast to females, however, only a small number of glomeruli were innervated by projection neurons of the m-ACT. Whereas all glomeruli in males were densely innervated by serotonergic processes, glomeruli innervated by sensory tract six lacked serotonergic innervations in the female castes. It appears that differences in general glomerular organization are subtle among the female castes, but sex-specific differences in the number, connectivity and neuromodulatory innervations of glomeruli are substantial and likely to promote differences in olfactory behavior. Calcium imaging experiments to monitor pheromonal and non-pheromonal processing in the ant AL revealed that odor responses were reproducible and comparable across individuals. Calcium responses to both odor groups were very sensitive (10-11 dilution), and patterns from both groups were partly overlapping indicating that processing of both odor classes is not spatially segregated within the AL. Intensity response patterns to the pheromone components tested (trail pheromone: nerolic acid; alarm pheromone: n-undecane), in most cases, remained invariant over a wide range of intensities (7-8 log units), whereas patterns in response to general odors (heptanal, octanol) varied across intensities. Durations of calcium responses to stimulation with the trail pheromone component nerolic acid increased with increasing odor concentration indicating that odor quality is maintained by a stable pattern (concentration invariance) and intensity is mainly encoded in the response durations of calcium activities. For n-undecane and both general odors increasing response dynamics were only monitored in very few cases. In summary, this is the first detailed structure-function analyses within the ant’s central olfactory system. The results contribute to a better understanding of important aspects of odor processing and olfactory adaptations in an insect’s central olfactory system. Furthermore, this study serves as an excellent basis for future anatomical and/or physiological experiments. N2 - Für Ameisen spielt die olfaktorische Kommunikation und Orientierung eine zentrale Rolle hinsichtlich der Organisation des Ameisenstaates. Ob sich kasten- und geschlechtsspezifische Verhaltensunterschiede auf neuronaler Ebene und besonders im olfaktorischen System der Ameise widerspiegeln ist die zentrale Frage meiner Arbeit. Im Speziellen stellte ich die Frage, ob sich in der olfaktorischen Bahn der Rossameise Camponotus floridanus strukturelle oder funktionelle Anpassungen an die Verarbeitung von Pheromonen und generellen Düften aufzeigen lassen. Zur Analyse hinsichtlich neuroanatomischer Spezialisierungen wurde die olfaktorische Bahn im Gehirn von großen und kleinen Arbeiterinnen, Jungköniginnen und Männchen der Rossameise C. floridanus mittels Fluoreszenzmassenfärbungen, Immunzytochemie, konfokaler Laserscanningmikroskopie und 3D-Auswertung untersucht. Um die Verarbeitung von Pheromonen und generellen Düften im primären olfaktorischen Neuropil, dem Antennallobus (AL), auf physiologischer Ebene zu charakterisieren wurden olfaktorische Projektionsneurone mittels Calcium Imaging untersucht. Obwohl sich das glomeruläre Gesamtvolumen der ALs zwischen Arbeiterinnenkasten und Jungköniginnen unterscheidet, lag die Gesamtzahl der Glomeruli im AL in einem ähnlichen Bereich. Der AL besteht in allen drei weiblichen Kasten aus bis zu 460 Glomeruli, die in sieben Clustern angeordnet sind und von sieben sensorischen Eingangstrakten innerviert werden. Der AL unterteilt sich in zwei Hemispheren, deren entsprechende Glomeruli von Projektionsneuronen innverviert werden, die vom AL über die Nervenbahn des “dual output pathway” in höhere Hirnregionen projizieren. Diese Nervenbahn besteht aus dem medialen (m) und lateralen (l) Antennocerebraltrakt (ACT) und verbindet den AL mit höheren Integrationszentren wie den Pilzkörpern (MB) und dem lateralen Horn (LH). M- und l-ACT unterscheiden sich in ihren Zielregionen im MB Calyx und dem LH. Drei weitere ACTs (mediolateral – ml) projizieren ausschließlich ins laterale Protocerebrum. Männchen besitzen ca. 45% weniger Glomeruli im Vergleich zur Weibchenkaste. Ihnen fehlt weiterhin einer der sieben sensorischen Eingangstrakte vollständig. Trotz der wesentlich geringeren Anzahl an Glomeruli, besitzen auch Männchen den “dual output pathway”. Im Gegensatz zu den Weibchen ist allerdings nur eine geringe Anzahl an Glomeruli durch m-ACT Projektionsneurone innerviert. Ein weiterer Unterschied im AL von Männchen und Weibchen findet sich in den Glomeruli des sensorische Trakts Nummer sechs, die bei Weibchen keinerlei serotonerge Innervierung aufweisen während beim Männchen der gesamte AL dichte serotonerge Verzweigungen besitzt. Es zeigt sich somit, dass die kastenspezifischen Unterschiede in der allgmeinen glomerulären Organisation des AL innerhalb der Weibchenkaste nur sehr fein sind. Im Gegensatz dazu sind die geschlechtsspezifischen Unterschiede in Anzahl, Konnektivität und neuromodulatorischer Innervierung von Glomeruli zwischen Weibchen- und Männchen wesentlich ausgeprägter was Unterschiede in olfaktorisch geprägten Verhaltensweisen begünstigen könnte. Die Calcium Imaging Experimente zur Untersuchung der Verarbeitung von Pheromonen und generellen Düften im AL der Ameise zeigten, dass Duftantworten reproduzierbar und zwischen Individuen vergleichbar waren. Die Sensitivität des Calcium Signals lag für beide Duftgruppen in einem sehr niedrigen Bereich (Verdünnung 10-11). Die Antortmuster beider Duftgruppen überlappten zum Teil, was die Annahme zuläßt, dass die Verarbeitung von Pheromonen und generellen Düften keiner räumlichen Trennung innerhalb des AL unterliegt. Die Intensität der Antwortmuster auf die Pheromonkomponenten (Spurpheromon: Nerolsäure; Alarmpheromon: n-Undecan) blieben in den meisten Fällen über einen weiten Konzentrationsbereich konstant (7-8 log Einheiten). Die Dauer der Calciumantwort nach Stimulation mit Nerolsäure verlängerte sich mit steigender Duftkonzentration. Dies läßt für das Spurpheromon den Schluß zu, dass die Duftqualität in einem konstanten Duftmuster (Konzentrationsinvarianz) repräsentiert und die Duftintensität über die Dauer des Calciumsignals abgebildet wird. Da die Antwortmuster auf generelle Düfte (Heptanal, Octanol) dagegen sehr viel stärker innerhalb des getesteten Konzentrationsbereichs varrieren ließ sich für n-Undecan und die beiden generellen Düfte eine solche Dynamik nur in einigen wenigen Fällen beobachtet. Zusammenfassend ist diese Studie die erste strukturelle und funktionelle Studie des olfaktorischen Systems der Ameise. Die Ergebnisse tragen zu einem besseren Verständnis der neuronalen Adaptationen und Mechanismen hinsichtlich Duftverarbeitung im zentralen Nervensystem von Insekten bei. Außerdem liefert diese Studie eine wichtige Grundlage für zukünftige neuroanatomische und –physiologische Untersuchungen auf dem Gebiet der Neurobiologie der Insekten. KW - Gehirn KW - Neuroethologie KW - Neuroanatomie KW - Geruchswahrnehmung KW - Neuronale Plastizität KW - Insekten KW - Antennallobus KW - Glomeruli KW - olfaktorische Bahn KW - Camponotus floridanus KW - Dufverarbeitung KW - antennal lobe KW - glomeruli KW - olfactory pathway KW - Campontous floridanus KW - odor processing Y1 - 2008 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-30383 ER - TY - JOUR A1 - Zoltner, Martin A1 - Krienitz, Nina A1 - Field, Mark C. A1 - Kramer, Susanne T1 - Comparative proteomics of the two T. brucei PABPs suggests that PABP2 controls bulk mRNA JF - PLoS Neglected Tropical Diseases N2 - Poly(A)-binding proteins (PABPs) regulate mRNA fate by controlling stability and translation through interactions with both the poly(A) tail and eIF4F complex. Many organisms have several paralogs of PABPs and eIF4F complex components and it is likely that different eIF4F/PABP complex combinations regulate distinct sets of mRNAs. Trypanosomes have five eIF4G paralogs, six of eIF4E and two PABPs, PABP1 and PABP2. Under starvation, polysomes dissociate and the majority of mRNAs, most translation initiation factors and PABP2 reversibly localise to starvation stress granules. To understand this more broadly we identified a protein interaction cohort for both T. brucei PABPs by cryo-mill/affinity purification-mass spectrometry. PABP1 very specifically interacts with the previously identified interactors eIF4E4 and eIF4G3 and few others. In contrast PABP2 is promiscuous, with a larger set of interactors including most translation initiation factors and most prominently eIF4G1, with its two partners TbG1-IP and TbG1-IP2. Only RBP23 was specific to PABP1, whilst 14 RNA-binding proteins were exclusively immunoprecipitated with PABP2. Significantly, PABP1 and associated proteins are largely excluded from starvation stress granules, but PABP2 and most interactors translocate to granules on starvation. We suggest that PABP1 regulates a small subpopulation of mainly small-sized mRNAs, as it interacts with a small and distinct set of proteins unable to enter the dominant pathway into starvation stress granules and localises preferentially to a subfraction of small polysomes. By contrast PABP2 likely regulates bulk mRNA translation, as it interacts with a wide range of proteins, enters stress granules and distributes over the full range of polysomes. KW - Trypanosoma KW - mRNA KW - T. brucei KW - PABPs Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-177126 VL - 12 IS - 7 ER - TY - JOUR A1 - Zoephel, Judith A1 - Reiher, Wencke A1 - Rexer, Karl-Heinz A1 - Kahnt, Jörg A1 - Wegener, Christian T1 - Peptidomics of the Agriculturally Damaging Larval Stage of the Cabbage Root Fly Delia radicum (Diptera: Anthomyiidae) JF - PLoS One N2 - The larvae of the cabbage root fly induce serious damage to cultivated crops of the family Brassicaceae. We here report the biochemical characterisation of neuropeptides from the central nervous system and neurohemal organs, as well as regulatory peptides from enteroendocrine midgut cells of the cabbage maggot. By LC-MALDI-TOF/TOF and chemical labelling with 4-sulfophenyl isothiocyanate, 38 peptides could be identified, representing major insect peptide families: allatostatin A, allatostatin C, FMRFamide-like peptides, kinin, CAPA peptides, pyrokinins, sNPF, myosuppressin, corazonin, SIFamide, sulfakinins, tachykinins, NPLP1-peptides, adipokinetic hormone and CCHamide 1. We also report a new peptide (Yamide) which appears to be homolog to an amidated eclosion hormone-associated peptide in several Drosophila species. Immunocytochemical characterisation of the distribution of several classes of peptide-immunoreactive neurons and enteroendocrine cells shows a very similar but not identical peptide distribution to Drosophila. Since peptides regulate many vital physiological and behavioural processes such as moulting or feeding, our data may initiate the pharmacological testing and development of new specific peptide-based protection methods against the cabbage root fly and its larva. KW - adult drosophila KW - central-nervous-system KW - blowfly calliphora-vomitoria KW - drosophila melanogaster KW - mass spectometry KW - feeding behavior KW - fruit fly KW - functional characterization KW - immunoreactive neurons KW - neobellieria bullata Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-131727 VL - 7 IS - 7 ER - TY - JOUR A1 - Zirkel, J. A1 - Cecil, A. A1 - Schäfer, F. A1 - Rahlfs, S. A1 - Ouedraogo, A. A1 - Xiao, K. A1 - Sawadogo, S. A1 - Coulibaly, B. A1 - Becker, K. A1 - Dandekar, T. T1 - Analyzing Thiol-Dependent Redox Networks in the Presence of Methylene Blue and Other Antimalarial Agents with RT-PCR-Supported in silico Modeling JF - Bioinformatics and Biology Insights N2 - BACKGROUND: In the face of growing resistance in malaria parasites to drugs, pharmacological combination therapies are important. There is accumulating evidence that methylene blue (MB) is an effective drug against malaria. Here we explore the biological effects of both MB alone and in combination therapy using modeling and experimental data. RESULTS: We built a model of the central metabolic pathways in P. falciparum. Metabolic flux modes and their changes under MB were calculated by integrating experimental data (RT-PCR data on mRNAs for redox enzymes) as constraints and results from the YANA software package for metabolic pathway calculations. Several different lines of MB attack on Plasmodium redox defense were identified by analysis of the network effects. Next, chloroquine resistance based on pfmdr/and pfcrt transporters, as well as pyrimethamine/sulfadoxine resistance (by mutations in DHF/DHPS), were modeled in silico. Further modeling shows that MB has a favorable synergism on antimalarial network effects with these commonly used antimalarial drugs. CONCLUSIONS: Theoretical and experimental results support that methylene blue should, because of its resistance-breaking potential, be further tested as a key component in drug combination therapy efforts in holoendemic areas. KW - methylene blue KW - malaria KW - elementary mode analysis KW - drug KW - resistance KW - combination therapy KW - pathway KW - metabolic flux Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-123751 N1 - This is an open access article. Unrestricted non-commercial use is permitted provided the original work is properly cited. VL - 6 ER - TY - CHAP A1 - Zimmermann, U. A1 - Stopper, Helga T1 - Electrofusion and electropermeabilization of cells N2 - No abstract available. KW - Elektrofusion KW - Elektroporation KW - Zelle Y1 - 1987 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-73065 ER - TY - JOUR A1 - Zimmermann, Henriette A1 - Subota, Ines A1 - Batram, Christopher A1 - Kramer, Susanne A1 - Janzen, Christian J. A1 - Jones, Nicola G. A1 - Engstler, Markus T1 - A quorum sensing-independent path to stumpy development in Trypanosoma brucei JF - PLoS Pathogens N2 - For persistent infections of the mammalian host, African trypanosomes limit their population size by quorum sensing of the parasite-excreted stumpy induction factor (SIF), which induces development to the tsetse-infective stumpy stage. We found that besides this cell density-dependent mechanism, there exists a second path to the stumpy stage that is linked to antigenic variation, the main instrument of parasite virulence. The expression of a second variant surface glycoprotein (VSG) leads to transcriptional attenuation of the VSG expression site (ES) and immediate development to tsetse fly infective stumpy parasites. This path is independent of SIF and solely controlled by the transcriptional status of the ES. In pleomorphic trypanosomes varying degrees of ES-attenuation result in phenotypic plasticity. While full ES-attenuation causes irreversible stumpy development, milder attenuation may open a time window for rescuing an unsuccessful antigenic switch, a scenario that so far has not been considered as important for parasite survival. KW - Trypanosoma KW - hyperexpression techniques KW - parasitic cell cycles KW - cloning KW - cell cycle and cell division KW - cell differentiation KW - tetracyclines KW - parasitic diseases Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-158230 VL - 13 IS - 4 ER - TY - THES A1 - Zimmermann, Henriette T1 - Antigenic variation and stumpy development in \(Trypanosoma\) \(brucei\) T1 - Antigene Variation und Stumpy Entwicklung in \(Trypanosoma\) \(brucei\) N2 - The eukaryotic parasite Trypanosoma brucei has evolved sophisticated strategies to persist within its mammalian host. Trypanosomes evade the hosts' immune system by antigenic variation of their surface coat, consisting of variant surface glycoproteins (VSGs). Out of a repertoire of thousands of VSG genes, only one is expressed at any given time from one of the 15 telomeric expression sites (ES). The VSG is stochastically exchanged either by a transcriptional switch of the active ES (in situ switch) or by a recombinational exchange of the VSG within the active ES. However, for infections to persist, the parasite burden has to be limited. The slender (sl) bloodstream form secretes the stumpy induction factor (SIF), which accumulates with rising parasitemia. SIF induces the irreversible developmental transition from the proliferative sl to the cell cycle-arrested but fly-infective stumpy (st) stage once a concentration threshold is reached. Thus, antigenic variation and st development ensure persistent infections and transmissibility. A previous study in monomorphic cells indicated that the attenuation of the active ES could be relevant for the development of trypanosomes. The present thesis investigated this hypothesis using the inducible overexpression of an ectopic VSG in pleomorphic trypanosomes, which possess full developmental competence. These studies revealed a surprising phenotypic plasticity: while the endogenous VSG was always down-regulated upon induction, the ESactivity determined whether the VSG overexpressors arrested in growth or kept proliferating. Full ES-attenuation induced the differentiation of bona fide st parasites independent of the cell density and thus represents the sole natural SIF-independent differentiation trigger to date. A milder decrease of the ES-activity did not induce phenotypic changes, but appeared to prime the parasites for SIF-induced differentiation. These results demonstrate that antigenic variation and development are linked and indicated that the ES and the VSG are independently regulated. Therefore, I investigated in the second part of my thesis how ES-attenuation and VSG-silencing can be mediated. Integration of reporters with a functional or defective VSG 3'UTR into different genomic loci showed that the maintenance of the active state of the ES depends on a conserved motif within the VSG 3'UTR. In situ switching was only triggered when the telomere-proximal motif was partially deleted, suggesting that it serves as a DNA-binding motif for a telomere-associated protein. The VSG levels seem to be additionally regulated in trans based on the VSG 3'UTR independent of the genomic context, which was reinforced by the regulation of a constitutively expressed reporter with VSG 3' UTR upon ectopic VSG overexpression. N2 - Der eukaryotische Parasit Trypanosoma brucei hat komplexe Strategien entwickelt, um in seinem Säugetierwirt zu überleben. Die Grundlage der Immunevasion ist die antigene Variation des Oberflächenmantels, der aus dem variablen Oberflächenglykoprotein (VSG) besteht. Von mehreren tausend VSG-Genen wird zu jedem Zeitpunkt nur ein einziges aus einer der 15 telomerischen Expressionsstellen (ES) exprimiert. Das VSG kann entweder durch einen transkriptionellen Wechsel der aktiven ES (in situ Wechsel) oder durch einen rekombinatorischen Wechsel des VSG-Gens innerhalb der aktiven ES stochastisch ausgetauscht werden. Damit jedoch eine langanhaltende Infektion des Wirts möglich wird, muss gleichzeitig der Parasitenbefall begrenzt werden. Mit ansteigender Parasitämie akkumuliert der 'stumpy induction factor' (SIF), welcher von der 'slender' (sl) Blutstromform sekretiert wird. Sobald ein Schwellenwert in der SIF-Konzentration erreicht ist, wird die irreversible Differenzierung der proliferativen sl in die zellzyklusarretierte 'stumpy'(st) Form eingeleitet, welche infektiös für den Fliegenvektor ist. Somit stellen antigene Variation und st- Differenzierung das Persistieren der Infektion und die Übertragung des Parasiten sicher. Eine frühere Arbeit mit monomorphen Zellen deutete darauf hin, dass die Attenuierung der aktiven ES eine Rolle für die Differenzierung der Trypanosomen spielen könnte. Diese Hypothese wurde in der vorliegenden Dissertation untersucht, indem in pleomorphen Zellen mit vollständiger Entwicklungskompetenz ein ektopisches VSG induzierbar überexprimiert wurde. Diese Studien offenbarten eine erstaunliche phänotypische Plastizität: während das endogene VSG nach Induktion runter reguliert wurde, arretierten die VSG-Überexpressoren in Abhängigkeit von der ES-Aktivität entweder im Wachstum oder teilten sich weiter. Die vollständige ES-Attenuierung löste die Differenzierung zu echten st Zellen unabhängig von der Zelldichte aus und ist somit der bisher einzige natürliche SIF-unabhängige Differenzierungsauslöser. Eine mildere Abnahme der ES-Aktivität verursachte keinen Phänotyp, scheint aber die Zellen auf die SIF-induzierte Differenzierung vorzubereiten. Diese Ergebnisse zeigen, dass antigene Variation und Differenzierung verbunden sind und deuteten an, dass die ES und das VSG unabhängig voneinander reguliert werden. Daher habe ich im zweiten Teil meiner Dissertation untersucht, wie ES-Attenuierung und VSG-Stilllegung vermittelt werden können. Die Integration eines Reporters mit funktioneller oder defekter VSG 3'UTR an verschiedenen Orten im Genom zeigte, dass die Aufrechterhaltung der ES-Aktivität von einem konservierten Motiv in der VSG 3'UTR abhängig ist. Ein in situ Wechsel wurde nur ausgelöst, wenn Teile des Telomer-proximalen Motiv deletiert wurden, was nahelegt, dass das Motiv auf DNA-Ebene von einem Telomerbindeprotein erkannt wird. Die VSG-Level scheinen unabhängig vom genomischen Kontext zusätzlich in trans basierend auf der VSG 3'UTR reguliert zu werden, was durch die Regulation eines konstitutiv exprimierten Reporters mit VSG 3'UTR nach VSG-Überexpression bekräftigt wurde. KW - Trypanosoma brucei KW - Genexpression KW - Entwicklung KW - Parasit KW - VSG KW - antigenic variation KW - monoallelic expression KW - stumpy development KW - differentiation Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-146902 ER - TY - JOUR A1 - Zielewska-Büttner, Katarzyna A1 - Heurich, Marco A1 - Müller, Jörg A1 - Braunisch, Veronika T1 - Remotely Sensed Single Tree Data Enable the Determination of Habitat Thresholds for the Three-Toed Woodpecker (Picoides tridactylus) JF - Remote Sensing N2 - Forest biodiversity conservation requires precise, area-wide information on the abundance and distribution of key habitat structures at multiple spatial scales. We combined airborne laser scanning (ALS) data with color-infrared (CIR) aerial imagery for identifying individual tree characteristics and quantifying multi-scale habitat requirements using the example of the three-toed woodpecker (Picoides tridactylus) (TTW) in the Bavarian Forest National Park (Germany). This bird, a keystone species of boreal and mountainous forests, is highly reliant on bark beetles dwelling in dead or dying trees. While previous studies showed a positive relationship between the TTW presence and the amount of deadwood as a limiting resource, we hypothesized a unimodal response with a negative effect of very high deadwood amounts and tested for effects of substrate quality. Based on 104 woodpecker presence or absence locations, habitat selection was modelled at four spatial scales reflecting different woodpecker home range sizes. The abundance of standing dead trees was the most important predictor, with an increase in the probability of TTW occurrence up to a threshold of 44–50 dead trees per hectare, followed by a decrease in the probability of occurrence. A positive relationship with the deadwood crown size indicated the importance of fresh deadwood. Remote sensing data allowed both an area-wide prediction of species occurrence and the derivation of ecological threshold values for deadwood quality and quantity for more informed conservation management. KW - deadwood KW - standing deadwood KW - dead tree KW - snags KW - three-toed woodpecker (Picoides tridactylus) KW - habitat suitability model (HSM) KW - habitat requirements KW - airborne laser scanning (ALS) KW - CIR aerial imagery Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-197565 SN - 2072-4292 VL - 10 IS - 12 ER - TY - JOUR A1 - Ziegler, Sabrina A1 - Weiss, Esther A1 - Schmitt, Anna-Lena A1 - Schlegel, Jan A1 - Burgert, Anne A1 - Terpitz, Ulrich A1 - Sauer, Markus A1 - Moretta, Lorenzo A1 - Sivori, Simona A1 - Leonhardt, Ines A1 - Kurzai, Oliver A1 - Einsele, Hermann A1 - Loeffler, Juergen T1 - CD56 Is a Pathogen Recognition Receptor on Human Natural Killer Cells JF - Scientific Reports N2 - Aspergillus (A.) fumigatus is an opportunistic fungal mold inducing invasive aspergillosis (IA) in immunocompromised patients. Although antifungal activity of human natural killer (NK) cells was shown in previous studies, the underlying cellular mechanisms and pathogen recognition receptors (PRRs) are still unknown. Using flow cytometry we were able to show that the fluorescence positivity of the surface receptor CD56 significantly decreased upon fungal contact. To visualize the interaction site of NK cells and A. fumigatus we used SEM, CLSM and dSTORM techniques, which clearly demonstrated that NK cells directly interact with A. fumigatus via CD56 and that CD56 is re-organized and accumulated at this interaction site time-dependently. The inhibition of the cytoskeleton showed that the receptor re-organization was an active process dependent on actin re-arrangements. Furthermore, we could show that CD56 plays a role in the fungus mediated NK cell activation, since blocking of CD56 surface receptor reduced fungal mediated NK cell activation and reduced cytokine secretion. These results confirmed the direct interaction of NK cells and A. fumigatus, leading to the conclusion that CD56 is a pathogen recognition receptor. These findings give new insights into the functional role of CD56 in the pathogen recognition during the innate immune response. KW - pattern recognition receptors KW - fungal infection KW - Aspergillus fumigatus KW - natural killer cells Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-170637 VL - 7 IS - 6138 ER - TY - JOUR A1 - Ziegler, Alice A1 - Meyer, Hanna A1 - Otte, Insa A1 - Peters, Marcell K. A1 - Appelhans, Tim A1 - Behler, Christina A1 - Böhning-Gaese, Katrin A1 - Classen, Alice A1 - Detsch, Florian A1 - Deckert, Jürgen A1 - Eardley, Connal D. A1 - Ferger, Stefan W. A1 - Fischer, Markus A1 - Gebert, Friederike A1 - Haas, Michael A1 - Helbig-Bonitz, Maria A1 - Hemp, Andreas A1 - Hemp, Claudia A1 - Kakengi, Victor A1 - Mayr, Antonia V. A1 - Ngereza, Christine A1 - Reudenbach, Christoph A1 - Röder, Juliane A1 - Rutten, Gemma A1 - Schellenberger Costa, David A1 - Schleuning, Matthias A1 - Ssymank, Axel A1 - Steffan-Dewenter, Ingolf A1 - Tardanico, Joseph A1 - Tschapka, Marco A1 - Vollstädt, Maximilian G. R. A1 - Wöllauer, Stephan A1 - Zhang, Jie A1 - Brandl, Roland A1 - Nauss, Thomas T1 - Potential of airborne LiDAR derived vegetation structure for the prediction of animal species richness at Mount Kilimanjaro JF - Remote Sensing N2 - The monitoring of species and functional diversity is of increasing relevance for the development of strategies for the conservation and management of biodiversity. Therefore, reliable estimates of the performance of monitoring techniques across taxa become important. Using a unique dataset, this study investigates the potential of airborne LiDAR-derived variables characterizing vegetation structure as predictors for animal species richness at the southern slopes of Mount Kilimanjaro. To disentangle the structural LiDAR information from co-factors related to elevational vegetation zones, LiDAR-based models were compared to the predictive power of elevation models. 17 taxa and 4 feeding guilds were modeled and the standardized study design allowed for a comparison across the assemblages. Results show that most taxa (14) and feeding guilds (3) can be predicted best by elevation with normalized RMSE values but only for three of those taxa and two of those feeding guilds the difference to other models is significant. Generally, modeling performances between different models vary only slightly for each assemblage. For the remaining, structural information at most showed little additional contribution to the performance. In summary, LiDAR observations can be used for animal species prediction. However, the effort and cost of aerial surveys are not always in proportion with the prediction quality, especially when the species distribution follows zonal patterns, and elevation information yields similar results. KW - biodiversity KW - species richness KW - LiDAR KW - elevation KW - partial least square regression KW - arthropods KW - birds KW - bats KW - predictive modeling Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-262251 SN - 2072-4292 VL - 14 IS - 3 ER - TY - JOUR A1 - Zhu, Min A1 - Shabala, Lana A1 - Cuin, Tracey A A1 - Huang, Xin A1 - Zhou, Meixue A1 - Munns, Rana A1 - Shabala, Sergey T1 - Nax loci affect SOS1-like Na\(^{+}\)/H\(^{+}\) exchanger expression and activity in wheat JF - Journal of Experimental Botany N2 - Salinity stress tolerance in durum wheat is strongly associated with a plant’s ability to control Na\(^{+}\) delivery to the shoot. Two loci, termed Nax1 and Nax2, were recently identified as being critical for this process and the sodium transporters HKT1;4 and HKT1;5 were identified as the respective candidate genes. These transporters retrieve Na\(^{+}\) from the xylem, thus limiting the rates of Na\(^{+}\) transport from the root to the shoot. In this work, we show that the Nax loci also affect activity and expression levels of the SOS1-like Na\(^{+}\)/H\(^{+}\) exchanger in both root cortical and stelar tissues. Net Na\(^{+}\) efflux measured in isolated steles from salt-treated plants, using the non-invasive ion flux measuring MIFE technique, decreased in the sequence: Tamaroi (parental line)>Nax1=Nax2>Nax1:Nax2 lines. This efflux was sensitive to amiloride (a known inhibitor of the Na\(^{+}\)/H\(^{+}\) exchanger) and was mirrored by net H\(^{+}\) flux changes. TdSOS1 relative transcript levels were 6–10-fold lower in Nax lines compared with Tamaroi. Thus, it appears that Nax loci confer two highly complementary mechanisms, both of which contribute towards reducing the xylem Na\(^{+}\) content. One enhances the retrieval of Na\(^{+}\) back into the root stele via HKT1;4 or HKT1;5, whilst the other reduces the rate of Na\(^{+}\) loading into the xylem via SOS1. It is suggested that such duality plays an important adaptive role with greater versatility for responding to a changing environment and controlling Na\(^{+}\) delivery to the shoot. KW - HKT transporter KW - potassium KW - salinity stress KW - sequestration KW - sodium KW - xylem loading Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-150236 VL - 67 IS - 3 ER - TY - THES A1 - Zhu, Ana Cheng T1 - Metagenomic analysis of genetic variation in human gut microbial species T1 - Metagenomische Analysen der genetischen Variationen in menschlichen Darmbakterien N2 - Microbial species (bacteria and archaea) in the gut are important for human health in various ways. Not only does the species composition vary considerably within the human population, but each individual also appears to have its own strains of a given species. While it is known from studies of bacterial pan-genomes, that genetic variation between strains can differ considerably, such as in Escherichia coli, the extent of genetic variation of strains for abundant gut species has not been surveyed in a natural habitat. This is mainly due to the fact that most of these species cannot be cultured in the laboratory. Genetic variation can range from microscale genomic rearrangements such as small nucleotide polymorphism (SNP) to macroscale large genomic rearrangements like structural variations. Metagenomics offers an alternative solution to study genetic variation in prokaryotes, as it involves DNA sequencing of the whole community directly from the environment. However, most metagenomic studies to date only focus on variation in gene abundance and hence are not able to characterize genetic variation (in terms of presence or absence of SNPs and genes) of gut microbial strains of individuals. The aim of my doctorate studies was therefore to study the extent of genetic variation in the genomic sequence of gut prokaryotic species and its phenotypic effects based on: (1) the impact of SNP variation in gut bacterial species, by focusing on genes under selective pressure and (2) the gene content variation (as a proxy for structural variation) and their effect on microbial species and the phenotypic traits of their human host. In the first part of my doctorate studies, I was involved in a project in which we created a catalogue of 10.3 million SNPs in gut prokaryotic species, based on metagenomes. I used this to perform the first SNP-based comparative study of prokaryotic species evolution in a natural habitat. Here, I found that strains of gut microbial species in different individuals evolve at more similar rates than the strains within an individual. In addition, I found that gene evolution can be uncoupled from the evolution of its originating species, and that this could be related to selective pressure such as diet, exemplified by galactokinase gene (galK). Despite the individuality (i.e. uniqueness of each individual within the studied metagenomic dataset) in the SNP profile of the gut microbiota that we found, for most cases it is not possible to link SNPs with phenotypic differences. For this reason I also used gene content as a proxy to study structural variation in metagenomes. In the second part of my doctorate studies, I developed a methodology to characterize the variability of gene content in gut bacterial species, using metagenomes. My approach is based on gene deletions, and was applied to abundant species (demonstrated using a set of 11 species). The method is sufficiently robust as it captures a similar range of gene content variability as has been detected in completely sequenced genomes. Using this procedure I found individuals differ by an average of 13% in their gene content of gut bacterial strains within the same species. Interestingly no two individuals shared the same gene content across bacterial species. However, this variation corresponds to a lower limit, as it is only accounts for gene deletion and not insertions. This large variation in the gene content of gut strain was found to affect important functions, such as polysaccharide utilization loci (PULs) and capsular polysaccharide synthesis (CPS), which are related with digestion of dietary fibers. In summary, I have shown that metagenomics based approaches can be robust in characterizing genetic variation in gut bacterial species. I also illustrated, using examples both for SNPs and gene content (galK, PULs and CPS), that this genetic variation can be used to predict the phenotypic characteristics of the microbial species, as well as predicting the phenotype of their human host (for example, their capacity to digest different food components). Overall, the results of my thesis highlight the importance of characterizing the strains in the gut microbiome analogous to the emerging variability and importance of human genomics. N2 - Mikrobielle Arten (Bakterien und Archaeen) im menschlichen Darm sind wichtige Begleiter für unsere Gesundheit. Jedoch gibt es nicht nur starke Unterschiede zwischen individuellen Wirten in der Artenzusammensetzung des Darmmikrobioms, sondern es scheint sogar Individuen-spezifische Bakterienstämme zu geben. Analysen von Bakterien wie z.B. Escherichia coli haben schon früh gezeigt, dass die Genome von Bakterienstämmen derselben Art große Unterschiede aufzeigen können; jedoch wurden diese Unterschiede bisher noch nicht in einer natürlichen Umgebung gezeigt. Genetische Variation kann viele Ausprägungen haben und reicht von kleinen Veränderungen wie „small nucleotide polymorphism“ (SNP) zu makroskopischen Veränderung, wie z.B. chromosomalen Restrukturierungen. All diese genetischen Variationen wurden bis jetzt nicht in der natürlichen Umgebung der Bakterien studiert, vorallem bedingt durch fehlende Methoden um die meisten dieser Bakterien um Labor zu kultivieren. Metagenomische Studien können hier helfen, da sie unabhängig von Kultivierungen jegliche DNS aus einer natürlichen Bakteriengemeinschaft untersuchen. Jedoch wurde dies in den meisten bisher veröffentlichten metagenomischen Studien nicht ausgenutzt da diese hauptsächlich auf die Anzahl der gefunden Gene ausgerichtet waren. Das Ziel meiner Doktorarbeit war es, die genetische Variation in Darmbakterien zu beschreiben und phenotypische Veränderungen zu untersuchen. Dies habe ich umgesetzt durch die Erforschung (1) der SNP-Varianz in Darmbakterien, mit besonderem Augenmerk auf Gene, die unter einem selektivem Druck stehen und (2) der Variationen in der Genzusammensetzung eines Genomes (als eine Annäherung an strukturelle Variationen) und welchen Effekt dies auf Mikrobenarten und Wirtsphenotypen hat. Im ersten Kapitel meiner Doktorarbeit beschreibe ich meine Arbeit in einem Projekt unserer Gruppe, in dem wir basierend auf metagenomischen Daten 10 Millionen SNPs in menschlichen Darmbakterien beschrieben haben. Diesen Datensatz habe ich verwendet um die erste SNP-basierte, vergleichende Studie