TY - JOUR A1 - Rutkowski, Andrzej J. A1 - Erhard, Florian A1 - L'Hernault, Anne A1 - Bonfert, Thomas A1 - Schilhabel, Markus A1 - Crump, Colin A1 - Rosenstiel, Philip A1 - Efstathiou, Stacey A1 - Zimmer, Ralf A1 - Friedel, Caroline C. A1 - Dölken, Lars T1 - Widespread disruption of host transcription termination in HSV-1 infection JF - Nature Communications N2 - Herpes simplex virus 1 (HSV-1) is an important human pathogen and a paradigm for virus-induced host shut-off. Here we show that global changes in transcription and RNA processing and their impact on translation can be analysed in a single experimental setting by applying 4sU-tagging of newly transcribed RNA and ribosome profiling to lytic HSV-1 infection. Unexpectedly, we find that HSV-1 triggers the disruption of transcription termination of cellular, but not viral, genes. This results in extensive transcription for tens of thousands of nucleotides beyond poly(A) sites and into downstream genes, leading to novel intergenic splicing between exons of neighbouring cellular genes. As a consequence, hundreds of cellular genes seem to be transcriptionally induced but are not translated. In contrast to previous reports, we show that HSV-1 does not inhibit co-transcriptional splicing. Our approach thus substantially advances our understanding of HSV-1 biology