der Bakterienevolution in einem natürlichen Habitat zu realisieren. Ich entdeckte, dass Bakterienstämme unabhängig vom Wirt ähnliche evolutionäre Raten haben. Genauer gesagt, die evolutionäre Rate für eine Art ist stabiler zwischen Wirten, als die von verschiedenen Spezies innerhalb eines Wirtes. Ausserdem fand ich heraus, dass die Evolution von einzelnen Genen unabhängig vom restlichen Genom einer Spezies ist. Dies könnte durch einen Selektionsdruck wie z.B. die Ernährung des Wirtes ausgelöst werden, was ich am Beispiel des Galactokinasegenes (galK) gezeigt habe. Obwohl wir zeigen konnten, dass das SNP-Profil der Darmbakterien spezifisch für den jeweiligen Wirt ist, konnten wir keine Assoziation zwischen SNPs und Wirtsphänotypen finden. Auch aus diesem Grund habe ich mich in meiner weiteren Arbeit verstärkt auf makroskopische Genomvariationen konzentriert. Im zweiten Teil meiner Doktoarbeit entwickelte ich eine neue Methode, um Variationen in der genomische Zusammensetzung von einzelnen Bakterienarten zu beschreiben, wieder basierend auf metagenomischen Daten. Hierbei fokussiere ich mich insbesondere auf Gene, die in unseren metagenomischen Daten im Verglich zum Referengenom fehlen und wende dies auf die 11 dominantesten Bakterienspezies an. Diese neue Methode ist robust, da die gefundene Genomvarianz in unseren metagenomischen Daten übereinstimmt mit Daten aus komplett sequenzierten Genomen. So konnte ich herausfinden, dass im Durchschnitt 13% der Gene einer Bakterienart zwischen einzelen Wirten varieren. Besonders interessant ist hier, dass wir keine zwei Wirte gefunden haben, die für eine Bakterienart genau diesselben Gene haben. Jedoch ist die erwarte Varianz aller Wahrscheinlichkeit nach noch größer, da ich mit dieser Methode nur fehlende Gene beschreiben kann, aber nicht neu hinzugekommende. Diese Varianz kann auch wichtige bakterielle Funktionen betreffen, z.B. Gene für „polysaccharide utilization loci“ (PULs) und „capsular polysaccharide synthesis“ (CPS), welche wichtig sind um Ballaststoffe in der Nahrung zu verwerten. Zusammenfassend konnte ich in dieser Arbeit zeigen, dass metagenomische Methoden robust genug sind um die genetische Varianz von Darmbakterien zu beschreiben. Ausserdem konnte ich zeigen, dass die beschriebene Varianz benutzt werden kann, um phenotypische Veränderungen von Bakterien vorherzusagen (demonstriert für die galK, PULs and CPS-Gene). Dies wiederrum könnte benutzt werden um Vorhersagen für den Wirt über z.B. seine Ernährung zu machen. Meine Doktorarbeit zeigt wie wichtig es ist, einzelne Bakterienstämme zu charakterisieren, ganz analog zu der Bedeutsamkeit der genetischen Varianz des menschlichen Genomes. KW - metagenomic KW - Darmflora KW - Metagenom Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-113890 ER - TY - THES A1 - Zhou, Qingchun T1 - Molecular analysis of the sex-determining region of the Y chromosome in the platyfish Xiphophorus maculatus T1 - Molekulare Analyse der geschlechtsbestimmenden Region des Y Chromosoms von Xiphophorus maculatus N2 - A large variety of sex determination systems have been described in fish. However, almost no information is available about sex determination in the classical fish models, the zebrafish Danio rerio and the pufferfish Takifugu rubripes. A DNA-binding protein gene called dmrt1bY (or DMY) has been recently described as an outstanding candidate for the primary sex-determining gene in the medaka fish Oryzias latipes. But this gene is not the universal master sex-determining gene in teleost fish, since dmrt1bY is not found in most other fishes. Hence, other fish models need to be examined including the platyfish Xiphophorus maculatus. Xiphophorus maculatus has three types of sex chromosomes (X, Y and W; females are XX, WX or WY; males are XY or YY). Its gonosomes are at an early stage of differentiation. The sex-determining locus on the sex chromosomes is flanked by two receptor tyrosine kinase genes, the Xmrk oncogene and its protooncogenic progenitor gene egfrb, which both delimit a region of about 0.6 centiMorgans. This situation should allow the positional cloning of the sex-determining gene (SD) of the platyfish. For this purpose, Bacterial Artificial Chromosome (BAC) contigs were assembled from a BAC library of XY males constructed in our laboratory, using the oncogene Xmrk, egfrb, as well as a Y-specific pseudogene called ps-criptY as starting points. The ps-criptY sequence was found to be closely linked to the SD gene, since no recombination was observed between SD and ps-criptY in more than 400 individuals tested. Two major BAC contigs for the X chromosome (about 2.5 Mb) and three major BAC contigs for the Y chromosome (about 3.5 Mb) were built up and analyzed by strategic sequencing. These are some of the largest contigs ever assembled for the sex chromosomes of a non-mammalian vertebrate species. The molecular analysis of the ps-criptY contig was the major objective of this work. The Y-specific ps-criptY contig has been extended over 1 Mb in this work with 58 identified molecular markers. Approximatively 700 kb of non-redundant sequences has been obtained from this contig by strategic sequencing. Numerous Y-linked markers from the contig including ps-criptY were also detected on the X chromosome. Nevertheless, major structural differences were observed between the X and Y chromosomes. Particularly, a large region, which is present at one copy on the X chromosome and contains several candidate genes, was found to be duplicated on the Y chromosome. Evidence for an inversion in the sex-determining region and for the Y-specific accumulation of a repeated sequence called XIR was also obtained. Such events might correspond to an initiation of differentiation between both types of gonosomes. Accumulation of transposable elements was also observed in the ps-criptY contig. A DNA transposable element, helitron, was isolated from the sex-determining region of X. maculatus. Three copies of helitron are located on the ps-criptY contig and one copy on the X-linked contig (helitron has roughly 15 copies per haploid genome). No in-frame stop codon, truncation or intron was found in these four copies, which present high nucleotide identities to each other. This suggests that helitron elements might be active or have been recently active in X. maculatus. A consensus open reading frame of helitron was also assembled from medaka (Oryzias latipes) genomic sequences. Two candidate genes from the ps-criptY contig are also located on the W chromosome in the X. maculatus Usumacinta strain (heterogamety). These markers show the relationship between the different types of gonosomes and allow to compare the male and female heterogameties in the platyfish. Several gene candidates were identified in the ps-criptY contig. However, some of them such as msh2, cript, igd and acr probably correspond to pseudogenes. Interestingly, a novel gene, called swimy, is exclusively expressed in spermatogonia of the adult testis. Swimy is a gene encoding a DNA-binding protein with several putative DNA-binding domains. The data suggest that swimy is a very promising candidate for the master SD gene. Another novel gene, which is called fredi and encodes a novel helix-turn-helix protein, is predominately expressed in the adult testis and currently under scrutiny. There is no doubt that the master SD gene of X. maculatus will be identified by positional cloning. Further molecular analysis of the contigs built in this work will shed new light on the molecular mechanism of sex determination and the evolution of sex chromosomes in fish. N2 - In Fischen wurde eine große Anzahl Geschlechtsbestimmungssysteme beschrieben. Allerdings gibt es kaum Informationen über die Geschlechtsbestimmung der klassischen Modellorganismen, des Zebrafisches Danio rerio und des Pufferfisches Takifugu rubripes. Das für ein DNA-bindendes Protein kodierende Gen dmrt1bY (oder DMY) wurde kürzlich als ein herausragender Kandidat für das primäre Geschlechts-bestimmungsgen im Medaka Oryzias latipes beschrieben. Dieses Gen ist jedoch nicht das universelle Geschlechtsbestimmungsgen der echten Knochenfische (Teleostei), da dmrt1bY in den meisten anderen Fischen nicht identifiziert werden konnte. Deshalb dienen andere Fische wie der Platy Xiphophorus maculatus als Modelle. Xiphophorus maculatus besitzt drei Geschlechtschromosomen X, Y und W in einem frühen Stadium der Differenzierung (Weibchen sind XX, WX oder WY, Männchen XY oder YY). Der geschlechtsbestimmende Locus wird flankiert von zwei Rezeportyrosinkinase-Genen, dem Onkogen Xmrk und seinem Vorläufer, dem Proto-onkogen egfrb. Sie markieren eine Region von ca. 0.6 centiMorgan, was die positionelle Klonierung des geschlechtsbestimmenden Gens SD des Platys erlauben sollte. Zu diesem Zweck wurden BAC- (Bacterial Artificial Chromosome-) Contigs der X- und Y-Chromosomen aus einer genomischen Bibliothek erstellt, wobei Xmrk, egfrb und das Y-spezifische Pseudogen ps-criptY als Startpunkte gewählt wurden. Ps-criptY ist eng an SD gekoppelt, wie die Analyse von über 400 Individuen zeigte. Zwei BAC-Contigs des X-Chromosoms (ca. 2.5 Mb) und drei BAC-Contigs des Y-Chromosoms (ca. 3.5 Mb) wurden erstellt und durch strategisches Sequenzieren analysiert. Dies sind einige der größten geschlechtschromosomalen Contigs, die je für eine Wirbeltierart außerhalb der Säuger erstellt wurden. Der Aufbau und die molekulare Analyse des BAC-Contigs um ps-criptY war Hauptziel dieser Arbeit. Dieses Y-spezifische Contig wurde durch die Analyse von 58 molekularen Markern in dieser Arbeit um über eine Megabase erweitert. Fast 700 kb nicht-redundanter Sequenz konnten durch strategisches Sequenzieren analysiert werden. Obwohl eine Vielzahl von Markern des Y-Chromosoms inklusive ps-criptY ebenfalls auf dem X-Chromosom detektiert wurden, konnten große strukturelle Unterschiede der Geschlechtschromosomen nachgewiesen werden. Im besonderen konnte die Duplikation einer großen Region des X-Chromosoms, die mehrere Genkandidaten enthält, auf dem Y-Chromosom gezeigt werden. Außerdem konnte die Inversion dieser Region inklusive einer Akkumulation der repetitiven Sequenz XIR konnte belegt werden. Solche Ereignisse entsprechen einer beginnenden Differenzierung zwischen heteromorphen Geschlechtschromosomen. Außerdem wurde die Akkumulation transposabler Elemente im ps-criptY-Contig beobachtet. Eines dieser Elemente, helitron, konnte aus der geschlechtsbestimmenden Region von X. maculatus isoliert werden. Von den vier Kopien der geschlechts-bestimmenden Region (3 Kopien im ps-criptY-Contig des Y-Chromosoms, 1 Kopie im Xmrk-Contig des X-Chromosoms, 15 im gesamten Genom) enthielt keine ein vorzeitiges Stop-Codon, Unterbrechung oder sonstige Störung des offenen Leserasters. Dies könnte darauf hinweisen, dass die helitron-Elemente in X. maculatus noch aktiv sind oder bis vor kurzem waren. Ein Konsensus-ORF des helitron-Elements konnte auch aus Datenbank-Sequenzen des Medaka (Oryzias latipes) erstellt werden. Zwei Genkandidaten des ps-criptY-Contigs konnten auch auf dem W-Chromosom von X. maculatus (Rio Usumacinta, weibliche Heterogametie) nachgewiesen werden. Diese Marker zeigen die enge Beziehung zwischen den Geschlechtschromosomen des Platys und ermöglichen eine detaillierte Untersuchung von männlicher und weiblicher Heterogametie im Platy. Verschiedene Genkandidaten konnten im ps-criptY-Contig identifiziert werden. Allerdings zeigte die Analyse, dass einige davon, wie msh2, cript, igd und acr Pseudogene darstellen. Interessanterweise ist eines dieser Gene, swimy, ausschließlich in Spermatogonien exprimiert. Dieses neue Gen kodiert für ein Protein mit mehreren DNA-bindenden Domänen. Diese Daten machen swimy zu einem vielversprechenden Kandidaten für SD. Ein weiteres neues Gen, fredi, kodiert für ein Helix-Loop-Helix Protein, ist ebenfalls im adulten Hoden exprimiert und wird gerade eingehender analysiert. Zweifellos wird das geschlechtsbestimmende Gen in X. maculatus durch positionelle Klonierung identifiziert werden. Weitergehende molekulare Analysen der geschlechtschromosomalen Contigs werden Licht in die molekularen Grundlagen der Geschlechtsbestimmung und die Evolution der Geschlechtschromosomen in Fischen bringen. KW - Platy KW - Geschlechtsbestimmung KW - Y-Chromosom KW - Genanalyse KW - Xiphophorus maculatus KW - Geschlechtsbestimmung KW - Y Chromosome KW - Xiphophorus maculatus KW - Sex determination KW - Y chromosome Y1 - 2005 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-13827 ER - TY - JOUR A1 - Zhang, Shaowu A1 - Si, Aung A1 - Pahl, Mario T1 - Visually guided decision making in foraging honeybees JF - Frontiers in Neuroscience N2 - Honeybees can easily be trained to perform different types of discrimination tasks under controlled laboratory conditions. This review describes a range of experiments carried out with free-flying forager honeybees under such conditions. The research done over the past 30 or so years suggests that cognitive abilities (learning and perception) in insects are more intricate and flexible than was originally imagined. It has become apparent that honeybees are capable of a variety of visually guided tasks, involving decision making under challenging situations: this includes simultaneously making use of different sensory modalities, such as vision and olfaction, and learning to use abstract concepts such as “sameness” and “difference.” Many studies have shown that decision making in foraging honeybees is highly flexible. The trained animals learn how to solve a task, and do so with a high accuracy, but when they are presented with a new variation of the task, they apply the learnt rules from the earlier setup to the new situation, and solve the new task as well. Honeybees therefore not only feature a rich behavioral repertoire to choose from, but also make decisions most apt to the current situation. The experiments in this review give an insight into the environmental cues and cognitive resources that are probably highly significant for a forager bee that must continually make decisions regarding patches of resources to be exploited. Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-124228 VL - 6 IS - 88 ER - TY - JOUR A1 - Zhan, Hong A1 - Stanciauskas, Ramunas A1 - Stigloher, Christian A1 - Dizon, Kevin K. A1 - Jospin, Maelle A1 - Bessereau, Jean-Luis A1 - Pinaud, Fabien T1 - In vivo single-molecule imaging identifies altered dynamics of calcium channels in dystrophin-mutant C. elegans JF - Nature Communications N2 - Single-molecule (SM) fluorescence microscopy allows the imaging of biomolecules in cultured cells with a precision of a few nanometres but has yet to be implemented in living adult animals. Here we used split-GFP (green fluorescent protein) fusions and complementation-activated light microscopy (CALM) for subresolution imaging of individual membrane proteins in live Caenorhabditis elegans (C. elegans). In vivo tissue-specific SM tracking of transmembrane CD4 and voltage-dependent Ca(2+) channels (VDCC) was achieved with a precision of 30 nm within neuromuscular synapses and at the surface of muscle cells in normal and dystrophin-mutant worms. Through diffusion analyses, we reveal that dystrophin is involved in modulating the confinement of VDCC within sarcolemmal membrane nanodomains in response to varying tonus of C. elegans body-wall muscles. CALM expands the applications of SM imaging techniques beyond the petri dish and opens the possibility to explore the molecular basis of homeostatic and pathological cellular processes with subresolution precision, directly in live animals. Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-121125 VL - 5 IS - 4974 ER - TY - JOUR A1 - Zentgraf, Hanswalter A1 - Trendelenburg, Michael F. A1 - Spring, Herbert A1 - Scheer, Ulrich A1 - Franke, Werner W. A1 - Müller, Ulrike A1 - Drury, Kenneth C. A1 - Rungger, Duri T1 - Mitochondrial DNA arranged into chromatin-like structures after injection into amphibian oocyte nuclei N2 - Purified mitochondrial DNA (mitDNA) from ovaries ofXenopus lae vis was injected into the nuclei (germinal vesicles) of large viteUogenic oocytes of the same organism and examined by electron microscopy ofthe spread nuclear contents. Normally located nuclei of untreated oocytes as weil as peripherally translocated nuclei of centrifuged oocytes were used. In addition, oocyte nuclei isolated and incubated under liquid paraffin oil were injected with DNA. The integrity oftranscriptional structures of endogenous chromosomal (Iampbrush chromosomes) and extrachromosomal (nucleoli) genes of the injected nuclei was demonstrated. Microinjected mitDN A was identified as circles of chromatin exhibiting polynucleosome-like organization and a me an contour length of 2.6 J.Lm, corresponding to a compaction ratio of the mitDN A of about 2 : I. This DNA packing ratio is similar to that observed after preparation of various kinds of native chromatin in low salt buffers. The chromatin circles formed from injected mitDNA only very rarely exhibited lateral fibrils suggestive of transcriptional activity. These results suggest that purified mitDNA can be transformed to normally structured chromatin when exposed to oocyte nuclear contents but is rarely , if at all , transcribed in this form and in this environment. Y1 - 1979 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-33174 ER - TY - JOUR A1 - Zentgraf, Hanswalter A1 - Scheer, Ulrich A1 - Franke, Werner W. T1 - Characterization and localization of the RNA synthesized in mature avian erythrocytes N2 - No abstract available Y1 - 1975 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-32410 ER - TY - JOUR A1 - Zentgraf, H. A1 - Müller, U. A1 - Scheer, Ulrich A1 - Franke, W. W. T1 - Evidence for the existence of globular units in the supranucleosomal organization of chromatin N2 - No abstract available Y1 - 1981 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-34123 ER - TY - THES A1 - Zeeshan, Ahmed T1 - Bioinformatics Software for Metabolic and Health Care Data Management T1 - Metabolische Flux-Analyse N2 - Computer Science approaches (software, database, management systems) are powerful tools to boost research. Here they are applied to metabolic modelling in infections as well as health care management. Starting from a comparative analysis this thesis shows own steps and examples towards improvement in metabolic modelling software and health data management. In section 2, new experimental data on metabolites and enzymes induce high interest in metabolic modelling including metabolic flux calculations. Data analysis of metabolites, calculation of metabolic fluxes, pathways and their condition-specific strengths is now possible by an advantageous combination of specific software. How can available software for metabolic modelling be improved from a computational point of view? A number of available and well established software solutions are first discussed individually. This includes information on software origin, capabilities, development and used methodology. Performance information is obtained for the compared software using provided example data sets. A feature based comparison shows limitations and advantages of the compared software for specific tasks in metabolic modeling. Often found limitations include third party software dependence, no comprehensive database management and no standard format for data input and output. Graphical visualization can be improved for complex data visualization and at the web based graphical interface. Other areas for development are platform independency, product line architecture, data standardization, open source movement and new methodologies. The comparison shows clearly space for further software application development including steps towards an optimal user friendly graphical user interface, platform independence, database management system and third party independence especially in the case of desktop applications. The found limitations are not limited to the software compared and are of course also actively tackled in some of the most recent developments. Other improvements should aim at generality and standard data input formats, improved visualization of not only the input data set but also analyzed results. We hope, with the implementation of these suggestions, metabolic software applications will become more professional, cheap, reliable and attractive for the user. Nevertheless, keeping these inherent limitations in mind, we are confident that the tools compared can be recommended for metabolic modeling for instance to model metabolic fluxes in bacteria or metabolic data analysis and studies in infection biology. ... N2 - Informatik Ansätze (Software, Datenbank, Management-Systeme) sind wichtige Werkzeuge für die Forschung in der Biologie. Ausgehend von einer vergleichenden Analyse zeigt diese Arbeit eigene Schritte und Beispiele zur Verbesserung von metabolischer Modellierungs-Software und Gesundheit Datenmanagementsystemen auf. Neue experimentelle Daten über Metaboliten und Enzyme führen zu hohem Interesse an metabolischen Modellierungen einschließlich Stoffwechselflusses Berechnungen. In Kapitel 2 zeigen wir, das die Datenanalyse von Metaboliten, die Berechnung der Stoffflüsse und Wege sowie die spezifischen Softwarestärken nur durch eine vorteilhafte Kombination voll ausgeschöpft werden. Wie kann Software zur metabolischen Modellierung von einer informatischen Sicht her verbessert werden? Eine Anzahl von verfügbaren und gut etablierten Softwareansätzen wird zunächst einzeln diskutiert. Dazu gehören Informationen über Software-Herkunft, Fähigkeiten, Entwicklung und verwendeten Methodik einschließlich Testdatensätzen und Modellen. Ein Vergleich zeigt, merkmalsbasierte Einschränkungen und Vorteile der verglichenen Software für spezifische Aufgaben in der metabolischen Modellierung. Häufige Einschränkungen der verglichenen Software sind ihre Abhängigkeit von Drittanbietern, kein umfassendes Datenbank-Management und kein Standard-Format für Dateneingabe und -ausgabe. Die grafische Visualisierung für komplexe Visualisierungen von Daten und die Web-basierte grafische Benutzeroberfläche kann oft noch verbessert werden. Andere Bereiche für weitere Entwicklung sind Plattformunabhängigkeit, Produktlinien-Architektur, Daten-Standardisierung, die Open-Source-Bewegung und neue Algorithmen und Methoden. Der Vergleich zeigt deutlich Möglichkeiten für weitere Entwicklung von Softwareanwendungen auf, einschließlich Schritten in Richtung einer optimalen, benutzerfreundlichen grafischen Benutzeroberfläche, Plattform-Unabhängigkeit, Datenbank-Management-System und Unabhängigkeit von weiterer software, vor allem im Falle von Desktop-Anwendungen. Die gefundenen Einschränkungen sind von allgemeiner Bedeutung für bioinformatische Modellierungssoftware einschließlich jüngster Entwicklungen. Weitere Verbesserungen betreffen standardisierte Formate und eine, verbesserte Visualisierung von Eingabedatensatz und analysierten Ergebnissen. Wir hoffen, dass mit der Umsetzung dieser Vorschläge metabolische Software-Anwendungen professioneller werden, billiger, zuverlässiger und attraktiver für den Anwender. Trotz dieser inhärenten Einschränkungen im Hinterkopf sind wir zuversichtlich und ... KW - Stoffwechsel KW - Modell KW - Software KW - Gesundheitswesen KW - Datenbanksystem KW - Metabolische Flux-Analyse KW - Massen-Isotopomer Verteilungs-Analyse KW - Datenbank KW - Management-Systeme KW - Metabolic Flux Analysis KW - Mass Isotopomers Distribution Analysis KW - Software KW - Database KW - Management System Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-73926 ER - TY - JOUR A1 - Zeeshan, Ahmed T1 - Towards Performance Measurement and Metrics Based Analysis of PLA Applications N2 - This article is about a measurement analysis based approach to help software practitioners in managing the additional level complexities and variabilities in software product line applications. The architecture of the proposed approach i.e. ZAC is designed and implemented to perform preprocessesed source code analysis, calculate traditional and product line metrics and visualize results in two and three dimensional diagrams. Experiments using real time data sets are performed which concluded with the results that the ZAC can be very helpful for the software practitioners in understanding the overall structure and complexity of product line applications. Moreover the obtained results prove strong positive correlation between calculated traditional and product line measures. KW - Programmierbare logische Anordnung KW - Analysis KW - Measurement KW - Software product lines KW - Variability Y1 - 2010 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-68188 ER - TY - THES A1 - Zeeshan [geb. Majeed], Saman T1 - Implementation of Bioinformatics Methods for miRNA and Metabolic Modelling T1 - Die Umsetzung der Bioinformatik-Methoden für miRNA-und der Metabolischen Modellierung N2 - Dynamic interactions and their changes are at the forefront of current research in bioinformatics and systems biology. This thesis focusses on two particular dynamic aspects of cellular adaptation: miRNA and metabolites. miRNAs have an established role in hematopoiesis and megakaryocytopoiesis, and platelet miRNAs have potential as tools for understanding basic mechanisms of platelet function. The thesis highlights the possible role of miRNAs in regulating protein translation in platelet lifespan with relevance to platelet apoptosis and identifying involved pathways and potential key regulatory molecules. Furthermore, corresponding miRNA/target mRNAs in murine platelets are identified. Moreover, key miRNAs involved in aortic aneurysm are predicted by similar techniques. The clinical relevance of miRNAs as biomarkers, targets, resulting later translational therapeutics, and tissue specific restrictors of genes expression in cardiovascular diseases is also discussed. In a second part of thesis we highlight the importance of scientific software solution development in metabolic modelling and how it can be helpful in bioinformatics tool development along with software feature analysis such as performed on metabolic flux analysis applications. We proposed the “Butterfly” approach to implement efficiently scientific software programming. Using this approach, software applications were developed for quantitative Metabolic Flux Analysis and efficient Mass Isotopomer Distribution Analysis (MIDA) in metabolic modelling as well as for data management. “LS-MIDA” allows easy and efficient MIDA analysis and, with a more powerful algorithm and database, the software “Isotopo” allows efficient analysis of metabolic flows, for instance in pathogenic bacteria (Salmonella, Listeria). All three approaches have been published (see Appendices). N2 - Dynamische Wechselwirkungen und deren Veränderungen sind wichtige Themen der aktuellen Forschung in Bioinformatik und Systembiologie. Diese Promotionsarbeit konzentriert sich auf zwei besonders dynamische Aspekte der zellulären Anpassung: miRNA und Metabolite. miRNAs spielen eine wichtige Rolle in der Hämatopoese und Megakaryozytopoese, und die Thrombozyten miRNAs helfen uns, grundlegende Mechanismen der Thrombozytenfunktion besser zu verstehen. Die Arbeit analysiert die potentielle Rolle von miRNAs bei der Proteintranslation, der Thrombozytenlebensdauer sowie der Apoptose von Thrombozyten und ermöglichte die Identifizierung von beteiligten Signalwegen und möglicher regulatorischer Schlüsselmoleküle. Darüber hinaus wurden entsprechende miRNA / Ziel-mRNAs in murinen Thrombozyten systematisch gesammelt. Zudem wurden wichtige miRNAs, die am Aortenaneurysma beteiligt sein könnten, durch ähnliche Techniken vorhergesagt. Die klinische Relevanz von miRNAs als Biomarker, und resultierende potentielle Therapeutika, etwa über eine gewebsspezifische Beeinflussung der Genexpression bei Herz-Kreislauf Erkrankungen wird ebenfalls diskutiert. In einem zweiten Teil der Dissertation wird die Bedeutung der Entwicklung wissenschaftlicher Softwarelösungen für die Stoffwechselmodellierung aufgezeigt, mit einer Software-Feature-Analyse wurden verschiedene Softwarelösungen in der Bioinformatik verglichen. Wir vorgeschlagen dann den "Butterfly"-Ansatz, um effiziente wissenschaftliche Software-Programmierung zu implementieren. Mit diesem Ansatz wurden für die quantitative Stoffflussanalyse mit Isotopomeren effiziente Software-Anwendungen und ihre Datenverwaltung entwickelt: LS-MIDA ermöglicht eine einfache und effiziente Analyse, die Software "Isotopo" ermöglicht mit einem leistungsfähigeren Algorithmus und einer Datenbank, eine noch effizientere Analyse von Stoffwechselflüssen, zum Beispiel in pathogenen Bakterien (Salmonellen, Listerien). Alle drei Ansätze wurden bereits veröffentlicht (siehe Appendix). KW - miRNS KW - Bioinformatics KW - miRNA KW - Metabolic Modelling KW - Spectral Data Analysis KW - Butterfly KW - Thrombozyt KW - Bioinformatik KW - Stoffwechsel KW - Modellierung KW - Metabolischen Modellierung Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-102900 ER - TY - THES A1 - Zachary, Marie T1 - Functional characterization of small non-coding RNAs of \(Neisseria\) \(gonorrhoeae\) T1 - Funktionelle Charakterisierung kleiner nicht-kodierender RNAs in \(Neisseria\) \(gonorrhoeae\) N2 - During infection, bacteria need to adapt to a changing environment and have to endure various stress conditions. Small non-coding RNAs are considered as important regulators of bacterial gene expression and so allow quick adaptations by altering expression of specific target genes. Regulation of gene expression in the human-restricted pathogen Neisseria gonorrhoeae, the causative agent of the sexually transmitted disease gonorrhoea, is only poorly understood. The present study aims a better understanding of gene regulation in N. gonorrhoeae by studying small non-coding RNAs. The discovery of antisense RNAs for all opa genes led to the hypothesis of asRNA-mediated degradation of out-of-frame opa transcripts. Analysis of asRNA expression revealed a very low abundance of the transcripts and inclusion of another phase-variable gene in the study indicates that the asRNAs are not involved in degradation of out-of-frame transcripts. This doctoral thesis focuses on the analysis of trans-acting sRNAs. The sibling sRNAs NgncR_162 and NgncR_163 were discovered as post-transcriptional regulators altering expression of genes involved in metabolic processes, amino acid uptake and transcriptional regulation. A more detailed analysis by in silico and transcriptomic approaches showed that the sRNAs regulate a broad variety of genes coding for proteins of central metabolism, amino acid biosynthesis and degradation and several transport processes. Expression levels of the sibling sRNAs depend on the growth phase of the bacteria and on the growth medium. This indicates that NgncR_162 and NgncR_163 are involved in the adaptation of the gonococcal metabolism to specific growth conditions. This work further initiates characterisation of the sRNA NgncR_237. An in silico analysis showed details on sequence conservation and a possible secondary structure. A combination of in silico target prediction and differential RNA sequencing resulted in the identification of several target genes involved in type IV pilus biogenesis and DNA recombination. However, it was not successful to find induction conditions for sRNA expression. Interestingly, a possible sibling sRNA could be identified that shares the target interaction sequence with NgncR_237 and could therefore target the same mRNAs. In conclusion, this thesis provides further insights in gene regulation by non-coding RNAs in N. gonorrhoeae by analysing two pairs of sibling sRNAs modulating bacterial metabolism or possibly type IV pilus biogenesis. N2 - Bakterien müssen sich während des Infektionsprozesses an eine sich veränderte Umgebung anpassen und sind dabei zahlreichen Stressfaktoren ausgesetzt. Kleine, nicht-kodierende RNAs gelten als wichtige Regulatoren der bakteriellen Genexpression und ermöglichen daher eine schnelle Anpassung durch eine Veränderung der Expression spezifischer Ziel-Gene. Die Regulation der Genexpression des Humanpathogens Neisseria gonorrhoeae, Auslöser der Geschlechtskrankheit Gonorrhö, ist bis jetzt kaum verstanden. Die vorliegende Studie soll durch die Analyse kleiner, nicht-kodierender RNAs zum besseren Verständnis der Genregulation in Gonokokken beitragen. Durch die Entdeckung von antisense-RNAs für alle opa Gene wurde die Hypothese entwickelt, dass diese für den Abbau von opa Transkripten außerhalb des Leserahmens verantwortlich sind. Eine Analyse der asRNA Expression zeigte jedoch, dass diese sehr wenig exprimiert werden und auch die Untersuchung eines anderen phasenvariablen Gens weist darauf hin, dass die asRNAs keine Bedeutung für den Abbau von Transkripten außerhalb des Leserahmens haben. Der Schwerpunkt der Doktorarbeit liegt auf der Untersuchung trans-codierter sRNAs. Die Zwillings-sRNAs NgncR_162 und NgncR_163 agieren als post-transkriptionelle Regulatoren, die die Expression von Genen verändern, die bei Stoffwechselprozessen, Aminosäureaufnahme und transkriptioneller Regulation eine Rolle spielen. Eine detailliertere Analyse durch in silico- und Transkriptom-Studien zeigte, dass die sRNAs ein großes Spektrum an Genen regulieren, die für Proteine des Zentralstoffwechsels, der Aminosäurebiosynthese und des –abbaus, sowie zahlreicher Transportprozesse kodieren. Die Expressionslevel der Zwillings-sRNAs hängen von der Wachstumsphase der Bakterien und dem Wachstumsmedium ab. Das weist darauf hin, dass NgncR_162 und NgncR_163 eine Rolle bei der Adaptation des Stoffwechsels von Gonokokken zu bestimmten Wachstumsbedingungen spielen. In dieser Arbeit wird zudem die Charakterisierung der sRNA NgncR_237 initiiert. Im Rahmen von in silico Analysen wurde die Sequenzkonservierung und mögliche Sekundärstruktur untersucht. Eine Kombination aus in silico Zielgen-Vorhersage und differentieller RNA Sequenzierung führte zur Identifizierung zahlreicher Zielgene, die in der Biogenese von Typ IV Pili und DNA Rekombination eine Rolle spielen. Allerdings konnten keine Induktionsbedingungen für die sRNA Expression gefunden werden. Interessanterweise konnte eine mögliche Zwillings-sRNA identifiziert werden, die dieselbe Targetinteraktionsdomäne wie NgncR_237 hat und somit dieselben Zielgene regulieren könnte. Zusammenfassend ermöglicht diese Arbeit neue Einblicke in die Genregulation durch nicht-kodierende RNAs in Gonokokken, indem zwei Paare Zwillings-sRNAs analysiert wurden, die den bakteriellen Stoffwechsel anpassen oder möglicherweise eine Rolle in der Typ IV Pilus Biogenese spielen. KW - Neisseria gonorrhoeae KW - Non-coding RNA KW - Genregulation KW - regulation of gene expression Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-245826 ER - TY - JOUR A1 - Yu, Yidong A1 - Wolf, Ann-Katrin A1 - Thusek, Sina A1 - Heinekamp, Thorsten A1 - Bromley, Michael A1 - Krappmann, Sven A1 - Terpitz, Ulrich A1 - Voigt, Kerstin A1 - Brakhage, Axel A. A1 - Beilhack, Andreas T1 - Direct Visualization of Fungal Burden in Filamentous Fungus-Infected Silkworms JF - Journal of Fungi N2 - Invasive fungal infections (IFIs) are difficult to diagnose and to treat and, despite several available antifungal drugs, cause high mortality rates. In the past decades, the incidence of IFIs has continuously increased. More recently, SARS-CoV-2-associated lethal IFIs have been reported worldwide in critically ill patients. Combating IFIs requires a more profound understanding of fungal pathogenicity to facilitate the development of novel antifungal strategies. Animal models are indispensable for studying fungal infections and to develop new antifungals. However, using mammalian animal models faces various hurdles including ethical issues and high costs, which makes large-scale infection experiments extremely challenging. To overcome these limitations, we optimized an invertebrate model and introduced a simple calcofluor white (CW) staining protocol to macroscopically and microscopically monitor disease progression in silkworms (Bombyx mori) infected with the human pathogenic filamentous fungi Aspergillus fumigatus and Lichtheimia corymbifera. This advanced silkworm A. fumigatus infection model could validate knockout mutants with either attenuated, strongly attenuated or unchanged virulence. Finally, CW staining allowed us to efficiently visualize antifungal treatment outcomes in infected silkworms. Conclusively, we here present a powerful animal model combined with a straightforward staining protocol to expedite large-scale in vivo research of fungal pathogenicity and to investigate novel antifungal candidates. KW - fungal infection model KW - calcofluor white staining KW - Aspergillus KW - Lichtheimia KW - silkworm Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-228855 SN - 2309-608X VL - 7 IS - 2 ER - TY - JOUR A1 - Yilmaz, Ayse A1 - Aksoy, Volkan A1 - Camlitepe, Yilmaz A1 - Giurfa, Martin T1 - Eye structure, activity rhythms, and visually-driven behavior are tuned to visual niche in ants JF - Frontiers in Behavioral Neuroscience N2 - Insects have evolved physiological adaptations and behavioral strategies that allow them to cope with a broad spectrum of environmental challenges and contribute to their evolutionary success. Visual performance plays a key role in this success. Correlates between life style and eye organization have been reported in various insect species. Yet, if and how visual ecology translates effectively into different visual discrimination and learning capabilities has been less explored. Here we report results from optical and behavioral analyses performed in two sympatric ant species, Formica cunicularia and Camponotus aethiops. We show that the former are diurnal while the latter are cathemeral. Accordingly, F. cunicularia workers present compound eyes with higher resolution, while C. aethiops workers exhibit eyes with lower resolution but higher sensitivity. The discrimination and learning of visual stimuli differs significantly between these species in controlled dual-choice experiments: discrimination learning of small-field visual stimuli is achieved by F. cunicularia but not by C. aethiops, while both species master the discrimination of large-field visual stimuli. Our work thus provides a paradigmatic example about how timing of foraging activities and visual environment match the organization of compound eyes and visually-driven behavior. This correspondence underlines the relevance of an ecological/evolutionary framework for analyses in behavioral neuroscience. KW - visual learning KW - ant KW - activity rhythm KW - camponotus aethiops KW - formica cunicularia KW - compound eye Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-119595 VL - 8 ER - TY - JOUR A1 - Ye, Mingyu A1 - Wilhelm, Martina A1 - Gentschev, Ivaylo A1 - Szalay, Aladár T1 - A modified limiting dilution method for monoclonal stable cell line selection using a real-time fluorescence imaging system: A practical workflow and advanced applications JF - Methods and Protocols N2 - Stable cell lines are widely used in laboratory research and pharmaceutical industry. They are mainly applied in recombinant protein and antibody productions, gene function studies, drug screens, toxicity assessments, and for cancer therapy investigation. There are two types of cell lines, polyclonal and monoclonal origin, that differ regarding their homogeneity and heterogeneity. Generating a high-quality stable cell line, which can grow continuously and carry a stable genetic modification without alteration is very important for most studies, because polyclonal cell lines of multicellular origin can be highly variable and unstable and lead to inconclusive experimental results. The most commonly used technologies of single cell originate monoclonal stable cell isolation in laboratory are fluorescence-activated cell sorting (FACS) sorting and limiting dilution cloning. Here, we describe a modified limiting dilution method of monoclonal stable cell line selection using the real-time fluorescence imaging system IncuCyte\(^®\)S3. KW - monoclonal stable cell KW - limiting dilution cloning KW - ncuCyte\(^®\)S3 Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-228896 VL - 4 IS - 1 ER - TY - JOUR A1 - Ye, Mingyu A1 - Keicher, Markus A1 - Gentschev, Ivaylo A1 - Szalay, Aladar A. T1 - Efficient selection of recombinant fluorescent vaccinia virus strains and rapid virus titer determination by using a multi-well plate imaging system JF - Biomedicines N2 - Engineered vaccinia virus (VACV) strains are used extensively as vectors for the development of novel cancer vaccines and cancer therapeutics. In this study, we describe for the first time a high-throughput approach for both fluorescent rVACV generation and rapid viral titer measurement with the multi-well plate imaging system, IncuCyte\(^®\)S3. The isolation of a single, well-defined plaque is critical for the generation of novel recombinant vaccinia virus (rVACV) strains. Unfortunately, current methods of rVACV engineering via plaque isolation are time-consuming and laborious. Here, we present a modified fluorescent viral plaque screening and selection strategy that allows one to generally obtain novel fluorescent rVACV strains in six days, with a minimum of just four days. The standard plaque assay requires chemicals for fixing and staining cells. Manual plaque counting based on visual inspection of the cell culture plates is time-consuming. Here, we developed a fluorescence-based plaque assay for quantifying the vaccinia virus that does not require a cell staining step. This approach is less toxic to researchers and is reproducible; it is thus an improvement over the traditional assay. Lastly, plaque counting by virtue of a fluorescence-based image is very convenient, as it can be performed directly on the computer. KW - fluorescent recombinant vaccinia virus KW - plaque isolation KW - IncuCyte\(^®\)S3 KW - plaque assay Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-245104 SN - 2227-9059 VL - 9 IS - 8 ER - TY - THES A1 - Yarali, Ayse T1 - Aspects of predictive learning in the fruit fly T1 - Aspekte des assoziatives Lernens bei Taufliegen N2 - Past experience contributes to behavioural organization mainly via learning: Animals learn otherwise ordinary cues as predictors for biologically significant events. This thesis studies such predictive, associative learning, using the fruit fly Drosophila melanogaster. I ask two main questions, which complement each other: One deals with the processing of those cues that are to be learned as predictors for an important event; the other one deals with the processing of the important event itself, which is to be predicted. Do fruit flies learn about combinations of olfactory and visual cues? I probe larval as well as adult fruit flies for the learning about combinations of olfactory and visual cues, using a so called ‘biconditional discrimination’ task: During training, one odour is paired with reinforcement only in light, but not in darkness; the other odour in turn is reinforced only in darkness, but not in light. Thus, neither the odours nor the visual conditions alone predict reinforcement, only combinations of both do. I find no evidence that either larval or adult fruit flies were to solve such task, speaking against a cross-talk between olfactory and visual modalities. Previous studies however suggest such cross-talk. To reconcile these results, I suggest classifying different kinds of interaction between sensory modalities, according to their site along the sensory-motor continuum: I consider an interaction ‘truly’ cross-modal, if it is between the specific features of the stimuli. I consider an interaction ’amodal’ if it instead engages the behavioural tendencies or ‘values’ elicited by each stimulus. Such reasoning brings me to conclude that different behavioural tasks require different kinds of interaction between sensory modalities; whether a given kind of interaction will be found depends on the neuronal infrastructure, which is a function of the species and the developmental stage. Predictive learning of pain-relief in fruit flies Fruit flies build two opposing kinds of memory, based on an experience with electric shock: Those odours that precede shock during training are learned as predictors for punishment and are subsequently avoided; those odours that follow shock during training on the other hand are learned as signals for relief and are subsequently approached. I focus on such relief learning. I start with a detailed parametric analysis of relief learning, testing for reproducibility as well as effects of gender, repetition of training, odour identity, odour concentration and shock intensity. I also characterize how relief memories, once formed, decay. In addition, concerning the psychological mechanisms of relief learning, first, I show that relief learning establishes genuinely associative conditioned approach behaviour and second, I report that it is most likely not mediated by context associations. These results enable the following neurobiological analysis of relief learning; further, they will form in the future the basis for a mathematical model; finally, they will guide the researchers aiming at uncovering relief learning in other experimental systems. Next, I embark upon neurogenetic analysis of relief learning. First, I report that fruit flies mutant for the so called white gene build overall more ‘negative’ memories about an experience with electric shock. That is, in the white mutants, learning about the painful onset of shock is enhanced, whereas learning about the relieving offset of shock is diminished. As they are coherently affected, these two kinds of learning should be in a balance. The molecular mechanism of the effect of white on this balance remains unresolved. Finally, as a first step towards a neuronal circuit analysis of relief learning, I compare it to reward learning and punishment learning. I find that relief learning is distinct from both in terms of the requirement for biogenic amine signaling: Reward and punishment are respectively signalled by octopamine and dopamine, for relief learning, either of these seem dispensible. Further, I find no evidence for roles for two other biogenic amines, tyramine and serotonin in relief learning. Based on these findings I give directions for further research. N2 - Vergangene Ereignisse beeinflussen die Organisation des Verhaltens hauptsächlich durch das Lernen: Tiere lernen natürlich vorkommende neutrale Reize als Signal für biologisch relevante Ereignisse zu nutzen. Diese Dissertation befasst sich mit derartigen assoziativen Lernvorgängen bei der Taufliege Drosophila melanogaster. Ich stelle zwei, sich ergänzende, grundlegende Fragen: Die eine Frage beschäftigt sich mit der Verarbeitung von Reizen, die als Signal für ein wichtiges Ereignis erlernt werden. Die andere Frage behandelt die Verarbeitung des Ereignisses selbst. Lernen Taufliegen etwas über Kombinationen von olfaktorischen und visuellen Reizen? Sowohl bei larvalen, als auch bei adulten Taufliegen wird das Lernen von Kombinationen aus olfaktorischen und visuellen Stimuli untersucht. Ich verwende einen sogenannten „bikonditionalen Diskriminierungs-Versuchsaufbau“: Während des Trainings wird ein Duft nur im Licht und nicht im Dunkeln mit Reinforcement kombiniert, während ein anderer Duft nur im Dunkeln und nicht im Licht mit Reinforcement kombiniert wird. Somit signalisieren weder die Düfte, noch die visuellen Bedingungen allein das Reinforcement, sondern nur eine Kombination aus Beiden. Ich finde keine Beweise dafür, dass larvale oder adulte Taufliegen eine solche Aufgabe lösen können. Dies spricht gegen eine Interaktion zwischen olfaktorischen und visuellen Modalitäten. Allerdings weisen frühere Studien auf derartige Interaktionen hin. Um meine Ergebnisse mit den bekannten Studien in Einklang zu bringen, ordne ich die unterschiedlichen Interaktionen zwischen den sensorischen Modalitäten nach ihrer Lage entlang des sensorisch-motorischen Kontinuums: Ich bezeichnen eine Interaktion für „echt“ cross-modal, wenn sie zwischen den spezifischen Eigenschaften der beiden Reize stattfindet. Ich halte eine Interaktion für „amodal“, wenn sie zwischen den von den Reizen induzierten Verhaltenstendenzen und „Werten“ stattfindet. Aufgrund dieser Argumentation komme ich zu der Schlussfolgerung, dass unterschiedliche Verhaltensaufgaben unterschiedliche Interaktionen zwischen den sensorischen Modalitäten erfordern. Ob eine Art von Interaktion gefunden wird oder nicht hängt von der neuronalen Vernetzung ab, welche charakteristisch für Art und Entwicklungsstadium ist. Assoziatives Lernen von Schmerz-Erleichterung bei Taufliegen Taufliegen entwickeln zwei unterschiedliche Arten von Gedächtnissen basierend auf Erfahrung mit Elektro-Schock: Düfte, die während des Trainings dem Schock vorausgehen, werden als Bestrafungssignale gelernt und deshalb vermieden. Düfte, die während des Trainings auf den Schock folgen, werden als Erleichterungssignale gelernt und deshalb bevorzugt. Ich beschäftige mich mit der zweiten Art dieses assoziativen Lernens, das ich als „Erleichterungslernen“ bezeichne. Ich beginne mit einer detaillierten parametrischen Analyse des Erleichterungslernens. Die Reproduzierbarkeit, sowie die Einflüsse des Geschlechts, der Anzahl an Trainingswiederholungen, der Duftintensität, der Duftkonzentration und der Schockintensität werden geprüft. Ich teste, wie das Erleichterungsgedächtnis, nachdem es gebildet wurde, wieder gelöscht wird. Des Weiteren gehe ich zwei wichtigen Fragen zu den psychologischen Mechanismen des Erleichterungslernen nach: Zum einen zeige ich, dass das Erleichterungslernen echtes assoziativ konditioniertes Annäherungsverhalten etabliert. Zum anderen zeige ich, dass vorausgegangenes Kontext-Schock Training das folgende Erleichterungslernen nicht beeinflusst. Das Erleichterungslernen wird also nicht durch Kontextassoziation vermittelt. Diese Ergebnisse erlauben die folgende neurobiologische Analyse des Erleichterungslernens. Außerdem werden sie in Zukunft als Grundlage für ein mathematisches Modell des Erleichterungslernens dienen. Schließlich werden die Forscher/innen, die das Erleichterungslernen in anderen experimentellen Systemen untersuchen, von diesen parametrischen Erkenntnissen profitieren. In einer neurobiologischen Analyse des Erleichterungslernens zeige ich, dass der Verlust der Funktion des sogenannten white Gens die beiden unterschiedlichen Arten von Schock-Induziertem Lernen zusammenhängend beeinflusst: Das Bestrafungslernen wird verstärkt und das Erleichterungslernen wird abgeschwächt. Auf Grund dieses Ergebnisses schlagen ich vor, dass sich diese zwei Arten von Lernen in einem Gleichgewicht befinden sollen, welches vom white Gen beeinflusst wird. Die zugrunde liegenden molekularen Mechanismen eines solchen Gleichgewichts sind noch nicht bekannt. Schließlich vergleiche ich das Erleichterungslernen mit dem Belohnungslernen und dem Bestrafungslernen. Ich zeige, dass das Erleichterungslernen anders ist als beide: Bestrafung und Belohnung werden entsprechend von Dopamin und Octopamin vermittelt. Für das Erleichterungslernen sind beide diese biogenen Aminen unnötig. Ebenso finde ich beim Erleichterungslernen keinen Beleg für die Rolle von zwei weiteren Aminen: Tyramin und Serotonin. Aufgrund dieser Ergebnisse schlage ich vor weitere Forschungsrichtungen. KW - Lernen KW - Drosophila KW - Neurogenetik KW - Lernverhalten KW - olfaktorik KW - sehen KW - erleichterungslernen KW - associative learning KW - drosophila KW - neurogenetic analyses KW - behavioural analyses KW - relief Y1 - 2008 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-28741 ER - TY - JOUR A1 - Yanku, Yifat A1 - Bitman-Lotan, Eliya A1 - Zohar, Yaniv A1 - Kurant, Estee A1 - Zilke, Norman A1 - Eilers, Martin A1 - Orian, Amir T1 - Drosophila HUWE1 ubiquitin ligase regulates endoreplication and antagonizes JNK signaling during salivary gland development JF - Cells N2 - The HECT-type ubiquitin ligase HECT, UBA and WWE Domain Containing 1, (HUWE1) regulates key cancer-related pathways, including the Myc oncogene. It affects cell proliferation, stress and immune signaling, mitochondria homeostasis, and cell death. HUWE1 is evolutionarily conserved from Caenorhabditis elegance to Drosophila melanogaster and Humans. Here, we report that the Drosophila ortholog, dHUWE1 (CG8184), is an essential gene whose loss results in embryonic lethality and whose tissue-specific disruption establishes its regulatory role in larval salivary gland development. dHUWE1 is essential for endoreplication of salivary gland cells and its knockdown results in the inability of these cells to replicate DNA. Remarkably, dHUWE1 is a survival factor that prevents premature activation of JNK signaling, thus preventing the disintegration of the salivary gland, which occurs physiologically during pupal stages. This function of dHUWE1 is general, as its inhibitory effect is observed also during eye development and at the organismal level. Epistatic studies revealed that the loss of dHUWE1 is compensated by dMyc proeitn expression or the loss of dmP53. dHUWE1 is therefore a conserved survival factor that regulates organ formation during Drosophila development. KW - HECT KW - HUWE1 KW - ubiquitin KW - salivary gland KW - endoreplication KW - JNK KW - dMyc KW - dmP53 Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-197630 SN - 2073-4409 VL - 7 IS - 10 ER - TY - JOUR A1 - Yang, Tao A1 - Heydarian, Motaharehsadat A1 - Kozjak-Pavlovic, Vera A1 - Urban, Manuela A1 - Harbottle, Richard P. A1 - Rudel, Thomas T1 - Folliculin Controls the Intracellular Survival and Trans-Epithelial Passage of Neisseria gonorrhoeae JF - Frontiers in Cellular and Infection Microbiology N2 - Neisseria gonorrhoeae, a Gram-negative obligate human pathogenic bacterium, infects human epithelial cells and causes sexually transmitted diseases. Emerging multi-antibiotic resistant gonococci and increasing numbers of infections complicate the treatment of infected patients. Here, we used an shRNA library screen and next-generation sequencing to identify factors involved in epithelial cell infection. Folliculin (FLCN), a 64 kDa protein with a tumor repressor function was identified as a novel host factor important for N. gonorrhoeae survival after uptake. We further determined that FLCN did not affect N. gonorrhoeae adherence and invasion but was essential for its survival in the cells by modulating autophagy. In addition, FLCN was also required to maintain cell to cell contacts in the epithelial layer. In an infection model with polarized cells, FLCN inhibited the polarized localization of E-cadherin and the transcytosis of gonococci across polarized epithelial cells. In conclusion, we demonstrate here the connection between FLCN and bacterial infection and in particular the role of FLCN in the intracellular survival and transcytosis of gonococci across polarized epithelial cell layers. KW - gonococcal invasion KW - folliculin KW - autophagy KW - polarized epithelium KW - polarized cell culture Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-211372 SN - 2235-2988 VL - 10 IS - 422 ER - TY - JOUR A1 - Yang, Manli A1 - Rajeeve, Karthika A1 - Rudel, Thomas A1 - Dandekar, Thomas T1 - Comprehensive Flux Modeling of Chlamydia trachomatis Proteome and qRT-PCR Data Indicate Biphasic Metabolic Differences Between Elementary Bodies and Reticulate Bodies During Infection JF - Frontiers in Microbiology N2 - Metabolic adaptation to the host cell is important for obligate intracellular pathogens such as Chlamydia trachomatis (Ct). Here we infer the flux differences for Ct from proteome and qRT-PCR data by comprehensive pathway modeling. We compare the comparatively inert infectious elementary body (EB) and the active replicative reticulate body (RB) systematically using a genome-scale metabolic model with 321 metabolites and 277 reactions. This did yield 84 extreme pathways based on a published proteomics dataset at three different time points of infection. Validation of predictions was done by quantitative RT-PCR of enzyme mRNA expression at three time points. Ct’s major active pathways are glycolysis, gluconeogenesis, glycerol-phospholipid (GPL) biosynthesis (support from host acetyl-CoA) and pentose phosphate pathway (PPP), while its incomplete TCA and fatty acid biosynthesis are less active. The modeled metabolic pathways are much more active in RB than in EB. Our in silico model suggests that EB and RB utilize folate to generate NAD(P)H using independent pathways. The only low metabolic flux inferred for EB involves mainly carbohydrate metabolism. RB utilizes energy -rich compounds to generate ATP in nucleic acid metabolism. Validation data for the modeling include proteomics experiments (model basis) as well as qRT-PCR confirmation of selected metabolic enzyme mRNA expression differences. The metabolic modeling is made fully available here. Its detailed insights and models on Ct metabolic adaptations during infection are a useful modeling basis for future studies. KW - metabolic modeling KW - metabolic flux KW - infection biology KW - elementary body KW - reticulate body KW - Chlamydia trachomatis Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-189434 SN - 1664-302X VL - 10 IS - 2350 ER - TY - JOUR A1 - Yan, Yan A1 - Hong, Ni A1 - Chen, Tiansheng A1 - Li, Mingyou A1 - Wang, Tiansu A1 - Guan, Guijun A1 - Qiao, Yongkang A1 - Chen, Songlin A1 - Schartl, Manfred A1 - Li, Chang-Ming A1 - Hong, Yunhan T1 - p53 Gene Targeting by Homologous Recombination in Fish ES Cells JF - PLoS One N2 - Background: Gene targeting (GT) provides a powerful tool for the generation of precise genetic alterations in embryonic stem (ES) cells to elucidate gene function and create animal models for human diseases. This technology has, however, been limited to mouse and rat. We have previously established ES cell lines and procedures for gene transfer and selection for homologous recombination (HR) events in the fish medaka (Oryzias latipes). Methodology and Principal Findings: Here we report HR-mediated GT in this organism. We designed a GT vector to disrupt the tumor suppressor gene p53 (also known as tp53). We show that all the three medaka ES cell lines, MES1 similar to MES3, are highly proficient for HR, as they produced detectable HR without drug selection. Furthermore, the positive-negative selection (PNS) procedure enhanced HR by similar to 12 folds. Out of 39 PNS-resistant colonies analyzed, 19 (48.7%) were positive for GT by PCR genotyping. When 11 of the PCR-positive colonies were further analyzed, 6 (54.5%) were found to be bona fide homologous recombinants by Southern blot analysis, sequencing and fluorescent in situ hybridization. This produces a high efficiency of up to 26.6% for p53 GT under PNS conditions. We show that p53 disruption and long-term propagation under drug selection conditions do not compromise the pluripotency, as p53-targeted ES cells retained stable growth, undifferentiated phenotype, pluripotency gene expression profile and differentiation potential in vitro and in vivo. Conclusions: Our results demonstrate that medaka ES cells are proficient for HR-mediated GT, offering a first model organism of lower vertebrates towards the development of full ES cell-based GT technology. KW - mouse KW - in-vitro KW - drug selection KW - chimera formation KW - medakafish oryzias latipes KW - embryonic stem-cells KW - zebrafish KW - differentiation KW - cultures KW - pluripotency Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-133416 VL - 8 IS - 3 ER - TY - JOUR A1 - Yadav, Preeti A1 - Selvaraj, Bhuvaneish T. A1 - Bender, Florian L. P. A1 - Behringer, Marcus A1 - Moradi, Mehri A1 - Sivadasan, Rajeeve A1 - Dombert, Benjamin A1 - Blum, Robert A1 - Asan, Esther A1 - Sauer, Markus A1 - Julien, Jean-Pierre A1 - Sendtner, Michael T1 - Neurofilament depletion improves microtubule dynamics via modulation of Stat3/stathmin signaling JF - Acta Neuropathologica N2 - In neurons, microtubules form a dense array within axons, and the stability and function of this microtubule network is modulated by neurofilaments. Accumulation of neurofilaments has been observed in several forms of neurodegenerative diseases, but the mechanisms how elevated neurofilament levels destabilize axons are unknown so far. Here, we show that increased neurofilament expression in motor nerves of pmn mutant mice, a model of motoneuron disease, causes disturbed microtubule dynamics. The disease is caused by a point mutation in the tubulin-specific chaperone E (Tbce) gene, leading to an exchange of the most C-terminal amino acid tryptophan to glycine. As a consequence, the TBCE protein becomes instable which then results in destabilization of axonal microtubules and defects in axonal transport, in particular in motoneurons. Depletion of neurofilament increases the number and regrowth of microtubules in pmn mutant motoneurons and restores axon elongation. This effect is mediated by interaction of neurofilament with the stathmin complex. Accumulating neurofilaments associate with stathmin in axons of pmn mutant motoneurons. Depletion of neurofilament by Nefl knockout increases Stat3-stathmin interaction and stabilizes the microtubules in pmn mutant motoneurons. Consequently, counteracting enhanced neurofilament expression improves axonal maintenance and prolongs survival of pmn mutant mice. We propose that this mechanism could also be relevant for other neurodegenerative diseases in which neurofilament accumulation and loss of microtubules are prominent features. KW - Amyotrophic-lateral-sclerosis KW - Transgenic mice KW - Mouse model KW - Alzheimers disease KW - Neurofilament KW - Progressive motor neuronopathy KW - Axonal transport KW - Intermediate filaments KW - Motoneuron disease KW - Lacking neurofilaments KW - Missense mutation KW - Axon degeneration KW - Microtubules KW - Stathmin KW - Stat3 Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-188234 VL - 132 IS - 1 ER - TY - JOUR A1 - Xu, Li A1 - He, Jianzheng A1 - Kaiser, Andrea A1 - Gräber, Nikolas A1 - Schläger, Laura A1 - Ritze, Yvonne A1 - Scholz, Henrike T1 - A Single Pair of Serotonergic Neurons Counteracts Serotonergic Inhibition of Ethanol Attraction in Drosophila JF - PLoS ONE N2 - Attraction to ethanol is common in both flies and humans, but the neuromodulatory mechanisms underlying this innate attraction are not well understood. Here, we dissect the function of the key regulator of serotonin signaling—the serotonin transporter–in innate olfactory attraction to ethanol in Drosophila melanogaster. We generated a mutated version of the serotonin transporter that prolongs serotonin signaling in the synaptic cleft and is targeted via the Gal4 system to different sets of serotonergic neurons. We identified four serotonergic neurons that inhibit the olfactory attraction to ethanol and two additional neurons that counteract this inhibition by strengthening olfactory information. Our results reveal that compensation can occur on the circuit level and that serotonin has a bidirectional function in modulating the innate attraction to ethanol. Given the evolutionarily conserved nature of the serotonin transporter and serotonin, the bidirectional serotonergic mechanisms delineate a basic principle for how random behavior is switched into targeted approach behavior. KW - attraction KW - ethanol KW - Drosophila melanogaster KW - serotonin transporter Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-166762 VL - 11 IS - 12 ER - TY - THES A1 - Xu, Jiajia T1 - A high-complexity lentiviral shRNA screen identifies synthetic lethal interactions with deregulated N-Myc in neuroblastoma cells T1 - Ein hoch-Komplexität Genom-weit RNAi Screen für synthetisch letale Interaktion mit dereguliertem N-Myc in Neuroblastomzellen N2 - In contrast to c-Myc, a deregulated expression of the MYCN gene is restricted to human neuroendocrine tumours. In most cases, the excessive activity of N-Myc results from a MYCN amplification. In neuroblastoma, amplification of MYCN is a predictor of poor prognosis and resistance to therapy. The inability to target the N-Myc protein directly necessitates the search for alternative targets. This project aimed at identifying genes specifically required for growth and survival of cells that express high levels of N-Myc using high-throughput shRNA screening combined with next generation sequencing. The identification and analysis of these genes will shed light on functional interaction partners of N-Myc. We screened a shRNA library containing 18,327 shRNAs and identified 148 shRNAs, which were selectively depleted in the presence of active N-Myc. In addition, shRNAs targeting genes that are involved in p53 and ARF turnover and apoptosis were depleted in the cell population during the screen. These processes are known to affect N-Myc-mediated apoptosis. Consequently, these results biologically validated the screen. The 148 shRNAs that showed a significant synthetic lethal interaction with high levels of N-Myc expression were further analysed using the bioinformatics program DAVID. We found an enrichment of shRNAs that target genes involved in specific biological processes. For example, we validated synthetic lethal interactions for genes such as, THOC1, NUP153 and LARP7, which play an important role in the process of RNA polymerase II-mediated transcription elongation. We also validated genes that are involved in the neddylation pathway. In the screen we identified Cullin 3, which is a component of the BTB-CUL3-Rbx1 ubiquitin ligase that is involved in the turnover of Cyclin E. Depletion of cullin 3 and activation of N-Myc was found to synergistically increase Cyclin E expression to supraphysiological levels, inducing S-phase arrest and a strong DNA damage response. Together with results from a proteomics analysis of N-Myc associated proteins, our results lead us to the following hypothesis: In a neuroblastoma cell, the high levels of N-Myc result in a conflict between RNA polymerase II and the replication machinery during S-phase. The newly identified interaction partners of N- Myc are required to solve this conflict. Consequently, loss of the interaction leads to a massive DNA damage and the induction of apoptosis. In addition, inhibition or depletion of the essential components of the neddylation pathway also results in an unresolvable problem during S-phase. N2 - 6.2 Zusammenfassung Im Gegensatz zu c-Myc findet man eine Deregulation von N-Myc nur in einer begrenzten Anzahl maligner Tumore die neuroektodermalen Ursprungs sind. Die übermäßige Aktivität ist dabei fast immer durch eine genomische Amplifikation von N-Myc begründet. Im Neuroblastom korreliert eine MYCN-Amplifikation mit einer schlechten Prognose. Da es auf Grund einer fehlenden katalytischen Domäne nicht möglich ist N-Myc direkt zu inhibieren, ist die Suche nach alternativen Targets notwendig. Das Ziel dieser Arbeit war es neue Gene zu identifizieren, die notwendig für das Wachstum und Überleben von MYCN amplifizierten Zellen sind. Dies wurde durch eine Kombination von Hochdurchsatz-RNAi-Screens und Next-Generation-Sequenzierung erreicht. Durch das Screenen einer shRNA-Bibliothek, die insgesamt 18327 shRNAs beinhaltet, konnten 148 shRNAs identifiziert werden, die selektiv nachteilig für das Überleben N-Myc überexpremierender Zellen sind. Die statistische Auswertung der Ergebnisse des Screens zeigte zusätzlich eine Anreichung von shRNAs gegen Gene, die p53-und ARF-abhängig Apoptose vermitteln. Da es bekannt ist, dass diese Gene in der N-Myc-vermittelten Apoptose involviert sind, konnte dadurch der Screen validiert werden. Die weitere Auswertung mit dem bioinformatischen Programm DAVID ergab, dass unter den 148 als synthetisch letal identifizierten shRNAs solche angereichert waren, die gegen Gene spezifischer biologischer Prozesse gerichtet sind. Zum einen wurden Gene wie THOC1, NUP153 und LARP7 validiert, die eine Rolle im Prozeß der Elongation der RNA Polymerase II spielen. Zum anderen konnten Gene validiert werden die einen Beitrag bei der Neddylierung von Proteinen leisten. Durch die Depletion von Cullin 3, ein Bestandteil des BTB-CUL3-Rbx1 Ubiquitin-Ligase-Komplexes, der am Abbau von Cyclin E beteiligt ist, konnte gezeigt werden, dass zusammen mit der Aktivierung von N-Myc eine supraphysiologische Erhöhung von Cyclin E induziert wird. Dies führt zu einem S-Phase Arrest in der Zelle, der die DNA-Schadens-Signalkaskade auslöst. Zusammen mit den Ergebnissen einer Proteomanalyse, bei der neue N-Myc-assoziierte Proteine identifiziert wurden, konnte folgende Hypothese aufgestellt werden: In einer Neuroblastomzelle helfen diese neuen Interaktionspartner den durch die N-Myc Überexpression in der S-phase entstehenden Konflikt zwischen RNA-Polymerase II und Replikationsmaschinerie zu lösen. Der Verlust dieser Interaktion führt zu einer massiven Schädigung der DNA, worauf in der Zelle Apoptose ausgelöst wird. Des Weiteren führen auch die Inhibition oder Ausschaltung wesentlicher Komponenten des Neddylierungs-Signalwegs zu unlösbaren Problemen in der S-Phase des Zellzyklus. KW - Neuroblastom KW - synthetic lethality KW - apoptosis KW - cul3 ring ligase KW - replicative stress KW - N-Myc KW - Deregulierung KW - RNS-Interferenz KW - synthetische Letalität Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-103157 ER - TY - THES A1 - Xian, Yibo T1 - Identification of essential genes and novel virulence factors of Neisseria gonorrhoeae by transposon mutagenesis T1 - Identifizierung von essentiellen Genen und neuen Virulenzfaktoren von Neisseria gonorrhoeae durch Transposonmutagenese N2 - Neisseria gonorrhoeae is a human-specific pathogen that causes gonorrhea. It is defined as a super bacterium by the WHO due to the emergence of gonococci that are resistant to a variety of antibiotics and a rapidly increasing infection incidence. Genome-wide investigation of neisserial gene essentiality and novel virulence factors is urgently required in order to identify new targets for anti-neisserial therapeutics. To identify essential genes and new virulence factors, a high-density mutant library in N. gonorrhoeae MS11 was generated by in vitro transposon mutagenesis. The transposon library harbors more than 100,000 individual mutants, a density that is unprecedented in gonococcal research. Essential genes in N. gonorrhoeae were determined by enumerating frequencies of transposon insertion sites (TIS) with Illumina deep sequencing (Tn-seq). Tn-seq indicated an average distance between adjacent TIS of 25 bp. Statistical analysis unequivocally demonstrated 781 genes that were significantly depleted in TIS and thus are essential for Neisseria survival. A subset of the genes was experimentally verified to comprise essential genes and thus support the outcome of the study. The hereby identified candidate essential genes thus may constitute excellent targets for the development of new antibiotics or vaccines. In a second study, the transposon mutant library was applied in a genome-scale “negative-selection strategy” to identify genes that are involved in low phosphate-dependent invasion (LPDI). LPDI is dependent on the Neisseria porin subtype PorBIA which acts as an epithelial cell invasin in absence of phosphate and is associated with severe pathogenicity in disseminated gonococcal infections (DGI). Tn-seq demonstrated 98 genes, which were involved in adherence to host cells and 43 genes involved in host cell invasion. E.g. the hypothetical protein NGFG_00506, an ABC transporter ATP-binding protein NGFG_01643, as well as NGFG_04218 encoding a homolog of mafI in N. gonorrhoeae FA1090 were experimentally verified as new invasive factors in LPDI. NGFG_01605, a predicted protease, was identified to be a common factor involved in PorBIA, Opa50 and Opa57-mediated neisserial engulfment by the epithelial cells. Thus, this first systematic Tn-seq application in N. gonorrhoeae identified a set of previously unknown N. gonorrhoeae invasive factors which demonstrate molecular mechanisms of DGI. N2 - Neisseria gonorrhoeae ist ein human-spezifisches Pathogen, das die Krankheit Gonorrhoe verursacht. Aufgrund der steigenden Anzahl antibiotikaresistenter Gonokokken und der damit verbundenen, rapide zunehmenden Anzahl von Infektionen erklärte die WHO Gonokokken 2012 zum Superbakterium. Daher ist eine genomweite Untersuchung der neisseriellen Genessentiatialität und neuer Virulenzfaktoren dringend erforderlich, um neue Ziele für die antineisserielle Therapie zu identifizieren. Hierzu wurde eine high-density Mutantenbibliothek in N. gonorrhoeae MS11 durch in vitro Transposonmutagenese generiert. Die Transposonbibliothek enthält mehr als 100.000 individuelle Mutanten - eine Dichte, die in der Gonokokken-Forschung beispiellos ist. Essentielle Gene von N. gonorrhoeae wurden durch die Ermittlung der Häufigkeit von Transposon insertion sites (TIS) mit Hilfe von Illumina deep sequencing (Tn-seq) bestimmt. Tn-seq ergab eine durchschnittliche Distanz von 25 Basenpaaren zwischen benachbarten TIS. Die statistische Analyse zeigte eindeutig 781 Gene, die signifikant weniger TIS aufwiesen und deshalb als essentiell für das Überleben der Neisserien verstanden werden können. Für ausgewählte Gene wurde experimentell bestätigt, dass sie essentielle Gene beinhalten, wodurch das Ergebnis der Tn-seq unterstützt wird. Die hierbei identifizierten essentiellen Gene könnten exzellente Targets für die Entwicklung neuer Antibiotika oder Impfstoffe darstellen. In einer zweiten Studie wurde die Transposon Mutanten Bibliothek für eine genomweite „negative Selektionsstrategie“ bereitgestellt. Es sollten Gene identifiziert werden, die an der phosphatfreien Invasion (low phosphate-dependent invasion = LPDI) beteiligt sind. Die LPDI ist vom neisseriellen Porin Subtyp PorBIA abhängig, welches bei Epithelzellen in Abwesenheit von Phosphat als Invasin fungiert und mit einer schweren Pathogenität in disseminierenden Gonokokkeninfektionen (DGI) assoziiert ist. Tn-seq ergab 98 Gene, die an der Adhärenz an die Wirtszelle, und 43 Gene, die an der Wirtszellinvasion beteiligt waren. Zum Beispiel wurden das hypothetische Protein NGFG_00506, ein ABC Transporter, das ATP-bindende Protein NGFG_01643, wie auch NGFG_04218, das für ein Homolog von mafI in N. gonorrhoeae FA1090 kodiert, experimentell als neue Invasionsfaktoren in der LPDI verifiziert. NGFG_01605, bei dem angenommen wird, dass es sich um eine Protease handelt, wurde als ein allgemeiner Faktor identifiziert, der an der PorBIA-, Opa50- and Opa57-vermittelten Einstülpung der Membran von Epithelzellen beteiligt ist. Die erste systematische Anwendung von Tn-seq in N. gonorrhoeae identifizierte eine Reihe bisher unbekannter Invasionsfaktoren von N. gonorrhoeae, die molekulare Mechanismen der DGI zeigen. KW - Neisseria gonorrhoeae KW - transposon mutagenesis KW - essential genes KW - virulence factors KW - Virulenzfaktor KW - Transposon KW - Mutagenese Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-102659 ER - TY - JOUR A1 - Wölfling, Mirko A1 - Becker, Mira C. A1 - Uhl, Britta A1 - Traub, Anja A1 - Fiedler, Konrad T1 - How differences in the settling behaviour of moths (Lepidoptera) may contribute to sampling bias when using automated light traps JF - European Journal of Entomology N2 - Quantitative community-wide moth surveys frequently employ flight-interception traps equipped with UV-light emitting sources as attractants. It has long been known that moth species differ in their responsiveness to light traps. We studied how the settling behaviour of moths at a light trap may further contribute to sampling bias. We observed the behaviour of 1426 moths at a light tower. Moths were classified as either, settling and remaining still after arrival, or continually moving on the gauze for extended periods of time. Moths that did not move after settling may not end up in the sampling container of the light trap and therefore are under-represented in automated trap samples relative to their true proportions in the community. Our analyses revealed highly significant behavioural differences between moths that differed in body size. Small moths were more likely to remain stationary after settling. As a corollary, representatives of three taxa, which in Europe are predominantly small species (Nolidae, Geometridae: Eupitheciini, Erebidae: Lithosiini), usually settled down immediately, whereas most other moths remained active on or flying around the trap for some time. Moth behaviour was also modulated by ambient temperature. At high temperatures, they were less likely to settle down immediately, but this behavioural difference was most strongly apparent among medium-sized moths. These results indicate the likely extent of the sampling bias when analysing and interpreting automated light-trap samples. Furthermore, to control for temperature modulated sampling bias temperature should always be recorded when sampling moths using flight-interception traps. KW - Lepidoptera KW - moths KW - biodiversity assessment KW - sampling method KW - light-trapping KW - sampling bias Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-191154 VL - 113 ER - TY - JOUR A1 - Wäschke, Nicole A1 - Hardge, Kerstin A1 - Hancock, Christine A1 - Hilker, Monika A1 - Obermaier, Elisabeth A1 - Meiners, Torsten T1 - Odour Environments: How Does Plant Diversity Affect Herbivore and Parasitoid Orientation? JF - PlOS ONE N2 - Plant diversity is known to affect success of host location by pest insects, but its effect on olfactory orientation of non-pest insect species has hardly been addressed. First, we tested in laboratory experiments the hypothesis that non-host plants, which increase odour complexity in habitats, affect the host location ability of herbivores and parasitoids. Furthermore, we recorded field data of plant diversity in addition to herbivore and parasitoid abundance at 77 grassland sites in three different regions in Germany in order to elucidate whether our laboratory results reflect the field situation. As a model system we used the herb Plantago lanceolata, the herbivorous weevil Mecinus pascuorum, and its larval parasitoid Mesopolobus incultus. The laboratory bioassays revealed that both the herbivorous weevil and its larval parasitoid can locate their host plant and host via olfactory cues even in the presence of non-host odour. In a newly established two-circle olfactometer, the weevils capability to detect host plant odour was not affected by odours from non-host plants. However, addition of non-host plant odours to host plant odour enhanced the weevils foraging activity. The parasitoid was attracted by a combination of host plant and host volatiles in both the absence and presence of non-host plant volatiles in a Y-tube olfactometer. In dual choice tests the parasitoid preferred the blend of host plant and host volatiles over its combination with non-host plant volatiles. In the field, no indication was found that high plant diversity disturbs host (plant) location by the weevil and its parasitoid. In contrast, plant diversity was positively correlated with weevil abundance, whereas parasitoid abundance was independent of plant diversity. Therefore, we conclude that weevils and parasitoids showed the sensory capacity to successfully cope with complex vegetation odours when searching for hosts. KW - dentichasmias busseolae KW - nonhost plant KW - volatiles KW - selection KW - invertebrate herbivory KW - location behavior KW - foraging behavior KW - background odor KW - natural enemies Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-117687 SN - 1932-6203 VL - 9 IS - 1 ER - TY - JOUR A1 - Wäldchen, Sina A1 - Lehmann, Julian A1 - Klein, Teresa A1 - van de Linde, Sebastian A1 - Sauer, Markus T1 - Light-induced cell damage in live-cell super-resolution microscopy JF - Scientific Reports N2 - Super-resolution microscopy can unravel previously hidden details of cellular structures but requires high irradiation intensities to use the limited photon budget efficiently. Such high photon densities are likely to induce cellular damage in live-cell experiments. We applied single-molecule localization microscopy conditions and tested the influence of irradiation intensity, illumination-mode, wavelength, light-dose, temperature and fluorescence labeling on the survival probability of different cell lines 20-24 hours after irradiation. In addition, we measured the microtubule growth speed after irradiation. The photo-sensitivity is dramatically increased at lower irradiation wavelength. We observed fixation, plasma membrane permeabilization and cytoskeleton destruction upon irradiation with shorter wavelengths. While cells stand light intensities of similar to 1 kW cm\(^{-2}\) at 640 nm for several minutes, the maximum dose at 405 nm is only similar to 50 J cm\(^{-2}\), emphasizing red fluorophores for live-cell localization microscopy. We also present strategies to minimize phototoxic factors and maximize the cells ability to cope with higher irradiation intensities. KW - optical reconstruction microscopy KW - tag fusion proteins KW - localization microscopy KW - photodynamic therapy KW - diffraction limit KW - illumination microscopy KW - structured illumination KW - fluorescent probes KW - in vitro KW - dynamics Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-145207 VL - 5 IS - 15348 ER - TY - JOUR A1 - Wunder, Juliane A1 - Pemp, Daniela A1 - Cecil, Alexander A1 - Mahdiani, Maryam A1 - Hauptstein, René A1 - Schmalbach, Katja A1 - Geppert, Leo N. A1 - Ickstadt, Katja A1 - Esch, Harald L. A1 - Dankekar, Thomas A1 - Lehmann, Leane T1 - Influence of breast cancer risk factors on proliferation and DNA damage in human breast glandular tissues: role of intracellular estrogen levels, oxidative stress and estrogen biotransformation JF - Archives of Toxicology N2 - Breast cancer etiology is associated with both proliferation and DNA damage induced by estrogens. Breast cancer risk factors (BCRF) such as body mass index (BMI), smoking, and intake of estrogen-active drugs were recently shown to influence intratissue estrogen levels. Thus, the aim of the present study was to investigate the influence of BCRF on estrogen-induced proliferation and DNA damage in 41 well-characterized breast glandular tissues derived from women without breast cancer. Influence of intramammary estrogen levels and BCRF on estrogen receptor (ESR) activation, ESR-related proliferation (indicated by levels of marker transcripts), oxidative stress (indicated by levels of GCLC transcript and oxidative derivatives of cholesterol), and levels of transcripts encoding enzymes involved in estrogen biotransformation was identified by multiple linear regression models. Metabolic fluxes to adducts of estrogens with DNA (E-DNA) were assessed by a metabolic network model (MNM) which was validated by comparison of calculated fluxes with data on methoxylated and glucuronidated estrogens determined by GC- and UHPLC-MS/MS. Intratissue estrogen levels significantly influenced ESR activation and fluxes to E-DNA within the MNM. Likewise, all BCRF directly and/or indirectly influenced ESR activation, proliferation, and key flux constraints influencing E-DNA (i.e., levels of estrogens, CYP1B1, SULT1A1, SULT1A2, and GSTP1). However, no unambiguous total effect of BCRF on proliferation became apparent. Furthermore, BMI was the only BCRF to indeed influence fluxes to E-DNA (via congruent adverse influence on levels of estrogens, CYP1B1 and SULT1A2). KW - metabolic network model KW - estrogens KW - human breast KW - multiple linear regression Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-265343 SN - 1432-0738 VL - 96 IS - 2 ER - TY - JOUR A1 - Wu, Yu A1 - Pons, Valérie A1 - Goudet, Amélie A1 - Panigai, Laetitia A1 - Fischer, Annette A1 - Herweg, Jo-Ana A1 - Kali, Sabrina A1 - Davey, Robert A. A1 - Laporte, Jérôme A1 - Bouclier, Céline A1 - Yousfi, Rahima A1 - Aubenque, Céline A1 - Merer, Goulven A1 - Gobbo, Emilie A1 - Lopez, Roman A1 - Gillet, Cynthia A1 - Cojean, Sandrine A1 - Popoff, Michel R. A1 - Clayette, Pascal A1 - Le Grand, Roger A1 - Boulogne, Claire A1 - Tordo, Noël A1 - Lemichez, Emmanuel A1 - Loiseau, Philippe M. A1 - Rudel, Thomas A1 - Sauvaire, Didier A1 - Cintrat, Jean-Christophe A1 - Gillet, Daniel A1 - Barbier, Julien T1 - ABMA, a small molecule that inhibits intracellular toxins and pathogens by interfering with late endosomal compartments JF - Scientific Reports N2 - Intracellular pathogenic microorganisms and toxins exploit host cell mechanisms to enter, exert their deleterious effects as well as hijack host nutrition for their development. A potential approach to treat multiple pathogen infections and that should not induce drug resistance is the use of small molecules that target host components. We identifed the compound 1-adamantyl (5-bromo-2-methoxybenzyl) amine (ABMA) from a cell-based high throughput screening for its capacity to protect human cells and mice against ricin toxin without toxicity. This compound efciently protects cells against various toxins and pathogens including viruses, intracellular bacteria and parasite. ABMA provokes Rab7-positive late endosomal compartment accumulation in mammalian cells without affecting other organelles (early endosomes, lysosomes, the Golgi apparatus, the endoplasmic reticulum or the nucleus). As the mechanism of action of ABMA is restricted to host-endosomal compartments, it reduces cell infection by pathogens that depend on this pathway to invade cells. ABMA may represent a novel class of broad-spectrum compounds with therapeutic potential against diverse severe infectious diseases. KW - biology KW - antimicrobials KW - high-throughput screening KW - infectious diseases Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-173170 VL - 7 ER - TY - JOUR A1 - Wu, Hao A1 - Zhao, Xiufeng A1 - Hochrein, Sophia M. A1 - Eckstein, Miriam A1 - Gubert, Gabriela F. A1 - Knöpper, Konrad A1 - Mansilla, Ana Maria A1 - Öner, Arman A1 - Doucet-Ladevèze, Remi A1 - Schmitz, Werner A1 - Ghesquière, Bart A1 - Theurich, Sebastian A1 - Dudek, Jan A1 - Gasteiger, Georg A1 - Zernecke, Alma A1 - Kobold, Sebastian A1 - Kastenmüller, Wolfgang A1 - Vaeth, Martin T1 - Mitochondrial dysfunction promotes the transition of precursor to terminally exhausted T cells through HIF-1α-mediated glycolytic reprogramming JF - Nature Communications N2 - T cell exhaustion is a hallmark of cancer and persistent infections, marked by inhibitory receptor upregulation, diminished cytokine secretion, and impaired cytolytic activity. Terminally exhausted T cells are steadily replenished by a precursor population (Tpex), but the metabolic principles governing Tpex maintenance and the regulatory circuits that control their exhaustion remain incompletely understood. Using a combination of gene-deficient mice, single-cell transcriptomics, and metabolomic analyses, we show that mitochondrial insufficiency is a cell-intrinsic trigger that initiates the functional exhaustion of T cells. At the molecular level, we find that mitochondrial dysfunction causes redox stress, which inhibits the proteasomal degradation of hypoxia-inducible factor 1α (HIF-1α) and promotes the transcriptional and metabolic reprogramming of Tpex cells into terminally exhausted T cells. Our findings also bear clinical significance, as metabolic engineering of chimeric antigen receptor (CAR) T cells is a promising strategy to enhance the stemness and functionality of Tpex cells for cancer immunotherapy. KW - cytotoxic T cells KW - infection KW - lymphocyte differentiation KW - translational research Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-358052 VL - 14 ER - TY - THES A1 - Worschech, Andrea T1 - Oncolytic Therapy with Vaccinia Virus GLV-1h68 - Comparative Microarray Analysis of Infected Xenografts and Human Tumor Cell Lines - T1 - Onkolytische Therapy mit Vaccinia Virus GLV-1h68 - Vergleichende Mikroarray Analyse von infizierten Xenografts und humanen Tumorzelllinien - N2 - Aim of this thesis was to study the contribution of the hosts immune system during tumor regression. A wild-type rejection model was studied in which tumor regression is mediated through an adaptive, T cell host response (Research article 1). Additionally, the relationship between VACV infection and cancer rejection was assessed by applying organism-specific microarray platforms to infected and non-infected xenografts. It could be shown that tumor rejection in this nude mouse model was orchestrated solely by the hosts innate immune system without help of the adaptive immunity. In a third study the inflammatory baseline status of 75 human cancer cell lines was tested in vitro which was correlated with the susceptibility to VACV and Adenovirus 5 (Ad5) replication of the respective cell line (Manuscript for Research article 3). Although xenografts by themselves lack the ability to signal danger and do not provide sufficient proinflammatory signals to induce acute inflammation, the presence of viral replication in the oncolytic xenograft model provides the "tissue-specific trigger" that activates the immune response and in concordance with the hypothesis, the ICR is activated when chronic inflammation is switched into an acute one. Thus, in conditions in which a switch from a chronic to an acute inflammatory process can be induced by other factors like the immune-stimulation induced by the presence of a virus in the target tissue, adaptive immune responses may not be necessary and immune-mediated rejection can occur without the assistance of T or B cells. However, in the regression study using neu expressing MMC in absence of a stimulus such as a virus and infected cancer cells thereafter, adaptive immunity is needed to provoke the switch into an acute inflammation and initiate tissue rejection. Taken together, this work is supportive of the hypothesis that the mechanisms prompting TSD differ among immune pathologies but the effect phase converges and central molecules can be detected over and over every time TSD occurs. It could be shown that in presence of a trigger such as infection with VACV and functional danger signaling pathways of the infected tumor cells, innate immunity is sufficient to orchestrate rejection of manifested tumors. N2 - Ziel dieser Arbeit war, die Beteiligung des Wirts-eigenen Immunsystems bei der Tumoregression zu analysieren. Mittels eines Wildtyp-Regressionsmodells, wurde der Anteil des adaptiven Immunsystems studiert (Research-Artikel 1). Mit Hilfe von Organismus-spezifischen Mikroarrays und Genexpressionsanalysen konnte in einem Nacktmausmodell gezeigt werden, dass erfolgreiche, durch onkolytische VACV-vermittelte Tumortherapie auch ohne Beteiligung des adaptiven Immunsystems möglich ist (Research Artikel 2). In einer dritten Studie wurden 75 humane Tumorzelllinien auf ihren intrinsischen Entzündungsstatus hin getestet und bezüglich eines Zusammenhanges von diesem mit der Replikationsfähigkeit von VACV und Adenovirus 5 (Ad5) analysiert (Manuskript für den Research-Artikel 3). Obwohl Xenografts allein kein ausreichendes „Gefahrsignal“ geben und durch das Fehlen einer pro-inflammatorischen Stimulierung keine akute Entzündung verursachen können, ist die Infektion mit onkolytischem VACV ausreichend, um den Gewebe-spezifischen „Trigger“ darzustellen. In diesem Fall wird die Immunantwort aktiviert und nach der Hypothese des „Immunologic Constant of Rejection“ (ICR) geschieht dies, wenn eine chronische in eine akute Inflammation verändert wird. In dem beschriebenen onkolytischen Regressionsmodell ist die Präsenz des Virus ausreichend, um das Immunsystem zu aktivieren, d.h. die chronische Entzündung im Tumor in eine akute umzuwandeln. Dabei ist die adaptive Immunität mit T- und B-Zell-Aktivierung nicht notwendig für die Rückbildung des Tumors. In Abwesenheit eines solchen Stimulus, wie in der ersten Studie mit neu-exprimierenden MMCs, wird die Spezifität der adaptiven Immunantwort benötigt, um die akute Inflammation anzustoßen und die Tumorregression voranzutreiben. Zusammengefasst unterstützt diese Arbeit die Hypothese, dass die Mechanismen, die zu „tissue specific destruction“ (TSD) führen, in verschiedenen immunologischen Erkrankungen zwar divergieren, der Effektor-Mechanismus aber stets der Gleiche ist. Es zeigte sich, dass in Anwesenheit eines „triggers“, wie z.B. der VACV-Infektion und intakten „danger signaling pathways“ der Tumorzellen, die angeborene Immunität allein ausreicht, um die Tumorrückbildung zu vermitteln. KW - Tumorimmunologie KW - Tumor KW - Vaccinia-Virus KW - Interferon KW - Interferon Regulator Faktor 1 KW - Tumorregression KW - HT-29 KW - GI-101A KW - tissue-specific destruction Y1 - 2010 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-45338 ER - TY - JOUR A1 - Woodcock, B. A. A1 - Garratt, M. P. D. A1 - Powney, G. D. A1 - Shaw, R. F. A1 - Osborne, J. L. A1 - Soroka, J. A1 - Lindström, S. A. M. A1 - Stanley, D. A1 - Ouvrard, P. A1 - Edwards, M. E. A1 - Jauker, F. A1 - McCracken, M. E. A1 - Zou, Y. A1 - Potts, S. G. A1 - Rundlöf, M. A1 - Noriega, J. A. A1 - Greenop, A. A1 - Smith, H. G. A1 - Bommarco, R. A1 - van der Werf, W. A1 - Stout, J. C. A1 - Steffan-Dewenter, I. A1 - Morandin, L. A1 - Bullock, J. M. A1 - Pywell, R. F. T1 - Meta-analysis reveals that pollinator functional diversity and abundance enhance crop pollination and yield JF - Nature Communications N2 - How insects promote crop pollination remains poorly understood in terms of the contribution of functional trait differences between species. We used meta-analyses to test for correlations between community abundance, species richness and functional trait metrics with oilseed rape yield, a globally important crop. While overall abundance is consistently important in predicting yield, functional divergence between species traits also showed a positive correlation. This result supports the complementarity hypothesis that pollination function is maintained by non-overlapping trait distributions. In artificially constructed communities (mesocosms), species richness is positively correlated with yield, although this effect is not seen under field conditions. As traits of the dominant species do not predict yield above that attributed to the effect of abundance alone, we find no evidence in support of the mass ratio hypothesis. Management practices increasing not just pollinator abundance, but also functional divergence, could benefit oilseed rape agriculture. KW - agroecology KW - agriculture KW - ecosystem services KW - environmental sciences Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-233787 VL - 10 ER - TY - THES A1 - Wong, Amanda T1 - Implications of Advanced Glycation Endproducts in Oxidative Stress and Neurodegenerative Disorders T1 - Verbindungen zwischen Oxidativen Stress und Advanced Glycation Endproducts in der Neurodegeneration N2 - The reactions of reducing sugars with primary amino groups are the most common nonenzymatic modifications of proteins. Subsequent rearrangements, oxidations, and dehydrations yield a heterogeneous group of mostly colored and fluorescent compounds, termed "Maillard products" or advanced glycation end products (AGEs). AGE formation has been observed on long-lived proteins such as collagen, eye lens crystalline, and in pathological protein deposits in Alzheimer's (AD) and Parkinson's disease (PD) and dialysis-related amyloidosis. AGE-modified proteins are also involved in the complications of diabetes. AGEs accumulate in the the ß-amyloid plaques and neurofibrillary tangles (NFT) associated with AD and in the Lewy bodies characteristic of PD. Increasing evidence supports a role for oxidative stress in neurodegenerative disorders such as AD and PD. AGEs have been shown to contribute towards oxidative damage and chronic inflammation, whereby activated microglia secrete cytokines and free radicals, including nitric oxide (NO). Roles proposed for NO in the pathophysiology of the central nervous system are increasingly diverse and range from intercellular signaling, through necrosis of cells and invading pathogens, to the involvement of NO in apoptosis. Using in vitro experiments, it was shown that AGE-modified bovine serum albumin (BSA-AGE) and AGE-modified ß-amyloid, but not their unmodified proteins, induce NO production in N-11 murine microglia cells. This was mediated by the receptor for AGEs (RAGE) and upregulation of the inducible nitric oxide synthase (iNOS). AGE-induced enzyme activation and NO production could be blocked by intracellular-acting antioxidants: Ginkgo biloba special extract EGb 761, the estrogen derivative, 17ß-estradiol, R-(+)-thioctic acid, and a nitrone-based free radical trap, N-tert.-butyl-*-phenylnitrone (PBN). Methylglyoxal (MG) and 3-deoxyglucosone (3-DG), common precursors in the Maillard reaction, were also tested for their ability to induce the production of NO in N-11 microglia. However, no significant changes in nitrite levels were detected in the cell culture medium. The significance of these findings was supported by in vivo immunostaining of AD brains. Single and double immunostaining of cryostat sections of normal aged and AD brains was performed with polyclonal antibodies to AGEs and iNOS and monoclonal antibodies to Aß and PHF-1 (marker for NFT) and reactive microglia. In aged normal individuals as well as early stage AD brains (i.e. no pathological findings in isocortical areas), a few astrocytes showed co-localisation of AGE and iNOS in the upper neuronal layers of the temporal (Area 22) and entorhinal (Area 28, 34) cortices compared with no astrocytes detected in young controls. In late AD brains, there was a much denser accumulation of astrocytes co-localised with AGE and iNOS in the deeper and particularly upper neuronal layers. Also, numerous neurons with diffuse AGE but not iNOS reactivity and some AGE and iNOS-positive microglia were demonstrated, compared with only a few AGE-reactive neurons and no microglia in controls. Finally, astrocytes co-localised with AGE and iNOS as well as AGE and ß-amyloid were found surrounding mature but not diffuse ß-amyloid plaques in the AD brain. Parts of NFT were AGE-immunoreactive. Immunohistochemical staining of cryostat sections of normal aged and PD brains was performed with polyclonal antibodies to AGEs. The sections were counterstained with monoclonal antibodies to neurofilament components and a-synuclein. AGEs and a-synuclein were colocalized in very early Lewy bodies in the substantia nigra of cases with incidental Lewy body disease. These results support an AGE-induced oxidative damage due to the action of free radicals, such as NO, occurring in the AD and PD brains. Furthermore, the involvement of astrocytes and microglia in this pathological process was confirmed immunohistochemically in the AD brain. It is suggested that oxidative stress and AGEs participate in the very early steps of Lewy body formation and resulting cell death in PD. Since the iNOS gene can be regulated by redox-sensitive transcription factors, the use of membrane permeable antioxidants could be a promising strategy for the treatment and prevention of chronic inflammation in neurodegenerative disorders. N2 - Die Glykierung oder Maillard-Reaktion ist neben der oxidativen Modifikation die bekannteste nicht-enzymatische posttranslationale Modifikation von Proteinen. Glykierung startet mit der Reaktion von reduzierenden Zuckern mit primären Aminogruppen. Nachfolgenden Umlagerungen, Oxidationen und Dehydra- tionen führen zu einer heterogenen Gruppe von farbigen und fluoreszierenden Verbindungen, den sogenannten "Maillard products" oder "advanced glycation end products" (AGEs). Diese Vorgänge werden besonders an langlebigen Proteinen wie Kollagen und Kristallin der Augenlinsen sowie in pathologischen Proteinab- lagerungen bei der Alzheimer-Demenz (AD), der Parkinson-Krankheit (PD) und bei Hämodialyse beobachtet. AGE-modifizierte Proteine sind auch aktiv beteiligt an den Spätkomplikationen des Diabetes mellitus. AGEs reichern sich im Alzheimer Gehirn in den ß-Amyloid-Plaques und den neurofibrillären Bündeln (tangles, NFT), sowie in den für PD charakteristisch- en Lewi-Körpern an. Immer mehr Befunde belegen die Rolle von oxidativem Stress in neurodegenerativen Erkrankungen wie AD und PD. Es konnte gezeigt werden, dass AGEs an oxidativer Schädigung und chronischer Entzündung Anteil haben, wobei aktivierte Mikroglia Cytokine und freie Radikale, inklusive Stickstoffmonoxid (NO) sezernieren. Vermutungen über die Rolle von NO in der Pathophysiologie des Zentralnervensystems gehen weit auseinander und reichen von interzellulärer Signalübertragung über nekrotischen Zelltod und eindringende pathogene Substanzen bis zur Beteiligung von NO an der Apoptose. In einem Zellkultur Modell konnte in vitro gezeigt werden, dass AGE- modifiziertes Albumin (BSA-AGE) und AGE-modifiziertes ß-Amyloid, aber nicht die unmodifizierten Proteine, die Synthese von NO in N-11 Maus-Mikrogliazellen induzieren. Diese wird möglicherweise vom Rezeptor für AGE (RAGE) und durch eine Steigerung der Expression der induzierbaren Stickstoffmonoxid-Synthase (iNOS) vermittelt. AGE-induzierte Enzymexpression und NO-Produktion konnten durch folgende intrazellulär wirkende Antioxidantien blockiert werden: Ginkgo biloba Spezialextrakt EGb 761, das Östrogenderivat 17ß-Estradiol, alpha- Liponsäure, und ein Radikalfänger, N-tert.-butyl-*-phenylnitrone (PBN). Neben AGEs wurden auch reaktive Dicarbonyle wie Methylglyoxal (MG) und 3- Deoxyglucosone (3-DG), Vorläufer der Maillard-Reaktion, auf ihre Fähigkeit untersucht, die Synthese von NO in N-11 Mikroglia zu induzieren. Es konnten jedoch keine Induktion der NO-Produktion festgestellt werden. Die Bedeutung dieser in vitro-Ergebnisse wurden durch in vivo Immunohisto- chemischen Untersuchungen an AD Gehirnen bestätigt. Einfache und doppelte Immunfärbungen wurden an Gefrierschnitten von normal gealterten Gehirnen und AD-Gehirnen mit polyklonalen Antikörpern gegen AGEs und iNOS und monoklonalen Antikörpern gegen Aß, PHF-1 (zur spezifischen Markierung der NFT) und reaktive Mikroglia angefertigt. Bei normal gealterten Personen sowie bei AD Erkrankten im Frühstadium (d.h. keine pathologischen Veränderungen in iso- kortikalen Gebieten) wiesen wenige Astrozyten eine Kolokalisation von AGE und iNOS in den oberen Neuronenschichten des temporalen (Area 22) und entorhinalen (Area 28, 34) Kortex auf. Im Vergleich dazu wurden keine Astrozyten in jungen Kontrollgehirnen gefunden. In fortgeschrittenen Alzheimergehirnen wurde eine viel dichtere Anreicherung von Astrozyten, kolokalisiert mit AGE und iNOS in den tieferen, und insbesondere in den oberen Neuronenschichten gefunden. Weiterhin konnten zahlreiche Neurone mit diffuser AGE-Reaktivität, aber ohne iNOS-Reaktivität, sowie einige AGE- und iNOS-positive Mikroglia gezeigt werden, im Vergleich zu nur wenigen AGE-reaktiven Neuronen und keinen Mikroglia in den Kontrollen. Schliesslich wurden in Astrozyten, die reife, aber nicht diffuse ß-Amyloid-Plaques im AD-Gehirn umlagern, AGE mit iNOS sowie mit ß-Amyloid kolokalisiert gefunden. Teile der NFT waren AGE-immunoreaktiv. Immunhistochemische Färbung an Gefrierschnitten von normal gealterten und PD- Gehirnen wurden mit polyklonalen Antikörpern gegen AGEs durchgeführt. Die Schnitte wurden mit monoklonalen Antikörpern gegen Neurofilamentkomponenten und a-Synuclein gegengefärbt. AGEs und a-Synuclein waren kolokalisiert in sehr frühen Lewi-Körpern der Substantia nigra in Gehirnen mit vorhandener Lewi-Körper-Demenz. Diese Ergebnisse unterstützen die These AGE-induzierter oxidativer Schädigung mittels freier Radikale wie z.B. NO in AD- und PD- Gehirnen. Ausserdem wurde die Beteiligung von Astrozyten und Mikroglia an diesem pathologischen Prozess immunhistochemisch im Alzheimergehirn bestätigt. Es liegt nahe, dass oxidativer Stress und AGEs an den sehr frühen Stufen der Lewi-Körper-Bildung und dem daraus resultierenden Zelltod in PD beteiligt sind. Da das iNOS-Gen durch redoxsensitive Transkriptionsfaktoren reguliert werden kann, könnte die Verwendung membranpermeabler Antioxidantien eine erfolgversprechende Strategie für die Behandlung und Prävention chronischer Entzündungen bei neurodegenera- tiven Erkrankungen darstellen. KW - Maillard-Reaktion KW - Alzheimer-Krankheit KW - Antioxidans KW - advanced glycation end products KW - Alzheimer Erkrankung KW - Antioxidantien KW - iNOS KW - advanced glycation end products KW - Alzheimer's disease KW - antioxidants KW - iNOS Y1 - 2001 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-2537 ER - TY - THES A1 - Wolter, Steve T1 - Single-molecule localization algorithms in super-resolution microscopy T1 - Einzelmoleküllokalisierungsalgorithmen in der superauflösenden Mikroskopie N2 - Lokalisationsmikroskopie ist eine Methodenklasse der superauflösenden Fluoreszenzmikroskopie, deren Methoden sich durch stochastische zeitliche Isolation der Fluoreszenzemission auszeichnen. Das Blinkverhalten von Fluorophoren wird so verändert, dass gleichzeitige Aktivierung von einander nahen Fluorophoren unwahrscheinlich ist. Bekannte okalisationsmikroskopische Methoden umfassen dSTORM, STORM, PALM, FPALM, oder GSDIM. Lokalisationsmikroskopie ist von hohem biologischem Interesse, weil sie die Auflösung des Fluoreszenzmikroskops bei minimalem technischem Aufwand um eine Größenordnung verbessert. Der verbundene Rechenaufwand ist allerdings erheblich, da Millionen von Fluoreszenzemissionen einzeln mit Nanometergenauigkeit lokalisiert werden müssen. Der Rechen- und Implementationsaufwand dieser Auswertung hat die Verbreitung der superauflösenden Mikroskopie lange verzögert. Diese Arbeit beschreibt meine algorithmische Grundstruktur für die Auswertung lokalisationsmikroskopischer Daten. Die Echtzeitfähigkeit, d.h. eine Auswertegeschwindigkeit oberhalb der Datenaufnahmegeschwindigkeit an normalen Messaufbauten, meines neuartigen und quelloffenen Programms wird demonstriert. Die Geschwindigkeit wird auf verbrauchermarktgängigen Prozessoren erreicht und dadurch spezialisierte Rechenzentren oder der Einsatz von Grafikkarten vermieden. Die Berechnung wird mit dem allgemein anerkannten Gaussschen Punktantwortmodell und einem Rauschmodell auf Basis der größten Poissonschen Wahrscheinlichkeit durchgeführt. Die algorithmische Grundstruktur wird erweitert, um robuste und optimale Zweifarbenauswertung zu realisieren und damit korrelative Mikroskopie zwischen verschiedenen Proteinen und Strukturen zu ermöglichen. Durch den Einsatz von kubischen Basissplines wird die Auswertung von dreidimensionalen Proben vereinfacht und stabilisiert, um präzisem Abbilden von mikrometerdicken Proben näher zu kommen. Das Grenzverhalten von Lokalisationsalgorithmen bei hohen Emissionsdichten wird untersucht. Abschließend werden Algorithmen für die Anwendung der Lokalisationsmikroskopie auf verbreitete Probleme der Biologie aufgezeigt. Zelluläre Bewegung und Motilität werden anhand der in vitro Bewegung von Myosin-Aktin-Filamenten studiert. Lebendzellbildgebung mit hellen und stabilen organischen Fluorophoren wird mittels SNAP-tag-Fusionsproteinen realisiert. Die Analyse des Aufbaus von Proteinklumpen zeigt, wie Lokalisationsmikroskopie neue quantitative Ansätze jenseits reiner Bildgebung bietet. N2 - Localization microscopy is a class of super-resolution fluorescence microscopy techniques. Localization microscopy methods are characterized by stochastic temporal isolation of fluorophore emission, i.e., making the fluorophores blink so rapidly that no two are likely to be photoactive at the same time close to each other. Well-known localization microscopy methods include dSTORM}, STORM, PALM, FPALM, or GSDIM. The biological community has taken great interest in localization microscopy, since it can enhance the resolution of common fluorescence microscopy by an order of magnitude at little experimental cost. However, localization microscopy has considerable computational cost since millions of individual stochastic emissions must be located with nanometer precision. The computational cost of this evaluation, and the organizational cost of implementing the complex algorithms, has impeded adoption of super-resolution microscopy for a long time. In this work, I describe my algorithmic framework for evaluating localization microscopy data. I demonstrate how my novel open-source software achieves real-time data evaluation, i.e., can evaluate data faster than the common experimental setups can capture them. I show how this speed is attained on standard consumer-grade CPUs, removing the need for computing on expensive clusters or deploying graphics processing units. The evaluation is performed with the widely accepted Gaussian PSF model and a Poissonian maximum-likelihood noise model. I extend the computational model to show how robust, optimal two-color evaluation is realized, allowing correlative microscopy between multiple proteins or structures. By employing cubic B-splines, I show how the evaluation of three-dimensional samples can be made simple and robust, taking an important step towards precise imaging of micrometer-thick samples. I uncover the behavior and limits of localization algorithms in the face of increasing emission densities. Finally, I show up algorithms to extend localization microscopy to common biological problems. I investigate cellular movement and motility by considering the in vitro movement of myosin-actin filaments. I show how SNAP-tag fusion proteins enable imaging with bright and stable organic fluorophores in live cells. By analyzing the internal structure of protein clusters, I show how localization microscopy can provide new quantitative approaches beyond pure imaging. KW - super-resolution microscopy KW - fluorescence KW - scientific computing KW - dSTORM KW - localization microscopy KW - PALM KW - 3D microscopy KW - two-color microscopy KW - Fluoreszenzmikroskopie KW - Bildauflösung KW - Bioinformatik Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-109370 ER - TY - JOUR A1 - Wolter, Patrick A1 - Hanselmann, Steffen A1 - Pattschull, Grit A1 - Schruf, Eva A1 - Gaubatz, Stefan T1 - Central spindle proteins and mitotic kinesins are direct transcriptional targets of MuvB, B-MYB and FOXM1 in breast cancer cell lines and are potential targets for therapy JF - Oncotarget N2 - The MuvB multiprotein complex, together with B-MYB and FOXM1 (MMB-FOXM1), plays an essential role in cell cycle progression by regulating the transcription of genes required for mitosis and cytokinesis. In many tumors, B-MYB and FOXM1 are overexpressed as part of the proliferation signature. However, the transcriptional targets that are important for oncogenesis have not been identified. Given that mitotic kinesins are highly expressed in cancer cells and that selected kinesins have been reported as target genes of MMB-FOXM1, we sought to determine which mitotic kinesins are directly regulated by MMB-FOXM1. We demonstrate that six mitotic kinesins and two microtubule-associated non-motor proteins (MAPs) CEP55 and PRC1 are direct transcriptional targets of MuvB, B-MYB and FOXM1 in breast cancer cells. Suppression of KIF23 and PRC1 strongly suppressed proliferation of MDA-MB-231 cells. The set of MMB-FOXM1 regulated kinesins genes and 4 additional kinesins which we referred to as the mitotic kinesin signature (MKS) is linked to poor outcome in breast cancer patients. Thus, mitotic kinesins could be used as prognostic biomarker and could be potential therapeutic targets for the treatment of breast cancer. KW - breast cancer KW - kinesin KW - cell cycle KW - cytokinesis Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-171851 VL - 8 IS - 7 ER - TY - JOUR A1 - Wolf, Matthias A1 - Chen, Shilin A1 - Song, Jingyuan A1 - Ankenbrand, Markus A1 - Müller, Tobias T1 - Compensatory Base Changes in ITS2 Secondary Structures Correlate with the Biological Species Concept Despite Intragenomic Variability in ITS2 Sequences – A Proof of Concept JF - PLoS ONE N2 - Compensatory base changes (CBCs) in internal transcribed spacer 2 (ITS2) rDNA secondary structures correlate with Ernst Mayr’s biological species concept. This hypothesis also referred to as the CBC species concept recently was subjected to large-scale testing, indicating two distinct probabilities. (1) If there is a CBC then there are two different species with a probability of ~0.93. (2) If there is no CBC then there is the same species with a probability of ~0.76. In ITS2 research, however, the main problem is the multicopy nature of ITS2 sequences. Most recently, 454 pyrosequencing data have been used to characterize more than 5000 intragenomic variations of ITS2 regions from 178 plant species, demonstrating that mutation of ITS2 is frequent, with a mean of 35 variants per species, respectively per individual organism. In this study, using those 454 data, the CBC criterion is reconsidered in the light of intragenomic variability, a proof of concept, a necessary criterion, expecting no intragenomic CBCs in variant ITS2 copies. In accordance with the CBC species concept, we could demonstrate that the probability that there is no intragenomic CBC is ~0.99. KW - citrus KW - concerted evolution KW - DNA sequences KW - Genome evolution KW - Phylogenetics KW - plant evolution KW - sequence alignment KW - sequence databases Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96450 ER - TY - JOUR A1 - Wolf, Matthias T1 - How to teach about what is a species JF - Biology N2 - To ask students what a species is always has something rhetorical about it. Too quickly comes the rote answer, often learned by heart without ever thinking about it: “A species is a reproductive community of populations (reproductively isolated from others), which occupies a specific niche in nature” (Mayr 1982). However, do two people look alike because they are twins or are they twins because they look alike? “Two organisms do not belong to the same species because they mate and reproduce, but they only are able to do so because they belong to the same species” (Mahner and Bunge 1997). Unfortunately, most biology (pre-university) teachers have no opinion on whether species are real or conceptual, simply because they have never been taught the question themselves, but rather one answer they still pass on to their students today, learned by heart without ever thinking about it. Species are either real or conceptual and, in my opinion, it is this “or” that we should teach about. Only then can we discuss those fundamental questions such as who or what is selected, who or what evolves and, finally, what is biodiversity and phylogenetics all about? Individuals related to each other by the tree of life. KW - biospecies KW - species as individuals KW - species as natural kinds KW - species concept KW - species problem Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-241052 SN - 2079-7737 VL - 10 IS - 6 ER - TY - JOUR A1 - Wolf, Markus A1 - Klug, Jörg A1 - Hackenberg, Reinhard A1 - Gessler, Manfred A1 - Grzeschik, Karl-Heinz A1 - Beato, Miguel A1 - Suske, Guntram T1 - Human CC10, the homologue of rabbit uteroglobin: genomic cloning, chromosomal localization and expression in endometrial cell lines N2 - No abstract available KW - Biochemie Y1 - 1992 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-59206 ER - TY - THES A1 - Wolf, Katarina T1 - Migration of tumor cells and leukocytes in extracellular matrix : proteolytic and nonproteolytic strategies for overcoming tissue barriers T1 - Migration von Tumorzellen und Leukozyten in extrazellulärer Matrix : proteolytische und nicht-proteolytische Strategien zur Überwindung von Gewebsbarrieren N2 - The extracellular matrix within connective tissues represents a structural scaffold as well as a barrier for motile cells, such as invading tumor cells or passenger leukocytes. It remains unclear how different cell types utilize matrix-degrading enzymes for proteolytic migration strategies and, on the other hand, non-proteolytic strategies to overcome 3D fibrillar matrix networks. To monitor cell migration, a 3D collagen model in vitro or the mouse dermis in vivo were used, in combination with time-lapse video-, confocal- or intravital multiphoton-microscopy, and computer-assisted cell tracking. Expression of proteases, including several MMPs, ADAMs, serine proteases and cathepsins, was shown by flow cytometry, Western blot, zymography, and RT-PCR. Protease activity by migrating HT-1080 fibrosarcoma cells resulting in collagenolysis in situ and generation of tube-like matrix defects was detected by three newly developed techniques:(i) quantitative FITC-release from FITC-labelled collagen, (ii) structural alteration of the pyhsical matrix structure (macroscopically and microscopically), and (iii) the visualization of focal in situ cleavage of individual collagen fibers. The results show that highly invasive ollagenolytic cells utilized a spindle-shaped "mesenchymal" migration strategy, which involved beta1 integrindependent interaction with fibers, coclustering of beta1 integrins and matrix metalloproteinases (MMPs) at fiber bundling sites, and the proteolytic generation of a tube-like matrix-defect by MMPs and additional proteases. In contrast to tumor cells, activated T cells migrated through the collagen fiber network by flexible "amoeboid" crawling including a roundish, elliptoid shape and morphological adaptation along collagen fibers, which was independent of collagenase function and fiber degradation. Abrogation of collagenolysis in tumor cells was achieved by a cocktail of broad-spectrum protease inhibitors at non-toxic conditions blocking collagenolysis by up to 95%. While in T cells protease inhibition induced neither morphodynamic changes nor reduced migration rates, in tumor cells a time-dependent conversion was obtained from proteolytic mesenchymal to non-proteolytic amoeboid migration in collagen lattices in vitro as well as the mouse dermis in vivo monitored by intravital microscopy. Tumor cells vigorously squeezed through matrix gaps and formed constriction rings in regions of narrow space, while the matrix structure remained intact. MMPs were excluded from fiber binding sites and beta1 integrin distribution was non-clustered linear. Besides for fibrosarcoma cells, this mesenchymal-toameboid transition (MAT) was confirmed for epithelial MDA-MB-231 breast carcinoma cells. In conclusion, cells of different origin exhibit significant diversity as well as plasticity of protease function in migration. In tumor cells, MAT could respresent a functionally important cellular and molecular escape pathway in tumor invasion and migration. N2 - Die extrazelluläre Matrix (EZM) des Bindegewebes stellt sowohl ein strukturelles Gerüst als auch eine Barriere für migrierende Zellen dar, wie z.B. invadierende Tumorzellen oder zirkulierende Leukozyten. Es ist bisher unklar, wie diese verschiedenen Zelltypen matrix-degradierende Enzyme für eine proteolytische Migrationsstrategie benutzen bzw. ob und wie sie ohne deren Hilfe durch das Gewebe gelangen. Um Zellmigration in EZM zu untersuchen, wurde ein dreidimensionales Kollagenmodell in vitro wie auch Maus-Dermis in vivo eingesetzt und Zellmigration mittels Zeitraffer-Video-, Konfokal- und Multiphoton-Mikroskopie sowie computer-gestützter Zelltracking-Analyse dargestellt. Expression von Proteasen verschiedener Klassen, wie der MMPs, ADAMs, Serinproteasen und Cathepsine, wurde mittels Durchfluss-Zytometrie, Western blot, Zymographie oder RT-PCR detektiert. Gegen Kollagen gerichtete zelluläre Protease-Aktivität wurde mit Hilfe drei neu entwickelter Techniken dargestellt: (i)quantitative Messung von löslichem FITC aus FITC-markiertem fibrillären Kollagen, (ii) mikro-und makroskopische Reorganisation der physikalischen Matrix-Struktur, und (iii) Visualisierung der Topologie fokaler Degradation von Matrixfasern. Die Ergebnisse zeigen, dass hochinvasive spindelförmige HT-1080 Fibrosarkomzellen eine sogenannte "mesenchymale" Migrationsstrategie mit folgenden Charakteristika entwickelten: (i) beta1 Integrin-abhängige Interaktion mit Kollagenfasern, (ii) das "Co-clustering" von beta1 Integrinen und Matrix-Metalloproteinasen an Faserzugstellen und (iii) eine röhrenförmige, durch Proteasen verursachte Matrixdefektbildung. Im Gegensatz zu proteolytischen Tumorzellen migrierten T-Zellen rundlich-elliptoid mittels flexibler Morphodynamik, ähnlich wie Amöben, durch das Kollagennetzwerk und orientierten sich entlang Kollagenfasern, wobei sie keine biochemisch und strukturell detektierbare Faserdegradation zeigten. Um Tumorzell-vermittelte Kollagenolyse zu hemmen, wurde ein Cocktail, bestehend aus Breitspektrum-Protease-Inhibitioren, etabliert, der die Kollagenolyse unter nicht-toxischen Bedingungen um bis zu 98% blockierte. Während in T-Zellen keine morphodynamischen Veränderungen detektiert wurden, entwickelten Tumorzellen eine Verschiebung von proteolytisch mesenchymaler zu unverminderter nicht-proteolytisch amöboider Migration (mesenchymale-amöboide Transition - MAT) aus, sowohl in Kollagenmatrices in vitro als auch in Maus-Dermis in vivo, dargestellt mittels Intravital-Multiphoton-Mikroskopie. Die Tumorzellen "quetschten" sich dabei durch Lücken in der Matrix und bildeten sogenannte Konstriktionsringe aus, während die Matrixstruktur intakt blieb. MMPs lokalisierten nicht mehr an Faser-Kontakstellen auf der Zelloberfläche, und beta1 Integrine lagen nicht mehr geclustert vor. Neben HT-1080 Fibrosarkomzellen wurde MAT auch für MDA-MB-231 Brustkrebszellen epithelialer Herkunft nach Protease-Blockade detektiert. Somit entwickeln migrierende Zellen verschiedener Herkunft eine signifikante Diversität wie auch Plastizität bei der Migration durch EZM aus, resultierend aus der Funktionalität von Matrix-Proteasen. In Tumorzellen könnte MAT einen funktionell wichtigen zellulären und molekularen Anpassungsmechanismus für die Tumorinvasion und -migration darstellen. KW - Zellmigration KW - Grundsubstanz KW - Tumorzelle KW - Leukozyt KW - Zellmigration KW - Invasion KW - Karzinomzellen KW - Leukozyten KW - Matrixproteasen KW - Kollagenasen KW - Proteaseinhibitoren KW - cell migration KW - invasion KW - carcinoma cells KW - leukozytes KW - matrix proteases KW - collagenases KW - protease inhibitors Y1 - 2002 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-5670 ER - TY - JOUR A1 - Wolf, Beat A1 - Kuonen, Pierre A1 - Dandekar, Thomas A1 - Atlan, David T1 - DNAseq workflow in a diagnostic context and an example of a user friendly implementation JF - BioMed Research International N2 - Over recent years next generation sequencing (NGS) technologies evolved from costly tools used by very few, to a much more accessible and economically viable technology. Through this recently gained popularity, its use-cases expanded from research environments into clinical settings. But the technical know-how and infrastructure required to analyze the data remain an obstacle for a wider adoption of this technology, especially in smaller laboratories. We present GensearchNGS, a commercial DNAseq software suite distributed by Phenosystems SA. The focus of GensearchNGS is the optimal usage of already existing infrastructure, while keeping its use simple. This is achieved through the integration of existing tools in a comprehensive software environment, as well as custom algorithms developed with the restrictions of limited infrastructures in mind. This includes the possibility to connect multiple computers to speed up computing intensive parts of the analysis such as sequence alignments. We present a typical DNAseq workflow for NGS data analysis and the approach GensearchNGS takes to implement it. The presented workflow goes from raw data quality control to the final variant report. This includes features such as gene panels and the integration of online databases, like Ensembl for annotations or Cafe Variome for variant sharing. KW - next generation sequencing KW - genome browser KW - mutation KW - algorithm KW - database KW - format KW - discovery KW - exome KW - variants KW - alignment Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-144527 IS - 403497 ER - TY - JOUR A1 - Wolf, Annette A1 - Akrap, Nina A1 - Marg, Berenice A1 - Galliardt, Helena A1 - Heiligentag, Martyna A1 - Humpert, Fabian A1 - Sauer, Markus A1 - Kaltschmidt, Barbara A1 - Kaltschmidt, Christian A1 - Seidel, Thorsten T1 - Elements of Transcriptional Machinery Are Compatible among Plants and Mammals JF - PLoS ONE N2 - In the present work, the objective has been to analyse the compatibility of plant and human transcriptional machinery. The experiments revealed that nuclear import and export are conserved among plants and mammals. Further it has been shown that transactivation of a human promoter occurs by human transcription factor NF-\(\kappa\) B in plant cells, demonstrating that the transcriptional machinery is highly conserved in both kingdoms. Functionality was also seen for regulatory elements of NF-\(\kappa\) B such as its inhibitor I\(\kappa\)B isoform \(\alpha\) that negatively regulated the transactivation activity of the p50/RelA heterodimer by interaction with NF-\(\kappa\)B in plant cells. Nuclear export of RelA could be demonstrated by FRAP-measurements so that RelA shows nucleo-cytoplasmic shuttling as reported for RelA in mammalian cells. The data reveals the high level of compatibility of human transcriptional elements with the plant transcriptional machinery. Thus, Arabidopsis thaliana mesophyll protoplasts might provide a new heterologous expression system for the investigation of the human NF-\(\kappa\)B signaling pathways. The system successfully enabled the controlled manipulation of NF-\(\kappa\)B activity. We suggest the plant protoplast system as a tool for reconstitution and analyses of mammalian pathways and for direct observation of responses to e. g. pharmaceuticals. The major advantage of the system is the absence of interference with endogenous factors that affect and crosstalk with the pathway. KW - complexes KW - in vivo KW - DNA-binding KW - nuclear proe KW - gene expression KW - NF-KAPPA-B KW - RNA-binding protein KW - alpha KW - inflammation KW - homodimers Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-131203 VL - 8 IS - 1 ER - TY - JOUR A1 - Wohlwend, Michael R. A1 - Craven, Dylan A1 - Weigelt, Patrick A1 - Seebens, Hanno A1 - Winter, Marten A1 - Kreft, Holger A1 - Zurell, Damaris A1 - Sarmento Cabral, Juliano A1 - Essl, Franz A1 - van Kleunen, Mark A1 - Pergl, Jan A1 - Pyšek, Petr A1 - Knight, Tiffany M. T1 - Anthropogenic and environmental drivers shape diversity of naturalized plants across the Pacific JF - Diversity and Distributions N2 - Aim The Pacific exhibits an exceptional number of naturalized plant species, but the drivers of this high diversity and the associated compositional patterns remain largely unknown. Here, we aim to (a) improve our understanding of introduction and establishment processes and (b) evaluate whether this information is sufficient to create scientific conservation tools, such as watchlists. Location Islands in the Pacific Ocean, excluding larger islands such as New Zealand, Japan, the Philippines and Indonesia. Methods We combined information from the most up‐to‐date data sources to quantify naturalized plant species richness and turnover across island groups and investigate the effects of anthropogenic, biogeographic and climate drivers on these patterns. In total, we found 2,672 naturalized plant species across 481 islands and 50 island groups, with a total of 11,074 records. Results Most naturalized species were restricted to few island groups, and most island groups have a low number of naturalized species. Island groups with few naturalized species were characterized by a set of widespread naturalized species. Several plant families that contributed many naturalized species globally also did so in the Pacific, particularly Fabaceae and Poaceae. However, many families were significantly over‐ or under‐represented in the Pacific naturalized flora compared to other regions of the world. Naturalized species richness increased primarily with increased human activity and island altitude/area, whereas similarity between island groups in temperature along with richness differences was most important for beta diversity. Main conclusions The distribution and richness of naturalized species can be explained by a small set of drivers. The Pacific region contains many naturalized plant species also naturalized in other regions in the world, but our results highlight key differences such as a stronger role of anthropogenic drivers in shaping diversity patterns. Our results establish a basis for predicting and preventing future naturalizations in a threatened biodiversity hotspot. KW - anthropogenic drivers KW - beta diversity KW - island biogeography KW - naturalized species KW - Pacific Ocean KW - plant invasion Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-239925 VL - 27 IS - 6 SP - 1120 EP - 1133 ER - TY - JOUR A1 - Wittbrodt, Joachim A1 - Lammers, Reiner A1 - Malitschek, Barbara A1 - Ullrich, Axel A1 - Schartl, Manfred T1 - Xmrk receptor tyrosine kinase is activated in Xiphophorus malignant melanoma N2 - Xmrk encodes a putative transmembrane glycoprotein of the tyrosine kinase family and is a melanoma-inducing gene in Xiphophorus. We attempted to investigate the biological function of the putative Xmrk receptor by characterizing its signalling properties. Since a potential Iigand for Xmrk has not yet been identified, it has been difficult to analyse the biochemical properlies and biological function of this cell surface protein. In an approach towards such analyses, the Xmrk extracellular domain was replaced by the closely related Iigand-binding domain sequences of the human epidennal growth factor receptor (HER) and the ligand-induced activity of the chimeric HER-Xmrk proteinwas examined. We show that the Xmrk protein is a functional receptor tyrosine kinase, is highly active in malignant melanoma and displays a constitutive autophosphorylation activity possibly due to an activating mutation in its extracellular or transmembrane domain. In the focus formation assay the HER-Xmrk chimera is a potent transfonning protein equivalent to other tyrosine kinase oncoproteins. KW - Physiologische Chemie KW - chimeric RTKs KW - melanoma KW - RTK KW - Xiphophorus Y1 - 1992 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-61699 ER - TY - JOUR A1 - Wittbrodt, J. A1 - Adam, D. A1 - Malitschek, B. A1 - Maueler, W. A1 - Raulf, F. A1 - Telling, A. A1 - Robertson, M. A1 - Schartl, Manfred T1 - Novel putative receptor tyrosine kinase encoded by the melanoma-inducing Tu locus in Xiphophorus N2 - No abstract available KW - Physiologische Chemie Y1 - 1989 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-61800 ER - TY - JOUR A1 - Wirth, Christine C. A1 - Glushakova, Svetlana A1 - Scheuermayer, Matthias A1 - Repnik, Urska A1 - Garg, Swatl A1 - Schaack, Dominik A1 - Kachman, Marika M. A1 - Weißbach, Tim A1 - Zimmerberg, Joshua A1 - Dandekar, Thomas A1 - Griffiths, Gareth A1 - Chitnis, Chetan E. A1 - Singh, Shallja A1 - Fischer, Rainer A1 - Pradel, Gabriele T1 - Perforin-like protein PPLP2 permeabilizes the red blood cell membrane during egress of Plasmodium falciparum gametocytes JF - Cellular Microbiology N2 - Egress of malaria parasites from the host cell requires the concerted rupture of its enveloping membranes. Hence, we investigated the role of the plasmodial perforin-like protein PPLP2 in the egress of Plasmodium falciparum from erythrocytes. PPLP2 is expressed in blood stage schizonts and mature gametocytes. The protein localizes in vesicular structures, which in activated gametocytes discharge PPLP2 in a calcium-dependent manner. PPLP2 comprises a MACPF domain and recombinant PPLP2 has haemolytic activities towards erythrocytes. PPLP2-deficient [PPLP2(−)] merozoites show normal egress dynamics during the erythrocytic replication cycle, but activated PPLP2(−) gametocytes were unable to leave erythrocytes and stayed trapped within these cells. While the parasitophorous vacuole membrane ruptured normally, the activated PPLP2(−) gametocytes were unable to permeabilize the erythrocyte membrane and to release the erythrocyte cytoplasm. In consequence, transmission of PPLP2(−) parasites to the Anopheles vector was reduced. Pore-forming equinatoxin II rescued both PPLP2(−) gametocyte exflagellation and parasite transmission. The pore sealant Tetronic 90R4, on the other hand, caused trapping of activated wild-type gametocytes within the enveloping erythrocytes, thus mimicking the PPLP2(−) loss-of-function phenotype. We propose that the haemolytic activity of PPLP2 is essential for gametocyte egress due to permeabilization of the erythrocyte membrane and depletion of the erythrocyte cytoplasm. Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-120895 VL - 16 IS - 5 ER - TY - JOUR A1 - Winkler, Christoph A1 - Wittbrodt, Joachim A1 - Lammers, Reiner A1 - Ullrich, Axel A1 - Schartl, Manfred T1 - Ligand-dependent tumor induction in medakafish embryos by a Xmrk receptor tyrosine kinase transgene N2 - Xmrk encodes a subclass 1 receptor tyrosine kinase (RTK) which has been cloned from the melanomainducing locus Tu of the poeciliid fish Xiphophorus. To demonstrate a high oncogenic potential in vivo we transferred the gene into early embryos of the closely related medakafish. Ectopic expression of the Xmrk oncogene under the control of a strong, constitutive promoter (CMVTk) led to the induction of embryonic tumors with high incidence, after short latency periods, and with a specific pattern of affected tissues. We demonstrate ligand-dependent transformation in vivo using a chimeric receptor consisting of the extracellular and transmembrane domains of the human EGF receptor (HER) and the cytoplasmatic domain of Xmrk. Expression of the chimeric receptor alone does not lead to ldnase activation or induction of tumors. Coexpression of the chimera with its corresponding ligand, human transforming growth factor alpha (bTGF(X), however, results in the activation of the chimeric RTK. In injected fish embryos the induction of the neoplastic growth is observed with similar incidence and tissue distribution as in embryos carrying the native Xmrk oncogene suggesting that the ligand as well as factors downstream of tbe RTK are required for tumor formation. In this study we show single-step induction of tumors by ectopic expression of RTKs in vivo substantiating tbe significance of autocrine stimulation in RTK induced tumors in vertebrales. KW - Japankärpfling KW - Ligand KW - Tumor Y1 - 1994 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-87107 ER - TY - JOUR A1 - Winkler, Christoph A1 - Vielkind, Jürgen R. A1 - Schartl, Manfred T1 - Transient expression of foreign DNA during embryonic and larval development of the medaka fish (Oryzias latipes) N2 - Species of small fish are becoming useful tools for studies on vertebrate development. Wehave investigated the developing embryo of the Japanese medaka for its application as a transient expression system for the in vivo analysis of gene regulation and function. The temporaland spatial expression patterns ofbacterial chloramphenicol acetyltransferase and galactosidase reporter genes injected in supercoiled plasmid form into the cytoplasm of one cell of the two-cell stage embryo was promoter-specific. The transient expression was found to be mosaic within the tissue and organs reflecting the unequal distribution of extrachromosomal foreign DNA and the intensive cell mixing movements that occur in fish embryogenesis. The expression data are consistent with data on DNA fate. Foreign DNA persisted during embryogenesis and was still detectable in some 3- and 9-month-old adult fish; it was found in high molecular weight form as weil as in circular plasmid conformations. The DNA was replicated during early and late embryogenesis. Our data indicate that the developing medaka embryo is a powerful in vivo assay system for studies of gene regulation and function. KW - Physiologische Chemie KW - Medaka - Genetransfer - Transient expression - DNA fate - Fish developmental biology Y1 - 1991 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-61743 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 - THES A1 - Winkler, Ann-Cathrin Nicole T1 - Identification of human host cell factors involved in \(Staphylococcus\) \(aureus\) 6850 infection T1 - Identifizierung von humanen Wirtszellfaktoren die eine Rolle bei der \(Staphylococcus\) \(aureus\) Infektion spielen N2 - Staphylococcus aureus is both a human commensal and a pathogen. 20%-30% of all individuals are permanently or occasionally carriers of S. aureus without any symptoms. In contrast to this, S. aureus can cause life-threatening diseases e.g. endocarditis, osteomyelitis or sepsis. Here, the increase in antibiotic resistances makes it more and more difficult to treat these infections and hence the number of fatalities rises constantly. Since the pharmaceutical industry has no fundamentally new antibiotics in their pipeline, it is essential to better understand the interplay between S. aureus and the human host cell in order to find new, innovative treatment options. In this study, a RNA interference based whole genome pool screen was performed to identify human proteins, which play a role during S. aureus infections. Since 1,600 invasion and 2,271 cell death linked factors were enriched at least 2 fold, the big challenge was to filter out the important ones. Here, a STRING pathway analysis proved to be the best option. Subsequently, the identified hits were validated with the help of inhibitors and a second, individualised small interfering RNA-based screen. In the course of this work two important steps were identified, that are critical for host cell death: the first is bacterial invasion, the second phagosomal escape. The second step is obligatory for intracellular bacterial replication and subsequent host cell death. Invasion in turn is determining for all following events. Accordingly, the effect of the identified factors towards these two crucial steps was determined. Under screening conditions, escape was indirectly measured via intracellular replication. Three inhibitors (JNKII, Methyl-beta-cyclodeytrin, 9-Phenantrol) could be identified for the invasion process. In addition, siRNAs targeted against 16 different genes (including CAPN2, CAPN4 and PIK3CG), could significantly reduce bacterial invasion. Seven siRNAs (FPR2, CAPN4, JUN, LYN, HRAS, AKT1, ITGAM) were able to inhibit intracellular replication significantly. Further studies showed that the IP3 receptor inhibitor 2-APB, the calpain inhibitor calpeptin and the proteasome inhibitor MG-132 are able to prevent phagosomal escape and as a consequence intracellular replication and host cell death. In this context the role of calpains, calcium, the proteasome and the mitochondrial membrane potential was further investigated in cell culture. Here, an antagonistic behaviour of calpain 1 and 2 during bacterial invasion was observed. Intracellular calcium signalling plays a major role, since its inhibition protects host cells from death. Beside this, the loss of mitochondrial membrane potential is characteristic for S. aureus infection but not responsible for host cell death. The reduction of membrane potential can be significantly diminished by the inhibition of the mitochondrial Na+/Ca2+ exchanger. All together, this work shows that human host cells massively contribute to different steps in S. aureus infection rather than being simply killed by bacterial pore-forming toxins. Various individual host cell factors were identified, which contribute either to invasion or to phagosomal escape and therefore to S. aureus induced cytotoxicity. Finally, several inhibitors of S. aureus infection were identified. One of them, 2-APB, was already tested in a sepsis mouse model and reduced bacterial load of kidneys. Thus, this study shows valuable evidence for novel treatment options against S. aureus infections, based on the manipulation of host cell signalling cascades. N2 - Staphylococcus aureus kann sowohl ein Bestandteil der natürlichen Hautflora als auch ein Krankheitserreger sein. 20%-30% aller Menschen werden, permanent oder zeitweise, von S. aureus besiedelt, ohne Krankheitssymptome aufzuweisen. Im Gegensatz dazu kann S. aureus lebensbedrohliche Krankheiten wie Endokarditis, Osteomyelitis oder Sepsis verursachen. Diese Infektionen können immer schlechter behandelt werden, da immer mehr Stämme Resistenzen gegen die vorhandenen Antibiotika aufweisen. Dies führt zu einer steigenden Anzahl an Todesfällen, die auf Staphylokokkeninfektionen zurückzuführen sind. Da die Pharmaindustrie keine grundlegend neuen Antibiotika kurz vor der Marktreife hat, ist ein besseres Verständnis für das Wechselspiel zwischen Staphylokokken und ihren menschlichen Wirtszellen unbedingt notwendig, um neue, innovative Behandlungsmöglichkeiten finden zu können. Dafür wurde in dieser Arbeit ein genomweiter RNA-interferenz basierter Screen durchgeführt. Es sollten so die Proteine identifiziert werden, die eine Rolle bei der Staphylokokkeninfektion spielen. Da 1.600 invasionsrelevante und 2.271 zelltodrelevante Faktoren mindestens 2-fach angereichert waren, musste ein Weg gefunden werden die wichtigen Faktoren herauszufiltern. Eine STRING-Pathwayanalyse stellte sich als die beste Methode hierfür heraus. In einem zweiten Schritt wurden die so identifizierten Faktoren mit Inhibitoren oder einzelnen siRNAs ein weiteres Mal herunterreguliert, um ihre tatsächlichen Auswirkungen auf den Infektionsverlauf zu untersuchen. Im Verlauf dieser Arbeit konnte gezeigt werden, dass dem S. aureus induzierten Wirtszelltod mindestens zwei wichtige Schritte vorausgehen müssen. Erstens die Invasion der Wirtszelle und zweitens der Ausbruch aus dem Phagosom. Nur so können sich im dritten Schritt die Bakterien intrazellulär vermehren und die Zelle töten. Daher wurde der Einfluss der identifizierten Faktoren auf diese beiden entscheidenden Prozesse untersucht. Der Ausbruch wurde unter Screenkonditionen indirekt über die intrazelluläre Vermehrung bestimmt. Es konnten drei Inhibitoren (JNKII, Methyl-beta-cyclodeytrin, 9-Phenantrol) identifiziert werden, die die bakterielle Invasion vermindern. Darüber hinaus wurden 16 Proteine (unter anderem CAPN2, CAPN4 und PIK3CG) gefunden, deren Herunterregulation durch siRNAs, eine signifikant reduzierte Invasion zur Folge hatten. Sieben siRNAs (FPR2, CAPN4, JUN, LYN, HRAS, AKT1, ITGAM) waren in der Lage die intrazelluläre Vermehrung signifikant zu verringern. In nachfolgenden Versuchen konnte gezeigt werden, dass der IP3-Rezeptorinhibitor 2-APB, der Calpaininhibitor Calpeptin und der Proteasominhibitor MG-132 den Ausbruch aus dem Phagosom, sowie die darauffolgenden Ereignisse (intrazelluläre Vermehrung und Wirtszelltod) inhibieren können. In diesem Zusammenhang wurden die Einflüsse von Calpainen, Calcium, dem Proteasom sowie dem mitochondrialen Membranpotentialverlust im Zellkulturmodell im Detail weiter untersucht. So konnte eine gegensätzliche Rolle von Calpain 1 und 2 bei der S. aureus Invasion festgestellt werden. Die intrazelluläre calciumabhängige Signalweiterleitung spielt eine bedeutende Rolle bei der S. aureus Infektion, da ihre Inhibition eine normale Infektion verhindert. Das mitochondriale Membranpotential (MMP) sinkt während einer S. aureus infektion, ist aber nicht für den Zelltod verantwortlich. Das Sinken des MMPs kann mit einem Inhibitor, der den mitochondrialen Na+/Ca2+ Austausch verhindert, signifikant reduziert werden. Zusammenfassend zeigt diese Arbeit, dass die menschliche Wirtszelle selbst relevant zu den verschiedenen Schritten der Staphylokokkeninfektion beiträgt, und nicht einfach, wie häufig angenommen, von porenbildenden bakteriellen Toxinen zerstört wird. Entsprechend konnten einzelne Wirtszellproteine identifiziert werden, die entweder zur bakteriellen Invasion oder zum phagosomalen Ausbruch und somit zum induzierten Wirtszelltod beitragen. Überdies konnte gezeigt werden, dass Inhibitoren, die diese Wirtszellproteine hemmen, die Wirtszellen zu unterschiedlichen Zeitpunkten vor einer S. aureus Infektion schützen können. Folglich liefert diese Arbeit wertvolle Hinweise für neue Behandlungsmöglichkeiten von S. aureus Infektionen, die auf der Manipulation von Wirtszellsignalkaskaden beruhen. KW - Staphylococcus aureus KW - Wirtszelle KW - RNS-Interferenz KW - Host cell death KW - RNAi KW - 2-APB KW - intracellular replication KW - calpain KW - Human Host KW - Inhibitor Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-114300 ER - TY - JOUR A1 - Williams, Richard D. A1 - Chagtai, Tasnim A1 - Alcaide-German, Marisa A1 - Apps, John A1 - Wegert, Jenny A1 - Popov, Sergey A1 - Vujanic, Gordan A1 - Van Tinteren, Harm A1 - Van den Heuvel-Eibrink, Marry M A1 - Kool, Marcel A1 - De Kraker, Jan A1 - Gisselsson, David A1 - Graf, Norbert A1 - Gessler, Manfred A1 - Pritchard-Jones, Kathy T1 - Multiple mechanisms of MYCN dysregulation in Wilms tumour JF - Oncotarget N2 - Genomic gain of the proto-oncogene transcription factor gene MYCN is associated with poor prognosis in several childhood cancers. Here we present a comprehensive copy number analysis of MYCN in Wilms tumour (WT), demonstrating that gain of this gene is associated with anaplasia and with poorer relapse-free and overall survival, independent of histology. Using whole exome and gene-specific sequencing, together with methylation and expression profiling, we show that MYCN is targeted by other mechanisms, including a recurrent somatic mutation, P44L, and specific DNA hypomethylation events associated with MYCN overexpression in tumours with high risk histologies. We describe parallel evolution of genomic copy number gain and point mutation of MYCN in the contralateral tumours of a remarkable bilateral case in which independent contralateral mutations of TP53 also evolve over time. We report a second bilateral case in which MYCN gain is a germline aberration. Our results suggest a significant role for MYCN dysregulation in the molecular biology of Wilms tumour. We conclude that MYCN gain is prognostically significant, and suggest that the novel P44L somatic variant is likely to be an activating mutation. KW - integrative genomics viewer KW - oncogene amplification KW - sequencing data KW - gene KW - gain KW - copy number KW - somatic mutations KW - beta-catenin KW - histology KW - reveals KW - Wilms tumour KW - MYCN KW - DNA methylation KW - prognostic marker Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-143471 VL - 6 IS - 9 ER - TY - JOUR A1 - Wilken, Norbert A1 - Kossner, Ursula A1 - Senécal, Jean-Luc A1 - Scheer, Ulrich A1 - Dabauvalle, Marie-Christine T1 - Nup180, a novel nuclear pore complex protein localizing to the cytoplasmic ring and associated fibrils N2 - No abstract available Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-32049 ER - TY - THES A1 - Wietek, Irina T1 - Human Interleukin-4 binding protein epitope involved in high-affinity binding of interleukin-4 N2 - No abstract available KW - Mensch KW - Interleukin 4 KW - Bindeproteine KW - Molekularbiologie Y1 - 2001 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-3190 ER - TY - THES A1 - Wiese, Katrin Evelyn T1 - Sensing supraphysiological levels of MYC : mechanisms of MIZ1-dependent MYC-induced Apoptosis in Mammary Epithelial Cells T1 - Mechanismen der MIZ1-abhängigen MYC-induzierten Apoptose in Brustepithelzellen N2 - Deregulated MYC expression contributes to cellular transformation as well as progression and maintenance of human tumours. Interestingly, in the absence of additional genetic alterations, potentially oncogenic levels of MYC sensitise cells to a variety of apoptotic stimuli. Hence, MYC-induced apoptosis has long been recognised as a major barrier against cancer development. However, it is largely unknown how cells discriminate physiological from supraphysiological levels of MYC in order to execute an appropriate biological response. The experiments described in this thesis demonstrate that induction of apoptosis in mammary epithelial cells depends on the repressive actions of MYC/MIZ1 complexes. Analysis of gene expression profiles and ChIP-sequencing experiments reveals that high levels of MYC are required to invade low-affinity binding sites and repress target genes of the serum response factor SRF. These genes are involved in cytoskeletal dynamics as well as cell adhesion processes and are likely needed to transmit survival signals to the AKT kinase. Restoration of SRF activity rescues MIZ1- dependent gene repression and increases AKT phosphorylation and downstream function. Collectively, these results indicate that association with MIZ1 leads to an expansion of MYC’s transcriptional response that allows sensing of oncogenic levels, which points towards a tumour-suppressive role for the MYC/MIZ1 complex in epithelial cells. N2 - Eine Deregulation der MYC Expression trägt entscheidend zur malignen Transformation und Progression humaner Tumoren bei. In Abwesenheit von zusätzlichen genetischen Läsionen machen potentiell onkogene MYC Proteinmengen Zellen jedoch anfällig für eine Reihe Apoptoseauslösender Reize. Daher kann MYC-induzierte Apoptose als bedeutende tumorsuppressive Maßnahme und wichtige Barriere gegen die Entstehung von Krebs betrachtet werden. Mechanistisch unklar ist allerdings wie genau Zellen physiologische von supraphysiologischen MYC-Mengen unterscheiden um adäquat darauf reagieren zu können. Die Experimente in dieser Dissertation zeigen, dass die repressive Eigenschaft von MYC/MIZ1 Komplexen für die Induktion von Apoptose in Brustepithelzellen essentiell ist. Die Analyse von Genexpressions- und ChIP-Sequenzier-Experimenten verdeutlicht, dass hohe Level an MYC benötigt werden um niedrig-affine Bindestellen im Genom zu besetzen und Zielgene des SRF (serum response factor ) Transkriptionsfaktors zu reprimieren. Diese Gene haben eine wichtige Funktion in Prozessen wie Zytoskelettdynamik und Zelladhäsion und sind vermutlich daran beteiligt notwendige Überlebenssignale an die Kinase AKT weiterzuleiten. Eine Wiederherstellung der SRF Aktivität revertiert die MIZ1-abhängige Repression der Zielgene und führt zu einer vermehrten AKT Phosphorylierung und Funktion. Insgesamt deuten diese Resultate auf eine tumorsuppressive Rolle des MYC/MIZ1 Komplexes in epithelialen Zellen hin, da eine Veränderung der genregulatorischen Aktivität als Folge der Assoziation mit MIZ1 dazu beiträgen könnte onkogene Mengen an MYC zu erkennen. KW - Myc KW - Apoptosis KW - Myc KW - Miz1 KW - Apoptose KW - Repression KW - ChIP-sequencing KW - Repression Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-132532 ER - TY - JOUR A1 - Wiegering, Armin A1 - Pfann, Christina A1 - Uthe, Friedrich Wilhelm A1 - Otto, Christoph A1 - Rycak, Lukas A1 - Mäder, Uwe A1 - Gasser, Martin A1 - Waaga-Gasser, Anna-Maria A1 - Eilers, Martin A1 - Germer, Christoph-Thomas T1 - CIP2A Influences Survival in Colon Cancer and Is Critical for Maintaining Myc Expression JF - PLoS ONE N2 - The cancerous inhibitor of protein phosphatase 2A (CIP2A) is an oncogenic factor that stabilises the c-Myc protein. CIP2A is overexpressed in several tumours, and expression levels are an independent marker for long-term outcome. To determine whether CIP2A expression is elevated in colon cancer and whether it might serve as a prognostic marker for survival, we analysed CIP2A mRNA expression by real-time PCR in 104 colon cancer samples. CIP2A mRNA was overexpressed in colon cancer samples and CIP2A expression levels correlated significantly with tumour stage. We found that CIP2A serves as an independent prognostic marker for disease-free and overall survival. Further, we investigated CIP2A-dependent effects on levels of c-Myc, Akt and on cell proliferation in three colon cancer cell lines by silencing CIP2A using small interfering (si) and short hairpin (sh) RNAs. Depletion of CIP2A substantially inhibited growth of colon cell lines and reduced c-Myc levels without affecting expression or function of the upstream regulatory kinase, Akt. Expression of CIP2A was found to be dependent on MAPK activity, linking elevated c-Myc expression to deregulated signal transduction in colon cancer. KW - caco-2 cells KW - carcinomas KW - colon KW - colorectal cancer KW - MAPK signaling cascades KW - metastasis KW - protein expression KW - small interferring RNA Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-97252 ER - TY - JOUR A1 - Wiegering, Armin A1 - Matthes, Niels A1 - Mühling, Bettina A1 - Koospal, Monika A1 - Quenzer, Anne A1 - Peter, Stephanie A1 - Germer, Christoph-Thomas A1 - Linnebacher, Michael A1 - Otto, Christoph T1 - Reactivating p53 and Inducing Tumor Apoptosis (RITA) Enhances the Response of RITA-Sensitive Colorectal Cancer Cells to Chemotherapeutic Agents 5-Fluorouracil and Oxaliplatin JF - Neoplasia N2 - Colorectal carcinoma (CRC) is the most common cancer of the gastrointestinal tract with frequently dysregulated intracellular signaling pathways, including p53 signaling. The mainstay of chemotherapy treatment of CRC is 5-fluorouracil (5FU) and oxaliplatin. The two anticancer drugs mediate their therapeutic effect via DNA damage-triggered signaling. The small molecule reactivating p53 and inducing tumor apoptosis (RITA) is described as an activator of wild-type and reactivator of mutant p53 function, resulting in elevated levels of p53 protein, cell growth arrest, and cell death. Additionally, it has been shown that RITA can induce DNA damage signaling. It is expected that the therapeutic benefits of 5FU and oxaliplatin can be increased by enhancing DNA damage signaling pathways. Therefore, we highlighted the antiproliferative response of RITA alone and in combination with 5FU or oxaliplatin in human CRC cells. A panel of long-term established CRC cell lines (n = 9) including p53 wild-type, p53 mutant, and p53 null and primary patient-derived, low-passage cell lines (n = 5) with different p53 protein status were used for this study. A substantial number of CRC cells with pronounced sensitivity to RITA (IC\(_{50}\)< 3.0 μmol/l) were identified within established (4/9) and primary patient-derived (2/5) CRC cell lines harboring wild-type or mutant p53 protein. Sensitivity to RITA appeared independent of p53 status and was associated with an increase in antiproliferative response to 5FU and oxaliplatin, a transcriptional increase of p53 targets p21 and NOXA, and a decrease in MYC mRNA. The effect of RITA as an inducer of DNA damage was shown by a strong elevation of phosphorylated histone variant H2A.X, which was restricted to RITA-sensitive cells. Our data underline the primary effect of RITA, inducing DNA damage, and demonstrate the differential antiproliferative effect of RITA to CRC cells independent of p53 protein status. We found a substantial number of RITA-sensitive CRC cells within both panels of established CRC cell lines and primary patient-derived CRC cell lines (6/14) that provide a rationale for combining RITA with 5FU or oxaliplatin to enhance the antiproliferative response to both chemotherapeutic agents. KW - colorectal carcinoma KW - reactivating p53 and inducing tumor apoptosis (RITA) KW - chemotherapy KW - 5-fluorouracil KW - oxaliplatin Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-171067 VL - 19 IS - 4 ER - TY - JOUR A1 - Wiegering, Armin A1 - Korb, Doreen A1 - Thalheimer, Andreas A1 - Kämmerer, Ulrike A1 - Allmanritter, Jan A1 - Matthes, Niels A1 - Linnebacher, Michael A1 - Schlegel, Nicolas A1 - Klein, Ingo A1 - Ergün, Süleyman A1 - Germer, Christoph-Thomas A1 - Otto, Christoph T1 - E7080 (Lenvatinib), a Multi-Targeted Tyrosine Kinase Inhibitor, Demonstrates Antitumor Activities Against Colorectal Cancer Xenografts N2 - Clinical prognosis of metastasized colorectal carcinoma (CRC) is still not at desired levels and novel drugs are needed. Here, we focused on the multi-tyrosine kinase inhibitor E7080 (Lenvatinib) and assessed its therapeutic efficacy against human CRC cell lines in vitro and human CRC xenografts in vivo. The effect of E7080 on cell viability was examined on 10 humanCRCcell lines and humanendothelial cells (HUVEC). The inhibitory effect of E7080 on VEGF-induced angiogenesis was studied in an ex vivo mouse aortic ring angiogenesis assay. In addition, the efficacy of E7080 against xenografts derived fromCRC cell lines and CRC patient resection specimenswithmutated KRASwas investigated in vivo. Arelatively low cytotoxic effect of E7080 on CRC cell viabilitywas observed in vitro. Endothelial cells (HUVEC)weremore susceptible to the incubation with E7080. This is in line with the observation that E7080 demonstrated an anti-angiogenic effect in a three-dimensional ex vivo mouse aortic ring angiogenesis assay. E7080 effectively disrupted CRC cell-mediated VEGF-stimulated growth of HUVEC in vitro. Daily in vivo treatment with E7080 (5 mg/kg) significantly delayed the growth of KRAS mutated CRC xenografts with decreased density of tumor-associated vessel formations and without tumor regression. This observation is in line with results that E7080 did not significantly reduce the number of Ki67-positive cells in CRC xenografts. The results suggest antiangiogenic activity of E7080 at a dosage thatwas well tolerated by nudemice. E7080 may provide therapeutic benefits in the treatment of CRC with mutated KRAS. KW - Chirurgie Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-111165 ER - TY - JOUR A1 - Wiegering, Armin A1 - Isbert, Christoph A1 - Dietz, Ulrich A. A1 - Kunzmann, Volker A1 - Ackermann, Sabine A1 - Kerscher, Alexander A1 - Maeder, Uwe A1 - Flentje, Michael A1 - Schlegel, Nicolas A1 - Reibetanz, Joachim A1 - Germer, Christoph-Thomas A1 - Klein, Ingo T1 - Multimodal therapy in treatment of rectal cancer is associated with improved survival and reduced local recurrence - a retrospective analysis over two decades N2 - Background The management of rectal cancer (RC) has substantially changed over the last decades with the implementation of neoadjuvant chemoradiotherapy, adjuvant therapy and improved surgery such as total mesorectal excision (TME). It remains unclear in which way these approaches overall influenced the rate of local recurrence and overall survival. Methods Clinical, histological and survival data of 658 out of 662 consecutive patients with RC were analyzed for treatment and prognostic factors from a prospectively expanded single-institutional database. Findings were then stratified according to time of diagnosis in patient groups treated between 1993 and 2001 and 2002 and 2010. Results The study population included 658 consecutive patients with rectal cancer between 1993 and 2010. Follow up data was available for 99.6% of all 662 treated patients. During the time period between 2002 and 2010 significantly more patients underwent neoadjuvant chemoradiotherapy (17.6% vs. 60%) and adjuvant chemotherapy (37.9% vs. 58.4%). Also, the rate of reported TME during surgery increased. The rate of local or distant metastasis decreased over time, and tumor related 5-year survival increased significantly with from 60% to 79%. Conclusion In our study population, the implementation of treatment changes over the last decade improved the patient’s outcome significantly. Improvements were most evident for UICC stage III rectal cancer. KW - Rectal cancer KW - Improved survival KW - TME Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-110606 ER - TY - JOUR A1 - Widmann, Annekathrin A1 - Artinger, Marc A1 - Biesinger, Lukas A1 - Boepple, Kathrin A1 - Peters, Christina A1 - Schlechter, Jana A1 - Selcho, Mareike A1 - Thum, Andreas S. T1 - Genetic Dissection of Aversive Associative Olfactory Learning and Memory in Drosophila Larvae JF - PLoS Genetics N2 - Memory formation is a highly complex and dynamic process. It consists of different phases, which depend on various neuronal and molecular mechanisms. In adult Drosophila it was shown that memory formation after aversive Pavlovian conditioning includes—besides other forms—a labile short-term component that consolidates within hours to a longer-lasting memory. Accordingly, memory formation requires the timely controlled action of different neuronal circuits, neurotransmitters, neuromodulators and molecules that were initially identified by classical forward genetic approaches. Compared to adult Drosophila, memory formation was only sporadically analyzed at its larval stage. Here we deconstruct the larval mnemonic organization after aversive olfactory conditioning. We show that after odor-high salt conditioning larvae form two parallel memory phases; a short lasting component that depends on cyclic adenosine 3’5’-monophosphate (cAMP) signaling and synapsin gene function. In addition, we show for the first time for Drosophila larvae an anesthesia resistant component, which relies on radish and bruchpilot gene function, protein kinase C activity, requires presynaptic output of mushroom body Kenyon cells and dopamine function. Given the numerical simplicity of the larval nervous system this work offers a unique prospect for studying memory formation of defined specifications, at full-brain scope with single-cell, and single-synapse resolution. KW - genetic dissection KW - Drosophila KW - memory formation Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-166672 VL - 12 IS - 10 ER - TY - JOUR A1 - Widder, Anna A1 - Kelm, Matthias A1 - Reibetanz, Joachim A1 - Wiegering, Armin A1 - Matthes, Niels A1 - Germer, Christoph-Thomas A1 - Seyfried, Florian A1 - Flemming, Sven T1 - Robotic-assisted versus laparoscopic left hemicolectomy — postoperative inflammation status, short-term outcome and cost effectiveness JF - International Journal of Environmental Research and Public Health N2 - Robotic-assisted colon surgery may contain advantages over the laparoscopic approach, but clear evidence is sparse. This study aimed to analyze postoperative inflammation status, short-term outcome and cost-effectiveness of robotic-assisted versus laparoscopic left hemicolectomy. All consecutive patients who received minimal-invasive left hemicolectomy at the Department of Surgery I at the University Hospital of Wuerzburg in 2021 were prospectively included. Importantly, no patient selection for either procedure was carried out. The robotic-assisted versus laparoscopic approaches were compared head to head for postoperative short-term outcomes as well as cost-effectiveness. A total of 61 patients were included, with 26 patients having received a robotic-assisted approach. Baseline characteristics did not differ among the groups. Patients receiving a robotic-assisted approach had a significantly decreased length of hospital stay as well as lower rates of complications in comparison to patients who received laparoscopic surgery (n = 35). In addition, C-reactive protein as a marker of systemic stress response was significantly reduced postoperatively in patients who were operated on in a robotic-assisted manner. Consequently, robotic-assisted surgery could be performed in a cost-effective manner. Thus, robotic-assisted left hemicolectomy represents a safe and cost-effective procedure and might improve patient outcomes in comparison to laparoscopic surgery. KW - robotic surgery KW - colon resection KW - postoperative inflammation KW - cost-effectiveness KW - left hemicolectomy Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-286203 SN - 1660-4601 VL - 19 IS - 17 ER - TY - JOUR A1 - Whisnant, Adam W. A1 - Jürges, Christopher S. A1 - Hennig, Thomas A1 - Wyler, Emanuel A1 - Prusty, Bhupesh A1 - Rutkowski, Andrzej J. A1 - L'hernault, Anne A1 - Djakovic, Lara A1 - Göbel, Margarete A1 - Döring, Kristina A1 - Menegatti, Jennifer A1 - Antrobus, Robin A1 - Matheson, Nicholas J. A1 - Künzig, Florian W. H. A1 - Mastrobuoni, Guido A1 - Bielow, Chris A1 - Kempa, Stefan A1 - Liang, Chunguang A1 - Dandekar, Thomas A1 - Zimmer, Ralf A1 - Landthaler, Markus A1 - Grässer, Friedrich A1 - Lehner, Paul J. A1 - Friedel, Caroline C. A1 - Erhard, Florian A1 - Dölken, Lars T1 - Integrative functional genomics decodes herpes simplex virus 1 JF - Nature Communications N2 - The predicted 80 open reading frames (ORFs) of herpes simplex virus 1 (HSV-1) have been intensively studied for decades. Here, we unravel the complete viral transcriptome and translatome during lytic infection with base-pair resolution by computational integration of multi-omics data. We identify a total of 201 transcripts and 284 ORFs including all known and 46 novel large ORFs. This includes a so far unknown ORF in the locus deleted in the FDA-approved oncolytic virus Imlygic. Multiple transcript isoforms expressed from individual gene loci explain translation of the vast majority of ORFs as well as N-terminal extensions (NTEs) and truncations. We show that NTEs with non-canonical start codons govern the subcellular protein localization and packaging of key viral regulators and structural proteins. We extend the current nomenclature to include all viral gene products and provide a genome browser that visualizes all the obtained data from whole genome to single-nucleotide resolution. Here, using computational integration of multi-omics data, the authors provide a detailed transcriptome and translatome of herpes simplex virus 1 (HSV-1), including previously unidentified ORFs and N-terminal extensions. The study also provides a HSV-1 genome browser and should be a valuable resource for further research. KW - infected-cell protein KW - messenger RNA KW - binding protein KW - type 1 KW - identification KW - ICP27 KW - translation KW - expression KW - sequence KW - domain Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-229884 VL - 11 ER - TY - JOUR A1 - Wersebeckmann, Vera A1 - Biegerl, Carolin A1 - Leyer, Ilona A1 - Mody, Karsten T1 - Orthopteran diversity in steep slope vineyards: the role of vineyard type and vegetation management JF - Insects N2 - The abandonment of traditional agricultural practices and subsequent succession are major threats to many open-adapted species and species-rich ecosystems. Viticulture on steep slopes has recently suffered from strong declines due to insufficient profitability, thus increasing the area of fallow land considerably. Changing cultivation systems from vertically oriented to modern vineyard terraces offers an opportunity to maintain management economically viable and thus reduces further abandonment. Hillside parallel terraces favor mechanization, and their embankments offer large undisturbed areas that could provide valuable habitats. We investigated the effects of vineyard abandonment, different vineyard management types (vertically oriented vs. terraced), and local parameters on Orthoptera diversity in 45 study sites along the Upper Middle Rhine Valley in Germany. Our results show that woody structures and vineyard abandonment reduced Orthoptera diversity at the local and landscape scale due to decreased habitat quality, especially for open-adapted species. In contrast, open inter-rows of actively managed vineyard types supported heat-adapted Caelifera species. On terrace embankments, extensive management and taller vegetation benefited Ensifera species, while short and mulched vegetation in vertically oriented vineyards favored the dominance of one single Caelifera species. Our results highlight the significance of maintaining viticultural management on steep slopes for the preservation of both open-adapted Orthoptera species and the cultural landscape. KW - abandonment KW - alternating management KW - biodiversity conservation KW - grasshopper KW - insect conservation KW - succession KW - traditional land use KW - vineyard terrace Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-304891 SN - 2075-4450 VL - 14 IS - 1 ER - TY - JOUR A1 - Werner, S. A1 - Sebald, Werner T1 - Immunological techniques for studies on the biogenesis of mitochondrial membrane proteins N2 - no abstract available KW - Biochemie Y1 - 1981 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-82044 ER - TY - THES A1 - Wenzel, Jens T1 - Regulation of TLR-induced macrophage responses by cytoskeleton-associated phosphoproteins T1 - Regulation der Antwort von Makrophagen auf TLR-Stimulation durch Zytoskelett-assoziierte Phosphoproteine N2 - Toll-like receptors (TLR) are pattern recognition receptors (PRR) by which macrophages (MØ) sense pathogen-associated molecular patterns (PAMPs). The recognition of lipopolysaccharide (LPS), the PAMP of gram negative bacteria, by TLR4 triggers signaling cascades and leads to the pro-inflammatory activation of the cells. A recent quantitative and kinetic analysis of the phosphoproteome of LPS-activated primary macrophages highlighted the cytoskeleton as a cell compartment with an enriched protein phosphorylation. In total 44 cytoskeleton-associated proteins were regulated by this post-translational modification and thus might be involved in the control and regulation of key macrophage functions like spreading, motility and phagocytosis. To investigate the control of cytoskeleton-associated cell functions by TLR4 activation, we first developed a method to quantitatively measure the spreading response of bone marrow MØ after stimulation with LPS. Fluorescence microscopy was used for cell imaging and visualisation of the MØ contact area. In collaboration with the Fraunhofer Institute Erlangen, we developed and validated a software tool for the semi-automated segmentation and quantitation of MØ fluorescence microscopy data, which allowed fast, robust and objective image analysis. Using this method, we observed that LPS caused time-dependent spreading, which was detectable after 1-2 h and maximal after 24 h. Next, the impact of genetic or pharmacological inhibition of known TLR signaling components was investigated. Deficiency in the adapter protein MYD88 strongly reduced spreading activity at the late time points, but had no impact early after LPS-stimulation. A similar effect was observed upon pharmacological inhibition of ERK1/2 signaling, indicating that ERK1/2 mediates MYD88-dependent MØ spreading. In contrast, MØ lacking the MAPK p38 were impaired in the initial spreading response but responded normally 8-24 h after stimulation. The genetic deletion of the MAPK phosphatases DUSP1 and DUSP16 resulted in impaired late spreading, corroborating the essential role for functional MAPK signaling in TLR4-driven MØ spreading. To identify the contribution of other cytoskeletal phosphoproteins to MØ spreading, siRNA knockdown of selected candidate genes in primary murine MØ was employed and combined with automated quantitative image analysis. These experiments revealed a functional role for the Myosins MYO1e and MYO1f in MØ spreading. These motor proteins are strongly phosphorylated in LPS-activated MØ. Because of their ability to simultaneously bind to actin filaments and cell membrane or other proteins, we investigated their role in phagocytosis, cytokine production and antigen presentation. Phagocytosis and killing of bacteria were not affected in Myo1e-/- macrophages. However, MYO1e plays a role in chemokine secretion and antigen presentation processes. MCP1 (CCL2) release was selectively increased in Myo1e-deficient MØ and dendritic cells (DC), while cytokine secretion was unaffected. Furthermore, macrophages and DCs lacking MYO1e showed lower levels of MHC-II on the cell surface. However, mRNA levels of CCL2 and of MHC-II were unaltered. These data suggest a role for MYO1e in the transport of selected chemokines and of MHC-II molecules to the cell surface. MHC-II-restricted antigen presentation assays revealed an impaired capacity of macrophages and DC lacking MYO1e to stimulate antigen-specific T cells, suggesting that the reduced MHC-II expression is functionally relevant. Taken together, in this study first a quantitative image analysis method was developed which allows the unbiased, robust and efficient investigation of the macrophage spreading response. Combination of this method with siRNA knockdown of selected cytoskeleton-associated phosphoproteins led to the identification of MYO1e and MYO1f as regulators of macrophage spreading. Furthermore, we identified MYO1e in MØ and DC to be essential for the intracellular transport of CCL2 and MHC-II to the cell surface and for optimal stimulation of antigen-specific CD4 T cells. N2 - Toll-like Rezeptoren (TLR) sind Mustererkennungsrezeptoren (PRR) durch die Makrophagen (MØ) pathogen-assoziierte molekulare Muster (PAMPs) erkennen. Die Erkennung von Lipopolysacchariden (LPS), dem PAMP gramnegativer Bakterien, durch TLR4 löst Signalkaskaden aus, die zu einer pro-inflammatorischen Aktivierung der Zellen führen. Eine quantitative und kinetische Analyse des Phosphoproteoms LPS-aktivierter primärer Makrophagen identifizierte das Zytoskelett als ein Zellkompartiment mit gesteigerter Proteinphosphorylierung. Insgesamt wurden 44 Zytoskelett-assoziierte Proteine identifiziert, die durch diese post-translationale Modifikation reguliert wurden und demzufolge an der Regulation wichtiger Zellfunktionen von Makrophagen wie Spreading, Motilität und Phagozytose beteiligt sein könnten. Um die Kontrolle Zytoskelett-vermittelter Zellfunktionen nach TLR4 Aktivierung zu untersuchen, entwickelten wir zunächst eine Methode zur quantitativen Messung der Spreadingantwort von Knochenmarksmakrophagen nach LPS Stimulation. Die Visualisierung der Zellen sowie ihrer Kontaktfläche erfolgte hierbei mittels Fluoreszenzmikroskopie. Für eine schnelle, robuste und objektive Analyse der Fluoreszenzaufnahmen entwickelten und validierten wir in Kollaboration mit dem Fraunhofer Institut in Erlangen eine Software zur halbautomatischen Segmentierung und Quantifizierung der Kontaktfläche. Unter Verwendung dieser Methode konnte eine zeitabhängige LPS-induzierte Zunahme der Zellkontaktfläche beobachtet werden, die nach 1-2 Stunden detektierbar war und ein Maximum nach 24 Stunden erreichte. Durch den Einsatz pharmakologischer Inhibitoren sowie genetisch veränderter Zellen wurde anschließend der Einfluss bekannter TLR4-Signalwegkomponenten untersucht. Die genetische Defizienz des Adapterproteins MYD88 führte hierbei zu einer stark reduzierten Spreadingaktivität der Zellen während der späten LPS Stimulationsphase, wohingegen das initiale Spreading nicht beeinflusst wurde. Ein vergleichbarer Effekt konnte unter Verwendung eines pharmakologischen Inhibitors zur Hemmung des ERK1/2 Signalweges identifiziert werden. Diese Beobachtungen deuten darauf hin, dass ERK1/2 für die Weiterleitung des MYD88 vermittelten Spreading notwendig ist. Im Gegensatz dazu wurde in p38-defizienten Makrophagen ein beeinträchtigtes initiales Spreading beobachtet, wohingegen das späte Spreading nach 8 – 24 Stunden nicht beeinflusst war. Die genetische Deletion der MAPK Phosphatasen DUSP1 und DUSP16 resultierte ebenfalls in einer Minderung des späten Spreadings, ebenfalls ein Hinweis auf die essentielle Rolle funktioneller MAPK Signalwege. Um die Beteiligung weiter Zytoskelett-Phosphoproteine am Zellspreading zu identifizieren, wurde die Expression ausgewählter Kandidatengene in primären Makrophagen mittels spezifischer siRNA unterdrückt und das Zellspreading mit Hilfe der entwickelten Software quantifiziert. Diese Versuche zeigten eine funktionelle Rolle der Myosine MYO1e und MYO1f. Diese Motorproteine weisen ebenfalls eine starke Phosphorylierung nach LPS Stimulation auf. Aufgrund ihrer Eigenschaft simultan mit Aktinfilamenten und Zellmembranen sowie anderen Proteinen zu interagieren, untersuchten wir ihre Rolle während der Phagozytose, Zytokinfreisetzung und Antigenpräsentation. Obwohl Myo1e defiziente Makrophagen keine Beeinträchtigung der Phagozytose oder Abtötung von Bakterien aufwiesen, spielte das Motorprotein eine wichtige Rolle in der Chemokinfreisetzung und Antigenpräsentation. Interessanterweise war die Sekretion des Chemokins MCP1 (CCL2) in Myo1e-defizienten Makrophagen und dendritischen Zellen (DC) selektiv erhöht, während die Zytokinfreisetzung unbeeinträchtigt war. Des Weiteren wiesen Myo1e KO Makrophagen und DC eine reduzierte MHC-II Oberflächen-Expression auf, obwohl die MHC-II als auch die CCL2 Transkription auf mRNA Ebene nicht beeinflusst war. Diese Daten legen nahe, dass MYO1e während des Transports bestimmter Chemokine, sowie von MHC-II zur Zelloberfläche eine wichtige Rolle spielt. Zudem zeigten Myo1e KO Makrophagen und DC in einem MHC-II-abhängigen Antigenpräsentationsassay eine abgeschwächte Fähigkeit zur Antigen-spezifischen T-Zell Aktivierung, was die funktionelle Relevanz der reduzierten Expression von MHC-II nahelegt. Zusammenfassend wurde in dieser Studie zunächst eine Methode zur quantitativen Bildanalyse entwickelt, welche eine unvoreingenommene, robuste und effiziente Untersuchung des Spreadings von Makrophagen erlaubte. Die Kombination dieser Methode mit dem spezifischen siRNA Knockdown ausgewählter Zytoskelett-assoziierter Phosphoproteine führte zur Identifizierung von MYO1e und MYO1f als wichtige Regulatoren dieser Zellfunktion. Darüber hinaus konnte in Makrophagen und DC eine essentielle Rolle für MYO1e im intrazellulären Transport von CCL2 und MHC-II an die Zelloberfläche identifiziert werden, sowie dessen Notwendigkeit für eine vollständige Aktivierung antigen-spezifischer CD4 T Zellen. KW - Toll-like-Rezeptoren KW - Makrophage KW - Phosphoproteine KW - Zellskelett KW - macrophage KW - cytoskeleton KW - phosphorylation KW - TLR4 Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-98843 ER - TY - THES A1 - Wenzel, Frank T1 - Smell and repel: Resin based defense mechanisms and interactions between Australian ants and stingless bees N2 - Bees are subject to permanent threat from predators such as ants. Their nests with large quantities of brood, pollen and honey represent lucrative targets for attacks whereas foragers have to face rivalry at food sources. This thesis focused on the role of stingless bees as third party interactor on ant-aphid-associations as well as on the predatory potential represented by ants and defense mechanisms against this threat. Regular observations of an aphid infested Podocarpus for approaching stingless bees yielded no results. Another aim of this thesis was the observation of foraging habits of four native and one introduced ant species for assessment of their predatory potential to stingless bees. All species turned out to be dietary balanced generalists with one mostly carnivorous species and four species predominantly collecting nectar roughly according to optimal foraging theory. Two of the species monitored, Rhytidoponera metallica and Iridomyrmex rufoniger were considered potential nest robbers. As the name implies, stingless bees lack the powerful weapon of their distant relatives; hence they specialized on other defense strategies. Resin is an important, multipurpose resource for stingless bees that is used as material for nest construction, antibiotic and for defensive means. For the latter purpose highly viscous resin is either directly used to stick down aggressors or its terpenic compounds are included in the bees cuticular surface. In a feeding choice experiment, three ant species were confronted with the choice between two native bee species - Tetragonula carbonaria and Austroplebeia australis - with different cuticular profiles and resin collection habits. Two of the ant species, especially the introduced Tetramorium bicarinatum did not show any preferences. The carnivorous R. metallica predominantly took the less resinous A. australis as prey. The reluctance towards T. carbonaria disappeared when the resinous compounds on its cuticle had been washed off with hexane. To test whether the repulsive reactions were related to the stickiness of the resinous surface or to chemical substances, hexane extracts of bees’ cuticles, propolis and three natural tree resins were prepared. In the following assay responses of ants towards extract treated surfaces were observed. Except for one of the resin extracts, all tested substances had repellent effects to the ants. Efficacy varied with the type of extract and species. Especially to the introduced T. bicarinatum the cuticular extract had no effect. GCMS-analyses showed that some of the resinous compounds were also found in the cuticular profile of T. carbonaria which featured reasonable analogies to the resin of Corymbia torelliana that is highly attractive for stingless bees. The results showed that repellent effects were only partially related to the sticky quality of resin but were rather caused by chemical substances, presumably sesqui- and diterpenes. Despite its efficacy this defense strategy only provides short time repellent effects sufficient for escape and warning of nest mates to initiate further preventive measures. N2 - Bienen sind permanent Gefahren ausgesetzt, ihre Nester voll Brut, Pollen und Honig bieten ein ertragreiches Ziel für Räuber und auch bei der Nahrungssuche droht Konkurrenz an den Futterquellen, beispielsweise durch Ameisen. Ziel dieser Arbeit war es zu untersuchen, welche Rolle stachellose Bienen in Australien als dritter Interaktionspartner an Ameisen-Blattlaus-Assoziationen einnehmen, welcher Bedrohung sie durch räuberische Ameisen ausgesetzt sind und wie sie sich gegen diese verteidigen. Regelmäßige Beobachtungen einer von Blattläusen befallenen Steineibe auf Besuche von stachellosen Bienen blieben erfolglos, es wurden keine Anflüge erfasst. Ein weiterer Fokus dieser Arbeit lag auf der Untersuchung des Nahrungseintrags von vier heimischen, sowie einer eingeschleppten Ameisenart zur Erfassung des räuberischen Potenzials gegenüber stachellosen Bienen. Alle Ameisenarten stellten sich als Generalisten mit ausgewogenem Nahrungseintrag heraus. Eine der Arten ernährte sich hauptsächlich räuberisch, während der Eintrag von Nektar für vier Arten die Hauptressource darstellte und annäherungsweise gemäß der „optimal foraging theory“ erfolgte. Zwei der untersuchten Arten, Rhytidoponera metallica und Iridomyrmex rufoniger, wurden als potenzielle Nesträuber eingestuft. Stachellose Bienen können sich nicht durch Stiche verteidigen, sie nutzen daher andere Strategien. Pflanzenharz stellt für Bienen eine vielseitige Ressource dar, welche als Baumaterial, Desinfiziens und auch zur Verteidigung eingesetzt wird. Das Harz wird entweder in zähflüssiger Form dazu verwendet, um Angreifer zu verkleben oder die darin enthaltenen Terpene gelangen in Bestandteilen auf die Oberfläche der Bienen. In einem Futterwahl-Experiment wurden Tetragonula carbonaria und Austroplebeia australis, zwei heimische Bienenarten mit unterschiedlichen Harzsammel-Gewohnheiten und Oberflächenprofilen, drei Ameisenarten als Beute vorgelegt. Während zwei der Ameisenarten, insbesondere die eingeführte Tetramorium bicarinatum, keinerlei Präferenzen zeigte, entschieden sich die karnivoren R. metallica vorrangig für A. australis, deren Oberflächenprofil weniger Harzkomponenten aufwies. Wurden die Oberflächenbestandteile von T. carbonaria durch Waschen mit Hexan entfernt, verschwand auch die Zurückhaltung der Räuber. Um zu untersuchen ob diese Abwehrreaktion durch die Klebrigkeit der Oberfläche oder durch chemische Substanzen verursacht wurde, wurden Hexan-Extrakte der Bienenoberflächen sowie von drei Baumharzen und Nestmaterial angefertigt. Die nachfolgenden Untersuchungen richteten sich daraufhin auf die Beobachtung der Reaktion von Ameisen bei Kontakt mit Extrakt-behandelten Oberflächen. Bis auf einen der Harzextrakte zeigten alle untersuchten Substanzen unterschiedlich stark abstoßende Effekte auf Ameisen. Die eingeführte T. bicarinatum wurde jedoch nicht durch Bienenextrakt in ihrem Verhalten beeinflusst. Eine GCMS-Analyse ergab, dass einige der Harzsubstanzen auch im Oberflächenprofil von T. carbonaria zu finden waren, welches vor allem Übereinstimmungen mit dem Harz von Corymbia torelliana aufwies, einer Pflanze deren Harz für Bienen besonders attraktiv ist. Es zeigte sich, dass nicht nur die Klebrigkeit, sondern auch chemische Substanzen, vermutlich Sesqui- und Diterpene, für abstoßende Effekte verantwortlich sind. Trotz der Effektivität dieses Mechanismus sorgt er nur für eine kurzzeitige Abwehrreaktion, ermöglicht jedoch die Gelegenheit zur Flucht und Warnung von Nestgenossen, sowie zur Einleitung weiterer Gegenwehr. KW - Stachellose Biene KW - Biene KW - Tierökologie KW - Verhaltensforschung KW - Ameisen KW - Interaktion KW - Abwehr KW - Verteidigung KW - Trophobiose KW - Nahrungserwerb KW - stingless bees KW - ants KW - interaction KW - resin KW - defense Y1 - 2011 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-65960 ER - TY - THES A1 - Wende, Beate T1 - Diversity of saproxylic beetles and host tree specialisation in differently managed forests across Germany T1 - Artenvielfalt und Wirtsbaumartenspezialiserung totholzbewohnender Käfer in verschiedenen Wäldern Deutschlands N2 - Chapter I The gradual turnover of dead organic material into mineral nutrients is a key ecological function, linking decomposition and primary production, the essential parts of the nutrient-energy cycle. However, disturbances in terms of species or resource losses might impair the equilibrium between production and decomposition. Humanity has converted large proportions of natural landscapes and intensified land-use activity for food production. Globally, only very few areas are totally unaffected by human activity today. To ensure the maintenance of both essential ecosystem services, knowledge about the interplay of biodiversity and ecosystem functioning as well as effects of intensified management on both is crucial. The vast majority of terrestrial biomass production as well as decomposition take place in forest ecosystems. Though forestry has a long sustainable history in Europe, its intensification during the last century has caused severe impacts on forest features and, consequently, on the associated biota, especially deadwood dependent organisms. Among these, saproxylic beetles are the most diverse group in terms of species numbers and functional diversity, but also most endangered due to habitat loss. These features classify them as ideal research organisms to study effects of intensified forestry on ecosystem services. The BELONGDEAD project located in Germany aimed to investigate deadwood decay and functional consequences of diversity changes in the associated fauna on the decomposition process from the initialisation of deadwood decay to complete degradation. As part of the BeLongDead project, this dissertation focussed on saproxylic beetle species, thereby evaluating (1) regionally effects of tree species identity of fresh deadwood and (2) forest management of varying intensities on the diversity, abundance and community composition of saproxylic beetles (chapter II); (3) the specialisation degree of different trophic guilds of saproxylic beetles, and thus the stability and robustness of their interaction networks against disturbances (chapter III); (4) the impact of environmental features of local to regional spatial scales on species richness of saproxylic beetles differing in their habitat niche in terms of deadwood decay stages (chapter IV). Chapter II The vast majority of European forest ecosystems have been anthropogenically affected, leaving less than 1% of the about 1 milliard hectare as natural forests. A long history of forestry and especially the technological progress during the last century have caused massive habitat fragmentation as well as substantial loss of essential resources in European forest ecosystems. Due to this, the substrate-dependent group of saproxylic beetles has experienced severe species losses. Thus, investigations concerning saproxylic diversity and deadwood volume were badly needed. However, the importance of different deadwood in terms of tree species identity for the colonization by saproxylic beetles under different local and regional management regimes is poorly understood. Therefore, we studied possible regional differences in colonization patterns of saproxylic beetle species in a total of 688 fresh deadwood logs of 13 tree species in 9 sites of managed conifer and beech forests, and unmanaged beech forests, respectively. We found that tree species identity was an important driver in determining saproxylic species composition and abundance within fresh deadwood. However, saproxylic species showed different colonization patterns of deadwood items of the same tree species among the study regions. Regionally consistent, conifer forests were most diverse. We attribute the latter result to the historically adaption of saproxylic beetle species to semi-open forests, which conditions are actually best reflected by conifer forests. To preserve a diverse local species pool of early successional saproxylic beetles, we suggest an equal high degree of deadwood diversity in a tree species context in due consideration of regional differences. Chapter III The extinction risk of a particular species corresponds with its species-specific requirements on resources and habitat conditions, in other words with the width of the species` ecological niche. Species with a narrow ecological niche are defined as specialists. Members of this group experience higher extinction risk by resource limitation than generalists, which are able to utilize a variety of resources. For the classification of species as specialists or generalists, thus evaluating possible extinction risks, ecologists use the concept of interaction networks. This method has often been applied for mutualistic or antagonistic plant-animal interactions, but information for networks of detritivores is scarce. Therefore, saproxylic beetle species sampled as described in chapter II were categorised according to their larval diet; additionally their interaction networks (N=108) with 13 dead host tree species were analysed. Specialisation degree was highest for wood-digesting beetles and decreased with increasing trophic level. Also the network indices evaluating robustness and generality indicated a higher susceptibility to species extinctions for xylophagous than for mycetophagous and predatory beetles. The specialisation of xylophagous species on specific tree species might be an adaption to tree species specific ingredients stored for defence against pathogens and pests. However, we conclude that the high specialisation degree of xylophages and thus their higher extinction risk by resource loss harbours certain dangers for ecosystem function and stability as species diversity is positively linked to both. Chapter IV Populations depend on individual emigration and immigration events to ensure genetic exchange. For successful migration it is of utmost importance that spatially separated populations are obtainable by specimen. Migratory success depends on the one hand on the species dispersal abilities and on the other on the availability of suitable habitats in the surrounding landscape in which the distinct host populations exist. However, consequences of intensive forest management correspond not only to severe reduction of local deadwood amount, but, among others, also a change in tree species composition and high levels of fragmentation in the surrounding forest area. Saproxylic beetle species differ in their dispersal behaviour according to the temporal availability of their preferred habitat. Generally, early successional saproxylic beetles are able to disperse over large distances, whereas beetles inhabiting advanced decayed wood often remain close to their larval habitat. Due to this, environmental factors might affect saproxylic beetle guilds differently. We classified the saproxylic beetles sampled as described in chapter II according to their calculated habitat niche as early, intermediate or late successional saproxylic beetles. For the different guilds the effects of 14 environmental factors on different spatial scales (stand factors at 0.1 km radius, landscape composition at 2 km radius, and regionally differing abiotic factors in 400 km to 700 km distance) were investigated. Consistently for all guilds, species richness decreased with fragmentation at local and landscape scale, and increased in warmer climate. However, we found contradictory results between the guilds to some extent. We relate this to guild specific habitat requirements of the saproxylic beetles. Therefore, for the development of appropriate conservation practices guild-specific requirements saproxylic beetles have to be considered not only locally but on larger spatial scales. Chapter V In conclusion, this dissertation identified main drivers of early successional saproxylic beetle species richness on various spatial scales. Our results emphasize the importance to develop management schemes meeting species-specific and guild-specific habitat requirements of the saproxylic beetle fauna at relevant spatial and temporal scales. Therefore, short-term actions suggested for sustainable forest management should be the focus on a diverse tree species composition consisting of indigenous tree species with respect to regional differences. Moreover, senescent trees, fallen and standing deadwood should remain in the forests, and some tree individuals should be allowed to grow old. Long-term actions should involve the reduction of forest fragmentation and the connection of spatial widely separated forest fragments. Furthermore, to fully understand the effects of forest management long-term research should be conducted to compare habitat requirements of intermediate and late successional beetles with the results presented in this dissertation. N2 - Kapitel I Die Mineralisierung von toter organischer Materie nimmt eine Schlüsselfunktion innerhalb eines Ökosystems ein, da sie die beiden essentiellen Komponenten des Energie-Nährstoff-Zyklus - Zersetzung und Primärproduktion - miteinander verbindet. Anthropogen bedingte Störungen wie z.B. Arten-, oder Ressourcenverluste können jedoch das Gleichgewicht zwischen den beiden wichtigen Ökosystemdienstleistungen Produktion und Abbau aus der Balance bringen. Um die Nahrungsversorgung der Menschheit zu gewährleisten, wurde bereits ein großer Teil der Natur in Agrarflächen umgewandelt und die Produktion durch intensive Bewirtschaftungsformen gesteigert. Weltweit gibt es nur noch wenige Gebiete ohne menschliche Beeinflussung. Um dauerhaft essentielle Ökosystemdienstleistungen zu gewährleisten, sind Kenntnisse über die Auswirkungen von intensiver Bewirtschaftung auf das Zusammenspiel zwischen Artenvielfalt und Ökosystemfunktionen unabdingbar. Der größte Teil der terrestrischen Biomasseproduktion wird von Wäldern geleistet. Obwohl die Waldbewirtschaftung in Europa lange Zeit nachhaltig war, wirkte sich deren Intensivierung während des letzten Jahrhunderts massiv auf die Waldstruktur und die damit assoziierte Fauna aus. Besonders betroffen sind die obligatorisch an Totholz gebundenen Organismen. Innerhalb der Totholzfauna sind xylobionte Käfer eine artenreiche und funktional hoch diverse Gruppe, doch aufgrund von Lebensraumverlusten sind viele Arten stark bedroht. All diese Eigenschaften klassifizieren Totholzkäfer zu idealen Forschungsobjekten, um die Auswirkungen von intensiver Waldbewirtschaftung auf Ökosystemfunktionen zu untersuchen. Das BELONGDEAD-Projekt hat als Ziel, die funktionalen Auswirkungen von Veränderungen in der Artengemeinschaft auf die Abbauraten von Totholz zu analysieren. Der Untersuchungszeitraum des in Deutschland beheimateten Projekts umfasst die Initialisierung des Zersetzungsprozesses bis zum vollständigen Abbau von experimentell ausgelegten Totholzstämmen unterschiedlicher Baumarten. Als Teil des BELONGDEAD-Projekts lag der Fokus der vorliegenden Dissertation auf der Totholzkäferfauna. Wir untersuchten (1) regionale Effekte der Baumartenzugehörigkeit von frischem Totholz und (2) die Auswirkungen von Waldbewirtschaftung unterschiedlicher Intensität auf die Artenvielfalt, Abundanz und Struktur der Artengemeinschaften von totholzbewohnenden Käfern (Kapitel II); (3) den Spezialisierungsgrad verschiedener trophischer Gilden von Totholzkäfern, sowie die Stabilität und Robustheit ihrer jeweiligen Netzwerke gegen Störungen (Kapitel III); (4) den Einfluss von Umweltfaktoren auf die Artenvielfalt xylobionter Käfergilden auf mehreren räumlichen Skalen. Kapitel II Der Großteil der europäischen Wälder ist anthropogen beeinflusst. In Europa bilden Naturwälder weniger als 1% der gesamten Waldfläche von ca. 1 Mrd. Hektar. Traditionelle Waldbewirtschaftung und vor allem der technologische Fortschritt des letzten Jahrhunderts fragmentierten die Waldfläche in hohem Maß, und verursachten beträchtliche Verluste an lebensnotwendigen Ressourcen. Besonders innerhalb der obligatorisch an Totholz gebundenen Gruppe der xylobionten Käfer verzeichnete man einen rasanten Artenrückgang. Daher gab es einen großen Bedarf an Studien, die Untersuchungen zur Mindestmenge an lokal vorhandenem Totholz zur Sicherung der xylobionten Artenvielfalt durchführten. Wenig beachtet wurde bisher jedoch die Bedeutung der Baumartenzugehörigkeit von Totholz für die Besiedlung durch xylobionter Käfer in verschiedenen Waldbewirtschaftungssystemen auf lokaler und regionaler Ebene. Wir untersuchten daher mögliche Unterschiede zwischen 3 Regionen im Besiedlungsmuster xylobionter Käfer bei insgesamt 651 experimentell ausgelegten Baumstämmen in einem frühen Sukzessionsstadium von 13 Baumarten auf jeweils 9 Untersuchungsflächen in bewirtschafteten Buchen- und Nadelwäldern, sowie in unbewirtschafteten Buchenwäldern. Bei den ausgelegten Totholzstämmen war die Baumartenzugehörigkeit ausschlaggebend für die Struktur der Artengemeinschaften und Abundanzen xylobionter Käfer. Aufgrund der unterschiedlichen regionalen Artenpools divergierten die Besiedlungsmuster xylobionter Käferarten von Totholz der gleichen Baumart in den verschiedenen Regionen stark voneinander. In allen Regionen zeigten die Totholzkäfer in Nadelwäldern die höchste Artenvielfalt. Dieses Ergebnis lässt sich auf die - historisch bedingte - Anpassung der Totholzkäferfauna an eine halboffene Waldstruktur zurückführen, die derzeit am besten durch Nadelwälder widergespiegelt wird. Um eine diverse lokale Artengemeinschaft xylobionter Käfer zu gewährleisten ist eine große Variabilität vom baumartspezifischen Totholz unabdingbar, wobei regionale Unterschiede in Betracht gezogen werden müssen. Kapitel III Das Aussterberisiko einer Art ist abhängig von den artspezifischen Ansprüchen an ihre Umwelt und den dort vorkommenden Ressourcen –auch definiert als die ökologische Nische der betrachteten Art. Arten mit geringer Nischenbreite sind per definitionem Spezialisten. Mitglieder dieser Gruppe stehen durch Verarmung ihres Ressourcenangebots unter einem höheren Aussterberisiko als Generalisten, die eine größere Variabilität in ihrem Ressourcenspektrum aufweisen. Interaktionsnetzwerke dienen in der Ökologie als wichtiges Werkzeug um das Aussterberisiko spezifischer Arten zu bewerten und eine Einteilung hinsichtlich Spezialist oder Generalist vorzunehmen. Bei mutualistischen oder antagonistischen Tier-Pflanzen-Interaktionen ist diese Methode etabliert, doch für die Gruppe der Zersetzer ist das Netzwerk-Konzept bisher nur sporadisch angewandt worden. Daher teilten wir die xylobionten Käferarten, die im Rahmen des in Kapitel II beschriebenen Experiments gesammelt wurden, anhand ihres larvalen Ernährungstyps in drei trophische Gilden (Xylophage, Mycetophage und Räuber) ein; anschließend wurden ihre Interaktionsnetzwerke (N= 108) mit den 13 Wirtsbaumarten analysiert. Rein xylophage Arten wiesen den höchsten Spezialisierungsgrad auf, der mit zunehmendem trophischem Grad geringer wurde. Die Netzwerkparameter Robustheit und Generalität ließen ebenfalls auf eine höhere Anfälligkeit für Artenverluste bei xylophagen als bei mycetophagen oder räuberischen Arten schließen. Die Spezialisierung xylophager Arten auf spezifische Baumarten ist möglicherweise eine Adaption an artenspezifische sekundäre Inhaltsstoffe, die als Schutz vor Schädlingen und Krankheitserregern in Holz und Rinde gespeichert werden. Der hohe Spezialisierungsgrad xylophager Käfer bedingt ein höheres Aussterberisiko bei Ressourcenverlust. Dies würde die Stabilität des Ökosystems und dessen Ökosystemfunktionen nachhaltig schwächen da eine hohe Artenvielfalt Garant für ein funktionierendes Ökosystem ist. Kapitel IV Individuelle Immigrations- und Emigrationsereignisse sind für die Sicherstellung des genetischen Austauschs zwischen Populationen essentiell. Daher ist von größter Wichtigkeit, dass die räumliche Distanz zwischen Populationen von den zu- oder abwandernden Individuen überwunden werden kann. Der Migrationserfolg ist dabei zum einen von der artspezifischen Ausbreitungsfähigkeit, und zum anderen von der Verfügbarkeit an geeigneten Habitaten in der Umgebung der Populationen abhängig. Die Folgen intensiver Waldbewirtschaftung sind jedoch nicht nur ein drastische Verminderung des lokalen Totholzvolumens, sondern unter anderem auch die Veränderung der Baumartengesellschaften, sowie hochgradige Fragmentierung der Waldflächen und der umgebenden Landschaft. Xylobionte Käferarten unterscheiden sich in ihrem Ausbreitungsverhalten hinsichtlich der zeitlichen Verfügbarkeit ihres bevorzugten Habitats. Im Allgemeinen können Besiedler früher Sukzessionsstadien weite Strecken überwinden, wohingegen Bewohner von Alttotholzstrukturen meist nahe ihrem Ursprungshabitat verbleiben. Dies legt die Vermutung nahe, dass Umweltparameter verschieden auf unterschiedliche Habitatgilden einwirken. Um diese Vermutung zu überprüfen, wurde für die gesammelten xylobionten Käferarten ihre jeweilige Habitatnische berechnet. Wir klassifizierten die Arten als Besiedler von entweder frühen, mittleren oder alten Totholzstrukturen. Für jede Gilde wurde der Einfluss von 14 Umweltparametern auf verschiedenen räumlichen Skalen - Standortfaktoren der Untersuchungsfläche (Radius: 100 m), Landschaftsparameter im Umkreis von 2 km der Untersuchungsfläche, sowie regionenspezifische abiotische Faktoren (Distanz zwischen den Regionen: 400 – 700 km) - untersucht. Bei starker lokaler und landschaftlicher Fragmentierung nahmen die Artenzahlen in den xylobionten Gilden ab, während sich höhere Jahresdurchschnittstemperatur positiv auf die Artenvielfalt auswirkte. Jedoch gab es hatten nicht alle Umweltfaktoren den gleichen Effekt auf die Gilden. Wir führen dies auf die unterschiedlichen Habitatansprüche der xylobionten Gilden zurück. Um adäquate Schutzmaßnahmen für Totholzkäfer zu entwickeln, müssen die spezifischen Habitatansprüche der verschiedenen xylobionten Gilden, nicht nur auf lokaler, sondern auch auf größeren räumlichen Ebenen in die Planungen miteinbezogen werden. Kapitel V In der vorliegenden Dissertation konnte ich wichtige Triebfedern der Artenvielfalt xylobionter Käfer identifizieren. Unsere Ergebnisse unterstreichen die Notwendigkeit der Entwicklung von nachhaltigen Waldbewirtschaftungskonzepten, die den art- und gildenspezifischen Anforderungen xylobionter Käfer an den Lebensraum auf den relevanten räumlichen und zeitlichen Skalen gerecht werden. Kurzfristige Maßnahmepläne für eine nachhaltige Forstwirtschaft sollte die Förderung von Mischwäldern mit einer vielfältigen Baumartengemeinschaft mit standortgemäßen einheimischen Hölzern unter Berücksichtigung regionaler Besonderheiten beinhalten. Alte Bäume, sowie liegendes und stehendes Totholz sollten im Wald verbleiben und einzelne Bäume aus der Nutzung genommen werden um die Strukturen altgewachsener Bäume langfristig zu gewährleisten. Langfristige Ziele sind die Verringerung der Waldfragmentierung und das Anlegen von Biotopverbundsystemen, um weit auseinanderliegende Waldflächen wieder miteinander zu verbinden. Um die Auswirkungen kommerzieller Forstwirtschaft im vollen Umfang zu erfassen, sind Langzeitstudien notwendig die die Habitatansprüche xylobionter Käfer aus mittleren und alten Totholzsukzessionsstadien mit den Ergebnissen der vorliegenden Dissertation vergleichen. KW - Saproxylophage KW - Käfer KW - Ökosystem KW - Saproxylic beetles KW - temperate forests KW - Deutschland KW - Wald KW - saproxylic Coleoptera KW - Forest management KW - Diversity Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-107049 ER - TY - JOUR A1 - Welter, Nils A1 - Wagner, Angelo A1 - Furtwängler, Rhoikos A1 - Melchior, Patrick A1 - Kager, Leo A1 - Vokuhl, Christian A1 - Schenk, Jens-Peter A1 - Meier, Clemens Magnus A1 - Siemer, Stefan A1 - Gessler, Manfred A1 - Graf, Norbert T1 - Correction: Welter et al. Characteristics of nephroblastoma/nephroblastomatosis in children with a clinically reported underlying malformation or cancer predisposition syndrome. Cancers 2021, 13, 5016 JF - Cancers N2 - In the original article [1] there was a mistake in Table 2 as published. Table 2 contains wrong percentages in lines Bilateral disease and Patients with CPS or GU. For this reason the table should be replaced with the correct one as shown below. KW - nephroblastomatosis Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-250135 SN - 2072-6694 VL - 13 IS - 22 ER - TY - JOUR A1 - Welter, Nils A1 - Wagner, Angelo A1 - Furtwängler, Rhoikos A1 - Melchior, Patrick A1 - Kager, Leo A1 - Vokuhl, Christian A1 - Schenk, Jens-Peter A1 - Meier, Clemens Magnus A1 - Siemer, Stefan A1 - Gessler, Manfred A1 - Graf, Norbert T1 - Characteristics of nephroblastoma/nephroblastomatosis in children with a clinically reported underlying malformation or cancer predisposition syndrome JF - Cancers N2 - (1) Background: about 10% of Wilms Tumor (WT) patients have a malformation or cancer predisposition syndrome (CPS) with causative germline genetic or epigenetic variants. Knowledge on CPS is essential for genetic counselling. (2) Methods: this retrospective analysis focused on 2927 consecutive patients with WTs registered between 1989 and 2017 in the SIOP/GPOH studies. (3) Results: Genitourinary malformations (GU, N = 66, 2.3%), Beckwith-Wiedemann spectrum (BWS, N = 32, 1.1%), isolated hemihypertrophy (IHH, N = 29, 1.0%), Denys-Drash syndrome (DDS, N = 24, 0.8%) and WAGR syndrome (N = 20, 0.7%) were reported most frequently. Compared to others, these patients were younger at WT diagnosis (median age 24.5 months vs. 39.0 months), had smaller tumors (349.4 mL vs. 487.5 mL), less often metastasis (8.2% vs. 18%), but more often nephroblastomatosis (12.9% vs. 1.9%). WT with IHH was associated with blastemal WT and DDS with stromal subtype. Bilateral WTs were common in WAGR (30%), DDS (29%) and BWS (31%). Chemotherapy induced reduction in tumor volume was poor in DDS (0.4% increase) and favorable in BWS (86.9% reduction). The event-free survival (EFS) of patients with BWS was significantly (p = 0.002) worse than in others. (4) Conclusions: CPS should be considered in WTs with specific clinical features resulting in referral to a geneticist. Their outcome was not always favorable. KW - nephroblastoma KW - clinical malformations KW - cancer predisposition syndromes KW - tumor surveillance KW - outcome Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-248434 SN - 2072-6694 VL - 13 IS - 19 ER - TY - JOUR A1 - Weiße, Sebastian A1 - Heddergott, Niko A1 - Heydt, Matthias A1 - Pflästerer, Daniel A1 - Maier, Timo A1 - Haraszti, Tamas A1 - Grunze, Michael A1 - Engstler, Markus A1 - Rosenhahn, Axel T1 - A Quantitative 3D Motility Analysis of Trypanosoma brucei by Use of Digital In-line Holographic Microscopy JF - PLoS One N2 - We present a quantitative 3D analysis of the motility of the blood parasite Trypanosoma brucei. Digital in-line holographic microscopy has been used to track single cells with high temporal and spatial accuracy to obtain quantitative data on their behavior. Comparing bloodstream form and insect form trypanosomes as well as mutant and wildtype cells under varying external conditions we were able to derive a general two-state-run-and-tumble-model for trypanosome motility. Differences in the motility of distinct strains indicate that adaption of the trypanosomes to their natural environments involves a change in their mode of swimming. KW - african trypanosomes KW - actin cortex KW - flagellum KW - tracking KW - surface KW - models Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-130666 VL - 7 IS - 5 ER - TY - THES A1 - Weiß, Sabine T1 - Function of the Spir actin nucleators in intracellular vesicle transport processes T1 - Funktion der Spir Aktin Nukleatoren in intrazellulären Vesikeltransportprozessen N2 - Spir proteins are the founding members of the novel class of WH2-actin nucleators. A C-terminal modified FYVE zinc finger motif is necessary to target Spir proteins towards intracellular membranes. The function and regulation of the Spir actin organizers at vesicular membranes is almost unknown. Live cell imaging analyses performed in this study show that Spir-2 is localized at tubular vesicles. Cytoplasmic Spir-2-associated vesicles branch and form protrusions, which can make contacts to the microtubule network, where the Spir-2 vesicles stretch and slide along the microtubule filaments. The analysis of living HeLa cells expressing eGFP-tagged Spir-2, Spir-2-ΔKIND and Spir-2-ΔKW (lacking the 4 WH2 domains and the KIND domain) showed Spir-2-associated tubular structures which differ in their length and motility. Throughout the course of that study it could be shown that the tail domain of the actin motor protein myosin Vb, as a force-generating molecule, is colocalizing and co-immunoprecipitating with Spir-2-ΔKW. By using the tail domain of myosin Vb as a dominant negative mutant for myosin Vb-dependent vesicle transport processes it could be shown that Spir-2-ΔKW/MyoVb-cc-tail- associated vesicles exhibit an increased elongation. Moreover, using the microtubule depolymerizing drug nocodazole it could be shown that the elongation and the motility of Spir-2-ΔKW-associated vesicles depends on an intact microtubule cytoskeleton. Motility and morphological dynamics of Spir-2-associated vesicles is therefore dependent on actin, actin motorproteins and microtubule filaments. These results propose a model in which myosin/F-actin forces mediate vesicle branching, allowing the vesicles to move to and in between the microtubule filaments and thereby providing a new degree of freedom in vesicular motility. To determine the exact subcellular localization of Spir-2, colocalization studies were performed. It could be shown that Spir-2 shows a partial colocalization to Rab11a-positive compartments. Furthermore, Spir-2 exhibits an almost identical localization to Arf1 and the Arf1 small G protein but not Rab11a could be immunoprecipitated with Spir-2-ΔKW. This suggests, that Arf1 recruits Spir-2 to Arf1/Rab11a-positive membranes. Another important function of the Spir-2 C-terminus is the membrane targeting by the FYVE domain. By performing a protein-lipid overlay assay, it has been shown that purified GST- and 6xHis-tagged Spir-2-ΔKW bind phosphatidic acid suggesting a mechanism in which Spir-2 is recruited to phosphatidic acid-enriched membranes. To further elucidate the mechanism in which Spir-2 membrane-targeting could be regulated, interaction studies of C-terminal parts of Spir-2 revealed that the Spir-2 proteins interact directly. N2 - Spir Proteine sind die ersten beschriebenen Mitglieder der neuen Klasse der WH2-Aktin Nukleatoren. Ein C-terminaler modifizierter FYVE Zinkfinger ist notwendig um Spir Proteine an intrazelluläre Membranen zu bringen. Die Funktion und die Regulation dieser Aktin Nukleatoren an vesikulären Membranen ist bis jetzt noch nahezu unbekannt. In dieser Studie durchgeführte “Live-cell-Imaging” Experimente zeigten, dass Spir-2 an tubulären Vesikeln lokalisiert ist. Zytoplasmatische Spir-2-assoziierte Vesikel formen Ausläufer, die Kontakte zum Mikrotubuli Netzwerk bilden. Spir-2 Vesikel haben die Fähigkeit sich entlang des Mikrotubuli Zytoskeletts auszudehnen und daran entlang zu gleiten. Die Analyse von lebenden HeLa Zellen, welche eGFP-Spir-2, eGFP-Spir-2-ΔKIND und eGFP-Spir-2-ΔKW (Deletion der 4 WH2 Domänen sowie der KIND Domäne) Fusionsproteine exprimieren, zeigen Spir-2-assoziierte tubuläre Vesikel, die sich in Länge und Beweglichkeit unterscheiden. Während dieser Studie konnte außerdem gezeigt werden, dass die “tail” Domäne des Aktinmotors myosin Vb mit Spir-2-ΔKW kolokalisiert und koimmunopräzipitiert. Die Verwendung der “tail” Domäne als dominant negative Mutante für myosin Vb-abhängigen Vesikeltransport zeigte, dass Spir-2-ΔKW/MyoVb-cc-tail-assoziierte Vesikel eine stark erhöhte Elongation aufweisen. Desweiteren konnte duch die Verwendung von Nocodazol, welches spezifisch Mikrotubulifilamente depolymerisiert, gezeigt werden, dass die Elongation und die Motilität der Spir-2-ΔKW-assoziierten Vesikel von einem intakten Mikrotubuli Zytoskelett abhängig ist. Motilität und morphologische Dynamik der Spir-2-ΔKW-assoziierten Vesikel ist daher abhängig von Aktinfilamenten, Aktin Motorproteinen und Mikrotubulifilamenten. Anhand dieser Ergebnisse lässt sich ein Modell erstellen, in welchem eine Myosin/F-actin induzierte Bewegung eine Verzweigung der Vesikel bewirkt. Dadurch ist eine Bewegung der Vesikel zu Mikrotubulifilamenten aber auch zwischen verschiedenen Mikrotubulifilamenten möglich, welches einen ganz neuen Freiheitsgrad in der vesikulären Bewegung eröffnet. Um die genaue zelluläre Lokalisation von Spir-2 zu analysieren wurden Kolokalisationsstudien durchgeführt. Hierbei konnte gezeigt werden, dass Spir-2 eine partielle Kolokalisation mit Rab11a-positiven Kompartimenten zeigt. Außerdem weist Spir-2 eine nahezu identische Lokalisation zu Arf1 auf. Arf1, aber nicht Rab11a, konnte mit Spir-2-ΔKW koimmunpräzipitiert werden. Arf1 könnte daher für die Rekrutierung von Spir-2 an Arf1/Rab11a-positive Membranen ausschlaggebend sein. Eine weitere wichtige Funktion des Spir-2 C-Terminus ist die Membranlokalisation, welche durch die FYVE Domäne vermittelt wird. Mittels Protein-Lipid Bindungsstudien konnte gezeigt werden, dass aufgereinigte GST- bzw. 6xHis-Spir-2-ΔKW-Fusionsproteine an Phosphatidylsäure binden. Dies deutet darauf hin, dass Spir-2 spezifisch zu Phosphatidylsäure-positiven Membranen rekrutiert wird. Um die weitere Regulation der Spir-2 Membranlokalisation aufzuklären, wurden Protein-Protein-Interaktionsstudien durchgeführt, welche eine direkte Interaktion von Spir-2 Proteinen anhand ihrer C-Termini ergaben. KW - Aktin KW - Vesikeltransport KW - Intrazellulärer Transport KW - Actin KW - vesicle transport Y1 - 2011 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-64589 ER - TY - JOUR A1 - Weiß, Clemens Leonard A1 - Schultz, Jörg T1 - Identification of divergent WH2 motifs by HMM-HMM alignments JF - BMC Research Notes N2 - Background The actin cytoskeleton is a hallmark of eukaryotic cells. Its regulation as well as its interaction with other proteins is carefully orchestrated by actin interaction domains. One of the key players is the WH2 motif, which enables binding to actin monomers and filaments and is involved in the regulation of actin nucleation. Contrasting conserved domains, the identification of this motif in protein sequences is challenging, as it is short and poorly conserved. Findings To identify divergent members, we combined Hidden-Markov-Model (HMM) to HMM alignments with orthology predictions. Thereby, we identified nearly 500 proteins containing so far not annotated WH2 motifs. This included shootin-1, an actin binding protein involved in neuron polarization. Among others, WH2 motifs of ‘proximal to raf’ (ptr)-orthologs, which are described in the literature, but not annotated in genome databases, were identified. Conclusion In summary, we increased the number of WH2 motif containing proteins substantially. This identification of candidate regions for actin interaction could steer their experimental characterization. Furthermore, the approach outlined here can easily be adapted to the identification of divergent members of further domain families. KW - WH2 domain KW - spire KW - shootin-1 KW - actin nucleation KW - HHblits Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-126413 VL - 8 IS - 18 ER - TY - JOUR A1 - Weisschuh, Nicole A1 - Mayer, Anja K. A1 - Strom, Tim M. A1 - Kohl, Susanne A1 - Glöckle, Nicola A1 - Schubach, Max A1 - Andreasson, Sten A1 - Bernd, Antje A1 - Birch, David G. A1 - Hamel, Christian P. A1 - Heckenlively, John R. A1 - Jacobson, Samuel G. A1 - Kamme, Christina A1 - Kellner, Ulrich A1 - Kunstmann, Erdmute A1 - Maffei, Pietro A1 - Reiff, Charlotte M. A1 - Rohrschneider, Klaus A1 - Rosenberg, Thomas A1 - Rudolph, Günther A1 - Vámos, Rita A1 - Varsányi, Balázs A1 - Weleber, Richard G. A1 - Wissinger, Bernd T1 - Mutation Detection in Patients with Retinal Dystrophies Using Targeted Next Generation Sequencing JF - PLoS ONE N2 - Retinal dystrophies (RD) constitute a group of blinding diseases that are characterized by clinical variability and pronounced genetic heterogeneity. The different nonsyndromic and syndromic forms of RD can be attributed to mutations in more than 200 genes. Consequently, next generation sequencing (NGS) technologies are among the most promising approaches to identify mutations in RD. We screened a large cohort of patients comprising 89 independent cases and families with various subforms of RD applying different NGS platforms. While mutation screening in 50 cases was performed using a RD gene capture panel, 47 cases were analyzed using whole exome sequencing. One family was analyzed using whole genome sequencing. A detection rate of 61% was achieved including mutations in 34 known and two novel RD genes. A total of 69 distinct mutations were identified, including 39 novel mutations. Notably, genetic findings in several families were not consistent with the initial clinical diagnosis. Clinical reassessment resulted in refinement of the clinical diagnosis in some of these families and confirmed the broad clinical spectrum associated with mutations in RD genes. KW - mutation detection KW - retinal dystrophies KW - next generation sequencing Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-167398 VL - 11 IS - 1 ER - TY - JOUR A1 - Weiss, H. A1 - Sebald, Walter A1 - Schwab, A. J. A1 - Kleinow, W. A1 - Lorenz, B. T1 - Contribution of mitochondrial and cytoplasmic protein synthesis to the formation of cytochrome b and cytochrome aa\(_3\) N2 - A cytochrome b preparation from Neurospora crassa mitochondria is found to consist of three polypeptides (apparent molecular weight 10 000, 11 000 and 32 000), a cytochrome aa3 preparation of six to seven polypeptides (apparent molecular weight 8 000, 11 000, 13 000, 18 000, 28 000 and 36 000). Selective incorporation of radioactive amino acids by eilher mitochondrial protein synthesis when the cytoplasmic one is blocked or by the cytoplasmic protein synthesis, when the mitochondrial one is blocked, indicates that one cytochrome b polypeptide (mw 32 000) and one to three cytochrome aa3 polypeptides (mw 36 000, 28 000 and 18 000) are mitochondrial translation products, the other cytochrome b and cytochrome aa3 polypeptides cytoplasmic translation products. The delayed appearance of labeling in the cytochrome b and cytochrome aa3 polypeptides compared to the average cell protein after a pulse of <~H leueine revealed that these polypeptides are derived from separate pools of precursor polypeptides. The pool sizes range from 2 p. cent to 25 p. cent of the amount of the corresponding polypeptide present in the cytochromes. The 32 000 molecular weight polypeptide of cytochrome band at least the 18 000 molecular weight polypeptide of cytochrome aa\(_3\) are mitochondrial translation products as well in the fungus Neurospora crassa as in the insect Locusta migratoria. So, despite the fact that the size of mitochondrial DNA and mitochondrial ribosomes is reduced in insects, the products have maintained their characteristics. KW - Biochemie Y1 - 1973 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-62835 ER - TY - JOUR A1 - Weiss, H. A1 - Sebald, Walter A1 - Bücher, T. T1 - Cycloheximide resistant incorporation of amino acids into a polypeptide of the cytochrome oxidase of Neurospora crassa N2 - Radioaetive leueine was ineorporated by N eurospora crassa mitoehondria in vivo in the presence of cyeloheximide. When the membrane protein of these mitochondria was ehromatographieally separated on oleyl polymethaerylie aeid resin, & nurober of fraetions were obtained whieh differ with respeet to their eontents of radioaetivity and eytoehromes. The highest speeifie radioaetivity was found in the fraction eontaining eytoehrome aa3• This fraetion proved to be a pure and enzymatically aetive cytoehrome oxidase. Its ratio of absorbanee at 280 nm (ox)/ 443 nm (red.) was 2.1. By means of sodium dodeeylsulfate gel-electrophoresis, this enzymewas separated into five polypeptides with molecular weights of 30000, 20000, 13000, 10000, and 8000. Only the polypeptide with the molecular weight 20000 displayed a high specific radioaetivity. KW - Biochemie Y1 - 1971 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-62866 ER - TY - JOUR A1 - Weiss, H. A1 - Sebald, Walter T1 - Purification of cytochrome oxidase from Neurospora crassa and other sources N2 - A chromatographic procedure 1 is described by means of which cytochrome oxidase has been purified from a variety of organisms including the fungus N eurospora crassa,2,3 the unicellular alga Po/ytoma mirum, 4 the insect Locusta migratoria ,5 the frog Xenopus muel/eri,4 and the mammal Rattus norwegicus. 4 This procedure can be used to equal effect for large-scale preparations, starting from grams of mitochondrial protein, or for small-scale preparations starting from milligrams. The cytochrome oxidase preparations from the different organisms are enzymically active. They show similar subunit compositions. KW - Biochemie Y1 - 1978 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-82082 ER - TY - JOUR A1 - Weiss, Esther A1 - Schlegel, Jan A1 - Terpitz, Ulrich A1 - Weber, Michael A1 - Linde, Jörg A1 - Schmitt, Anna-Lena A1 - Hünniger, Kerstin A1 - Marischen, Lothar A1 - Gamon, Florian A1 - Bauer, Joachim A1 - Löffler, Claudia A1 - Kurzai, Oliver A1 - Morton, Charles Oliver A1 - Sauer, Markus A1 - Einsele, Hermann A1 - Loeffler, Juergen T1 - Reconstituting NK Cells After Allogeneic Stem Cell Transplantation Show Impaired Response to the Fungal Pathogen Aspergillus fumigatus JF - Frontiers in Immunology N2 - Delayed natural killer (NK) cell reconstitution after allogeneic stem cell transplantation (alloSCT) is associated with a higher risk of developing invasive aspergillosis. The interaction of NK cells with the human pathogen Aspergillus (A.) fumigatus is mediated by the fungal recognition receptor CD56, which is relocated to the fungal interface after contact. Blocking of CD56 signaling inhibits the fungal mediated chemokine secretion of MIP-1α, MIP-1β, and RANTES and reduces cell activation, indicating a functional role of CD56 in fungal recognition. We collected peripheral blood from recipients of an allograft at defined time points after alloSCT (day 60, 90, 120, 180). NK cells were isolated, directly challenged with live A. fumigatus germ tubes, and cell function was analyzed and compared to healthy age and gender-matched individuals. After alloSCT, NK cells displayed a higher percentage of CD56\(^{bright}\)CD16\(^{dim}\) cells throughout the time of blood collection. However, CD56 binding and relocalization to the fungal contact side were decreased. We were able to correlate this deficiency to the administration of corticosteroid therapy that further negatively influenced the secretion of MIP-1α, MIP-1β, and RANTES. As a consequence, the treatment of healthy NK cells ex vivo with corticosteroids abrogated chemokine secretion measured by multiplex immunoassay. Furthermore, we analyzed NK cells regarding their actin cytoskeleton by Structured Illumination Microscopy (SIM) and flow cytometry and demonstrate an actin dysfunction of NK cells shown by reduced F-actin content after fungal co-cultivation early after alloSCT. This dysfunction remains until 180 days post-alloSCT, concluding that further actin-dependent cellular processes may be negatively influenced after alloSCT. To investigate the molecular pathomechansism, we compared CD56 receptor mobility on the plasma membrane of healthy and alloSCT primary NK cells by single-molecule tracking. The results were very robust and reproducible between tested conditions which point to a different molecular mechanism and emphasize the importance of proper CD56 mobility. KW - natural killer cell KW - stem cell transplantation KW - corticosteroids KW - CCL3 KW - CCL4 KW - CCL5 Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-212581 SN - 1664-3224 VL - 11 ER - TY - JOUR A1 - Weising, K. A1 - Fiala, Brigitte A1 - Ramloch, K. A1 - Kahl, K. A1 - Epplen, J. T. T1 - Olingonucleotide fingerprinting in angiosperms N2 - No abstract available Y1 - 1990 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-42884 ER - TY - THES A1 - Weisert, Nadine T1 - Characterization of telomere-associated proteins in \(Trypanosoma\) \(brucei\) T1 - Charakterisierung Telomer-assoziierter Proteine in \(Trypanosoma\) \(brucei\) N2 - The unicellular pathogen Trypanosoma brucei is the causative agent of African trypanosomiasis, an endemic disease prevalent in sub-Saharan Africa. Trypanosoma brucei alternates between a mammalian host and the tsetse fly vector. The extracellular parasite survives in the mammalian bloodstream by periodically exchanging their ˈvariant surface glycoproteinˈ (VSG) coat to evade the host immune response. This antigenic variation is achieved through monoallelic expression of one VSG variant from subtelomeric ˈbloodstream form expression sitesˈ (BES) at a given timepoint. During the differentiation from the bloodstream form (BSF) to the procyclic form (PCF) in the tsetse fly midgut, the stage specific surface protein is transcriptionally silenced and replaced by procyclins. Due to their subtelomeric localization on the chromosomes, VSG transcription and silencing is partly regulated by homologues of the mammalian telomere complex such as TbTRF, TbTIF2 and TbRAP1 as well as by ˈtelomere-associated proteinsˈ (TelAPs) like TelAP1. To gain more insights into transcription regulation of VSG genes, the identification and characterization of other TelAPs is critical and has not yet been achieved. In a previous study, two biochemical approaches were used to identify other novel TelAPs. By using ˈco-immunoprecipitationˈ (co-IP) to enrich possible interaction partners of TbTRF and by affinity chromatography using telomeric repeat oligonucleotides, a listing of TelAP candidates has been conducted. With this approach TelAP1 was identified as a novel component of the telomere complex, involved in the kinetics of transcriptional BES silencing during BSF to PCF differentiation. To gain further insights into the telomere complex composition, other previously enriched proteins were characterized through a screening process using RNA interference to deplete potential candidates. VSG expression profile changes and overall proteomic changes after depletion were analyzed by mass spectrometry. With this method, one can gain insights into the functions of the proteins and their involvement in VSG expression site regulation. To validate the interaction of proteins enriched by co-IP with TbTRF and TelAP1 and to identify novel interaction proteins, I performed reciprocal affinity purifications of the four most promising candidates (TelAP2, TelAP3, PPL2 and PolIE) and additionally confirmed colocalization of two candidates with TbTRF via immunofluorescence (TelAP2, TelAP3). TelAP3 colocalizes with TbTRF and potentially interacts with TbTRF, TbTIF2, TelAP1 and TelAP2, as well as with two translesion polymerases PPL2 and PolIE in BSF. PPL2 and PolIE seem to be in close contact to each other at the telomeric ends and fulfill different roles as only PolIE is involved in VSG regulation while PPL2 is not. TelAP2 was previously characterized to be associated with telomeres by partially colocalizing with TbTRF and cells show a VSG derepression phenotype when the protein was depleted. Here I show that TelAP2 interacts with the telomere-binding proteins TbTRF and TbTIF2 as well as with the telomere-associated protein TelAP1 in BSF and that TelAP2 depletion results in a loss of TelAP1 colocalization with TbTRF in BSF. In conclusion, this study demonstrates that characterizing potential TelAPs is effective in gaining insights into the telomeric complex's composition and its role in VSG regulation in Trypanosoma brucei. Understanding these interactions could potentially lead to new therapeutic targets for combatting African trypanosomiasis. N2 - Der einzellige Pathogen Trypanosoma brucei ist der Erreger der afrikanischen Trypanosomiasis, eine endemische Krankheit vertreten in der Sub-Sahara Zone Afrikas. Trypanosoma brucei wechselt zwischen einem Säugerwirt und dem Insektenvektor, der Tsetse-Fliege. Der im Blutstrom des Säugers vorkommende, extrazelluläre Parasit ändert seinen Oberflächenmantel bestehend aus dem ˈvariablen Oberflächenproteinˈ (VSG) in periodischen Abständen, um der Immunantwort des Wirtes auszuweichen. Diese antigenetische Variation wird durch die monoallelische Expression einer einzelnen VSG-Variante, lokalisiert auf den ˈBlutstromform Expressionsseitenˈ (BES), zu einem bestimmten Zeitpunkt erreicht. Diese stadienspezifischen Oberflächenproteine werden während der Differenzierung der ˈBlutstromformˈ (BSF) zur ˈprozyklischen Formˈ (PCF) im Mitteldarm der Tsetse-Fliege stillgelegt und durch Prozykline ersetzt. Wegen der subtelomeren Lokalisation wird die VSG Transkription und Stilllegung teilweise durch Homologe des Säuger Telomerkomplexes TbTRF, TbTIF2 und TbRAP1 als auch durch Telomer-assoziierte Proteine (TelAPs) wie TelAP1 reguliert. Um Einblicke in die Transkriptionsregulation der VSG Gene zu erhalten, ist die Identifikation und Charakterisierung anderer Telomer-assoziierter Proteine von großem Interesse. In einer vorherigen Studie wurden zwei komplementäre biochemische Versuchsansätze verwendet, um weitere neue TelAPs zu identifizieren. Es wurde eine ko-Immunpräzipitation (co-IP) durchgeführt, um mögliche Interaktionspartner von TbTRF zu identifizieren, sowie eine Affinitätschromatographie unter Verwendung telomerischen Wiederholungseinheiten. Hierdurch wurde eine Liste von potenziellen Kandidaten generiert. Mit diesem Ansatz wurde TelAP1 als neue Komponente des Telomerkomplexes identifiziert, welches an der Kinetik der transkriptionellen BES-Stilllegung während der Differenzierung von BSF zu PCF beteiligt ist. Um weitere Einblicke in die Zusammensetzung des Telomerkomplexes zu erhalten, wurden zuvor angereicherte Proteine durch einen Screening-Prozess unter Verwendung von RNA-Interferenz charakterisiert. Nach der Depletion von 21 Proteinen wurden massenspektrometrische Analysen der VSG Expressionsprofiländerungen sowie allgemeine Veränderungen des Proteomenprofils analysiert. Mit dieser Methode können Erkenntnisse über die Funktion der jeweiligen Proteine und ihrer Beteiligung an der Regulierung der antigenetischen Variation von T. brucei gewonnen werden. Um die Interaktionen von Proteinen zu validieren, welche bei den Co-Immunpräzipitationen mit TbTRF und TelAP1 angereichert wurden, habe ich eine reziproke Affinitätschromatographie mit vier der vielversprechendsten Kandidaten durchgeführt (TelAP2, TelAP3, PPL2 und PolIE). Zusätzlich bestätigte ich die Co-lokalisation von zwei Kandidaten mit TbTRF via Immunfluoreszenzaufnahmen (TelAP2, TelAP3). TelAP3 ko-lokalisiert mit TbTRF und TelAP1 und interagiert potenziell mit TbTRF, TbTIF2, TelAP1 und TelAP2 als auch mit den zwei Transläsionspolymerasen PPL2 und PolIE in BSF. PPL2 und PolIE stehen in engem Kontakt zueinander und nehmen an den Telomerenden unterschiedliche Funktionen ein, da nur PolIE an der VSG Regulation beteiligt ist. TelAP2 wurde in einer vorherigen Publikation als Telomer-assoziiertes Protein durch partielle Co-Lokalisation mit TbTRF identifiziert und Zellen zeigen nach der Depletion von TelAP2 eine Derepression von zuvor stillgelegten VSGs. In dieser Studie zeige ich, dass TelAP2 mit den Telomer-bindenden Proteinen TbTRF und TbTIF2 sowie mit dem telomerassoziierten Protein TelAP1 in BSF interagiert und dass die Depletion von TelAP2 zu dem Verlust der Co-Lokalisation von TelAP1 mit TbTRF in BSF führt. Zusammenfassend zeigt diese Studie, dass die Charakterisierung potenzieller TelAPs dazu beiträgt, Einblicke in die Zusammensetzung des Telomerkomplexes und dessen Rolle bei der VSG-Regulation in Trypanosoma brucei zu gewinnen. Das Verständnis dieser Interaktionen könnte möglicherweise zu neuen therapeutischen Ansatzpunkten zur Bekämpfung der afrikanischen Trypanosomiasis führen. KW - Telomer KW - Trypanosoma brucei KW - telomere-associated protein Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-352732 ER - TY - JOUR A1 - Weisenberger, Dieter A1 - Scheer, Ulrich A1 - Benavente, Ricardo T1 - The DNA topoisomerase I inhibitor camptothecin blocks postmitotic reformation of nucleoli in mammmalian cells N2 - No abstract available KW - Cytologie KW - Nucleolus-DNA KW - opoisomerase I KW - camptothecin KW - mitosis Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-41434 ER - TY - JOUR A1 - Weigel, U. A1 - Meyer, M. A1 - Sebald, Walter T1 - Mutant proteins of human interleukin 2. Renaturation yield, proliferative activity and receptor binding N2 - No abstract available KW - Biochemie Y1 - 1989 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-62543 ER - TY - THES A1 - Weidenmüller, Anja T1 - From individual behavior to collective structure T1 - Von individuellem Verhalten zu kollektiven Strukturen N2 - The social organization of insect colonies has long fascinated naturalists. One of the main features of colony organization is division of labor, whereby each member of the colony specializes in a subset of all tasks required for successful group functioning. The most striking aspect of division of labor is its plasticity: workers switch between tasks in response to external challenges and internal perturbations. The mechanisms underlying flexible division of labor are far from being understood. In order to comprehend how the behavior of individuals gives rise to flexible collective behavior, several questions need to be addressed: We need to know how individuals acquire information about their colony's current demand situation; how they then adjust their behavior according; and which mechanisms integrate dozens or thousands of insect into a higher-order unit. With these questions in mind I have examined two examples of collective and flexible behavior in social bees. First, I addressed the question how a honey bee colony controls its pollen collection. Pollen foraging in honey bees is precisely organized and carefully regulated according to the colony's needs. How this is achieved is unclear. I investigated how foragers acquire information about their colony's pollen need and how they then adjust their behavior. A detailed documentation of pollen foragers in the hive under different pollen need conditions revealed that individual foragers modulate their in-hive working tempo according to the actual pollen need of the colony: Pollen foragers slowed down and stayed in the hive longer when pollen need was low and spent less time in the hive between foraging trips when pollen need of their colony was high. The number of cells inspected before foragers unloaded their pollen load did not change and thus presumably did not serve as cue to pollen need. In contrast, the trophallactic experience of pollen foragers changed with pollen need conditions: trophallactic contacts were shorter when pollen need was high and the number and probability of having short trophallactic contacts increased when pollen need increased. Thus, my results have provided support for the hypothesis that trophallactic experience is one of the various information pathways used by pollen foragers to assess their colony's pollen need. The second example of collective behavior I have examined in this thesis is the control of nest climate in bumble bee colonies, a system differing from pollen collection in honey bees in that information about task need (nest climate parameters) is directly available to all workers. I have shown that an increase in CO2 concentration and temperature level elicits a fanning response whereas an increase in relative humidity does not. The fanning response to temperature and CO2 was graded; the number of fanning bees increased with stimulus intensity. Thus, my study has evidenced flexible colony level control of temperature and CO2. Further, I have shown that the proportion of total work force a colony invests into nest ventilation does not change with colony size. However, the dynamic of the colony response changes: larger colonies show a faster response to perturbations of their colony environment than smaller colonies. Thus, my study has revealed a size-dependent change in the flexible colony behavior underlying homeostasis. I have shown that the colony response to perturbations in nest climate is constituted by workers who differ in responsiveness. Following a brief review of current ideas and models of self-organization and response thresholds in insect colonies, I have presented the first detailed investigation of interindividual variability in the responsiveness of all workers involved in a collective behavior. My study has revealed that bumble bee workers evidence consistent responses to certain stimulus levels and differ in their response thresholds. Some consistently respond to low stimulus intensities, others consistently respond to high stimulus intensities. Workers are stimulus specialists rather than task specialists. Further, I have demonstrated that workers of a colony differ in two other parameters of responsiveness: response probability and fanning activity. Response threshold, response probability and fanning activity are independent parameters of individual behavior. Besides demonstrating and quantifying interindividual variability, my study has provided empirical support for the idea of specialization through reinforcement. Response thresholds of fanning bees decreased over successive trials. I have discussed the importance of interindividual variability for specialization and the collective control of nest climate and present a general discussion of self-organization and selection. This study contributes to our understanding of individual behavior and collective structure in social insects. A fascinating picture of social organization is beginning to emerge. In place of centralized systems of communication and information transmission, insect societies frequently employ mechanisms based upon self-organization. Self-organization promises to be an important and unifying principle in physical, chemical and biological systems. N2 - Ein besonderes Merkmal sozialer Insekten ist die Arbeitsteilung. Die Mitglieder einer Kolonie führen jeweils unterschiedliche Arbeiten aus und wechseln, je nach Bedarfslage der Kolonie, flexibel zwischen den verschiedenen Tätigkeiten. Die Mechanismen dieser flexiblen Arbeitsteilung sind bislang weitgehend unverstanden. Wie erfahren einzelne Arbeiterinnen welche Tätigkeiten gerade notwendig sind? Nach welchen Regeln ändern sie ihr Verhalten, wenn sich die Anforderungen an die Kolonie ändern? Wie wird das Verhalten vieler Einzelindividuen so koordiniert, daß die Kolonie als Ganzes sinnvoll auf eine sich verändernde Umwelt reagieren kann? In der vorliegenden Arbeit bin ich diesen Fragen an zwei unterschiedlichen Systemen nachgegangen. Im ersten Kapitel dieser Arbeit untersuchte ich die Regulation des Pollensammelns bei Honigbienen. Pollen ist für Honigbienen eine wichtige Proteinquelle zur Aufzucht der Brut. Sowohl die Menge an Brut als auch die bereits im Stock vorhanden Menge an Pollen beeinflußt die Sammelaktivität. Bislang ist unklar, wie die Sammelbienen Information über den Pollenbedarf ihrer Kolonie erhalten und wie sie ihr Verhalten dementsprechend ändern. Meine Versuche zeigten, daß Pollensammlerinnen ihr Arbeitstempo der aktuellen Bedarfslage anpassen: Ist der Pollenbedarf der Kolonie hoch, verbringen sie wenig Zeit im Stock, ist ausreichend Pollen vorhanden, gehen sie ihrer Sammeltätigkeit langsamer nach. Während ihres Aufenthalts im Stock haben die Sammlerinnen eine Vielzahl trophallaktischer Kontakte mit anderen Bienen. Die Anzahl solcher Kontakte änderte sich mit dem Pollenbedarf der Kolonie: Bei hohem Pollenbedarf sind die trophallaktischen Kontakte kürzer und die Anzahl sehr kurzer Kontakte hoch. Diese Ergebnisse unterstützen die Hypothese, daß Änderungen in der trophallaktischen Erfahrung eine wichtige Informationsquelle über den aktuellen Pollenbedarf einer Kolonie darstellen. Das zweite Beispiel flexibler Arbeitsteilung, welches ich in dieser Arbeit untersucht habe, ist die Regulation des Nestklimas in Hummelkolonien. Dieses System unterscheidet sich von dem oben dargestellten grundlegend, da Information über Änderungen im Bedarf an Arbeitskraft jedem Koloniemitglied zugänglich ist. Jedes Koloniemitglied im Nest kann direkt erfahren wie sich das Nestklima ändert. Ich konnte zeigen, daß Hummelkolonien auf einen Temperaturanstieg und eine Zunahme der Kohlendioxidkonzentration im Nest mit Ventilationsverhalten reagieren. Einzelne Hummeln fächeln dabei mit ihren Flügeln und sorgen so für Evaporationskühlung bzw. eine verstärkte Belüftung des Nestes. Erhöhte Luftfeuchtigkeit löste diese Reaktion nicht aus. Die Anzahl fächelnder Hummeln war abhängig von den Temperatur/CO2 Werten, die Kolonie reagierte fein abgestimmt auf die aktuellen Bedingungen. Unabhängig von ihrer Größe investierten die untersuchten Kolonien einen bestimmten Anteil ihrer Arbeiterinnen in die Ventilation des Nestes. Große Kolonien unterschieden sich jedoch von kleinen Kolonien in ihrer Antwortgeschwindigkeit: Große Kolonien antworten schneller auf einen Temperatur / CO2 Anstieg als kleine. Die flexible und fein abgestimmte Kolonieantwort auf Veränderungen im Nestklima basiert auf dem Verhalten vieler Einzelindividuen. Im dritten Kapitel dieser Arbeit stellte ich aktuelle Ideen und Hypothesen zu Selbstorganisation und dem Einfluß interindividueller Variabilität auf Kolonieverhalten dar. Regulation des Nestklimas in Hummelkolonien ist ein ideales System um interindividuelle Variabilität und ihre Auswirkungen zu untersuchen. Ich konnte zum ersten Mal Unterschiede im Antwortverhalten aller an einem kollektiven Verhalten beteiligten Koloniemitglieder quantifizieren. Neben Unterschieden in Antwortschwellen, die in der Literatur zwar viel diskutiert, aber noch nie schlüssig nachgewiesen wurden, konnte ich zeigen, daß sich Arbeiterinnen einer Kolonie in zwei weiteren Parametern unterscheiden: Die Wahrscheinlichkeit auf einen Stimulus zu reagieren und die Dauer, mit der die Arbeiterinnen das Verhalten ausführen (Aktivität) ist zwischen Individuen unterschiedlich. Diese drei Parameter (Reaktionsschwelle, Antwortwahrscheinlichkeit und Aktivität) sind vermutlich unabhängige Parameter individuellen Verhaltens. Neben diesen interindividuellen Unterschieden konnte ich nachweisen, daß sich die Antwortschwellen verändern, je häufiger eine Hummel fächelt: Arbeiterinnen reagieren von Mal zu Mal auf niedrigere Stimulusintensitäten. Diese Ergebnisse sind für unser Verständnis von Arbeitsteilung und Spezialisierung bei sozialen Insekten von besonderer Bedeutung. In dieser Arbeit habe ich sowohl das Verhalten individueller Arbeiterinnen als auch die daraus resultierende kollektive Antwort der Kolonie untersucht. Es wird zunehmend deutlicher, daß dem faszinierenden Verhalten sozialer Insekten häufig nicht zentrale Informationsverarbeitung sondern Selbstorganisation zugrunde liegt. KW - Hummeln KW - Soziale Insekten KW - Thermoregulation KW - Arbeitsteilung KW - Bienenstaat KW - Pollen KW - Sammeln KW - Arbeitsteilung KW - Pollen KW - Nestklima KW - Thermoregultion KW - CO2 KW - Antwortschwellen KW - Selbstorgansation KW - social organization KW - division of labor KW - pollen foraging KW - nest climate KW - thermoregulation KW - CO2 KW - response threshold models KW - self-organization Y1 - 2001 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-2448 ER - TY - JOUR A1 - Weich, H. A. A1 - Sebald, Walter A1 - Schairer, H. U. A1 - Hoppe, J. T1 - The human osteosarcoma cell line U-2 OS expresses a 3.8 kilobase mRNA which codes for the sequence of the PDGF-B chain N2 - A cDNA clone of about 2500 basepairswas prepared from the human osteosarcoma cellline U-2 OS by hybridizing with a v-sis probe. Sequence analysis showed that this cDNA contains the coding region for the PDGF-B chain. Here we report that the mitogen secreted by these osteosarcoma cells contains the PDGF-B chain and is probably a homodimer of two B-chains. KW - Biochemie KW - Platelet-derived growthfactor KW - cDNA KW - Oncogene KW - Tumor cell Y1 - 1986 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-62588 ER - TY - JOUR A1 - Wegert, Jenny A1 - Vokuhl, Christian A1 - Collord, Grace A1 - Del Castillo Velasco-Herrera, Martin A1 - Farndon, Sarah J. A1 - Guzzo, Charlotte A1 - Jorgensen, Mette A1 - Anderson, John A1 - Slater, Olga A1 - Duncan, Catriona A1 - Bausenwein, Sabrina A1 - Streitenberger, Heike A1 - Ziegler, Barbara A1 - Furtwängler, Rhoikos A1 - Graf, Norbert A1 - Stratton, Michael R. A1 - Campbell, Peter J. A1 - Jones, David TW A1 - Koelsche, Christian A1 - Pfister, Stefan M. A1 - Mifsud, William A1 - Sebire, Neil A1 - Sparber-Sauer, Monika A1 - Koscielniak, Ewa A1 - Rosenwald, Andreas A1 - Gessler, Manfred A1 - Behjati, Sam T1 - Recurrent intragenic rearrangements of EGFR and BRAF in soft tissue tumors of infants JF - Nature Communications N2 - Soft tissue tumors of infancy encompass an overlapping spectrum of diseases that pose unique diagnostic and clinical challenges. We studied genomes and transcriptomes of cryptogenic congenital mesoblastic nephroma (CMN), and extended our findings to five anatomically or histologically related soft tissue tumors: infantile fibrosarcoma (IFS), nephroblastomatosis, Wilms tumor, malignant rhabdoid tumor, and clear cell sarcoma of the kidney. A key finding is recurrent mutation of EGFR in CMN by internal tandem duplication of the kinase domain, thus delineating CMN from other childhood renal tumors. Furthermore, we identify BRAF intragenic rearrangements in CMN and IFS. Collectively these findings reveal novel diagnostic markers and therapeutic strategies and highlight a prominent role of isolated intragenic rearrangements as drivers of infant tumors. KW - cancer KW - genetics Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-233446 VL - 9 ER - TY - JOUR A1 - Wegert, Jenny A1 - Vokuh, Christian A1 - Ziegler, Barbara A1 - Ernestus, Karen A1 - Leuschner, Ivo A1 - Furtwängler, Rhoikos A1 - Graf, Norbert A1 - Gessler, Manfred T1 - TP53 alterations in Wilms tumour represent progression events with strong intratumour heterogeneity that are closely linked but not limited to anaplasia JF - The Journal of Pathology: Clinical Research N2 - TP53 mutations have been associated with anaplasia in Wilms tumour, which conveys a high risk for relapse and fatal outcome. Nevertheless, TP53 alterations have been reported in no more than 60% of anaplastic tumours, and recent data have suggested their presence in tumours that do not fulfil the criteria for anaplasia, questioning the clinical utility of TP53 analysis. Therefore, we characterized the TP53 status in 84 fatal cases of Wilms tumour, irrespective of histological subtype. We identified TP53 alterations in at least 90% of fatal cases of anaplastic Wilms tumour, and even more when diffuse anaplasia was present, indicating a very strong if not absolute coupling between anaplasia and deregulation of p53 function. Unfortunately, TP53 mutations do not provide additional predictive value in anaplastic tumours since the same mutation rate was found in a cohort of non-fatal anaplastic tumours. When classified according to tumour stage, patients with stage I diffuse anaplastic tumours still had a high chance of survival (87%), but this rate dropped to 26% for stages II–IV. Thus, volume of anaplasia or possible spread may turn out to be critical parameters. Importantly, among non-anaplastic fatal tumours, 26% had TP53 alterations, indicating that TP53 screening may identify additional cases at risk. Several of these non-anaplastic tumours fulfilled some criteria for anaplasia, for example nuclear unrest, suggesting that such partial phenotypes should be under special scrutiny to enhance detection of high-risk tumours via TP53 screening. A major drawback is that these alterations are secondary changes that occur only later in tumour development, leading to striking intratumour heterogeneity that requires multiple biopsies and analysis guided by histological criteria. In conclusion, we found a very close correlation between histological signs of anaplasia and TP53 alterations. The latter may precede development of anaplasia and thereby provide diagnostic value pointing towards aggressive disease. KW - tumour heterogeneity KW - Wilms tumour KW - nephroblastoma KW - anaplasia KW - TP53 Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-158302 VL - 3 ER - TY - JOUR A1 - Wegert, Jenny A1 - Bausenwein, Sabrina A1 - Kneitz, Susanne A1 - Roth, Sabine A1 - Graf, Norbert A1 - Geissinger, Eva A1 - Gessler, Manfred T1 - Retinoic acid pathway activity in Wilms tumors and characterization of biological responses in vitro N2 - Background: Wilms tumor (WT) is one of the most common malignancies in childhood. With current therapy protocols up to 90% of patients can be cured, but there is still a need to improve therapy for patients with aggressive WT and to reduce treatment intensity where possible. Prior data suggested a deregulation of the retinoic acid (RA) signaling pathway in high-risk WT, but its mode of action remained unclear. Results: The association of retinoid signaling and clinical parameters could be validated in a large independent tumor set, but its relevance in primary nephrectomy tumors from very young children may be different. Reduced RA pathway activity and MYCN overexpression were found in high risk tumors as opposed to tumors with low/ intermediate risk, suggesting a beneficial impact of RA especially on advanced WT. To search for possible modes of action of retinoids as novel therapeutic options, primary tumor cell cultures were treated in vitro with all-trans-RA (ATRA), 9cis-RA, fenretinide and combinations of retinoids and a histone deacetylase (HDAC) inhibitor. Genes deregulated in high risk tumors showed opposite changes upon treatment suggesting a positive effect of retinoids. 6/7 primary cultures tested reduced proliferation, irrespective of prior RA signaling levels. The only variant culture was derived from mesoblastic nephroma, a distinct childhood kidney neoplasm. Retinoid/HDAC inhibitor combinations provided no synergistic effect. ATRA and 9cis-RA induced morphological changes suggestive of differentiation, while fenretinide induced apoptosis in several cultures tested. Microarray analysis of ATRA treated WT cells revealed differential expression of many genes involved in extracellular matrix formation and osteogenic, neuronal or muscle differentiation. The effects documented appear to be reversible upon drug withdrawal, however. Conclusions: Altered retinoic acid signaling has been validated especially in high risk Wilms tumors. In vitro testing of primary tumor cultures provided clear evidence of a potential utility of retinoids in Wilms tumor treatment based on the analysis of gene expression, proliferation, differentiation and apoptosis. KW - Krebs KW - Wilms tumor KW - nephroblastoma KW - primary tumor cell culture KW - tumor model KW - retinoic acid Y1 - 2011 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-69137 ER - TY - JOUR A1 - Wegener, Christian A1 - Karsai, Gergely A1 - Pollák, Edit A1 - Wacker, Matthias A1 - Vömel, Matthias A1 - Selcho, Mareike A1 - Berta, Gergely A1 - Nachman, Ronald J. A1 - Isaac, R. Elwyn A1 - Molnár, László T1 - Diverse in- and output polarities and high complexity of local synaptic and non-synaptic signaling within a chemically defined class of peptidergic Drosophila neurons JF - Frontiers in Neural Circuits N2 - Peptidergic neurons are not easily integrated into current connectomics concepts, since their peptide messages can be distributed via non-synaptic paracrine signaling or volume transmission. Moreover, the polarity of peptidergic interneurons in terms of in- and out-put sites can be hard to predict and is very little explored. We describe in detail the morphology and the subcellular distribution of fluorescent vesicle/dendrite markers in CCAP neurons (NCCAP), a well defined set of peptidergic neurons in the Drosophila larva. NCCAP can be divided into five morphologically distinct subsets. In contrast to other subsets, serial homologous interneurons in the ventral ganglion show a mixed localization of in- and output markers along ventral neurites that defy a classification as dendritic or axonal compartments. Ultrastructurally, these neurites contain both pre- and postsynaptic sites preferably at varicosities. A significant portion of the synaptic events are due to reciprocal synapses. Peptides are mostly non-synaptically or parasynaptically released, and dense-core vesicles and synaptic vesicle pools are typically well separated. The responsiveness of the NCCAP to ecdysis-triggering hormone may be at least partly dependent on a tonic synaptic inhibition, and is independent of ecdysteroids. Our results reveal a remarkable variety and complexity of local synaptic circuitry within a chemically defined set of peptidergic neurons. Synaptic transmitter signaling as well as peptidergic paracrine signaling and volume transmission from varicosities can be main signaling modes of peptidergic interneurons depending on the subcellular region. The possibility of region-specific variable signaling modes should be taken into account in connectomic studies that aim to dissect the circuitry underlying insect behavior and physiology, in which peptidergic neurons act as important regulators. KW - synaptic signaling KW - volume transmission KW - paracrine release KW - neuromodulation KW - ecdysis KW - bursicon KW - CCAP KW - myoinhibitory peptide Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96914 ER - TY - JOUR A1 - Wegener, Christian A1 - Chen, Jiangtian T1 - Allatostatin A signalling: progress and new challenges from a paradigmatic pleiotropic invertebrate neuropeptide family JF - Frontiers in Physiology N2 - Neuropeptides have gained broad attraction in insect neuroscience and physiology, as new genetic tools are increasingly uncovering their wide-ranging pleiotropic functions with high cellular resolution. Allatostatin A (AstA) peptides constitute one of the best studied insect neuropeptide families. In insects and other panarthropods, AstA peptides qualify as brain-gut peptides and have regained attention with the discovery of their role in regulating feeding, growth, activity/sleep and learning. AstA receptor homologs are found throughout the protostomia and group with vertebrate somatostatin/galanin/kisspeptin receptors. In this review, we summarise the current knowledge on the evolution and the pleiotropic and cell-specific non-allatostatic functions of AstA. We speculate about the core functions of AstA signalling, and derive open questions and challengesfor future research on AstA and invertebrate neuropeptides in general. KW - neuropeptide signalling KW - feeding KW - intestinal control KW - sleep/activity KW - kisspeptin/galanin/spexin signalling KW - metabolism and growth KW - learning KW - cardioactive factor Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-278749 SN - 1664-042X VL - 13 ER - TY - JOUR A1 - Wech, Tobias A1 - Ankenbrand, Markus Johannes A1 - Bley, Thorsten Alexander A1 - Heidenreich, Julius Frederik T1 - A data-driven semantic segmentation model for direct cardiac functional analysis based on undersampled radial MR cine series JF - Magnetic Resonance in Medicine N2 - Purpose Image acquisition and subsequent manual analysis of cardiac cine MRI is time-consuming. The purpose of this study was to train and evaluate a 3D artificial neural network for semantic segmentation of radially undersampled cardiac MRI to accelerate both scan time and postprocessing. Methods A database of Cartesian short-axis MR images of the heart (148,500 images, 484 examinations) was assembled from an openly accessible database and radial undersampling was simulated. A 3D U-Net architecture was pretrained for segmentation of undersampled spatiotemporal cine MRI. Transfer learning was then performed using samples from a second database, comprising 108 non-Cartesian radial cine series of the midventricular myocardium to optimize the performance for authentic data. The performance was evaluated for different levels of undersampling by the Dice similarity coefficient (DSC) with respect to reference labels, as well as by deriving ventricular volumes and myocardial masses. Results Without transfer learning, the pretrained model performed moderately on true radial data [maximum number of projections tested, P = 196; DSC = 0.87 (left ventricle), DSC = 0.76 (myocardium), and DSC =0.64 (right ventricle)]. After transfer learning with authentic data, the predictions achieved human level even for high undersampling rates (P = 33, DSC = 0.95, 0.87, and 0.93) without significant difference compared with segmentations derived from fully sampled data. Conclusion A 3D U-Net architecture can be used for semantic segmentation of radially undersampled cine acquisitions, achieving a performance comparable with human experts in fully sampled data. This approach can jointly accelerate time-consuming cine image acquisition and cumbersome manual image analysis. KW - undersampling KW - cardiovascular magnetic resonance (CMR) KW - deep learning KW - radial KW - semantic segmentation Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-257616 VL - 87 IS - 2 ER -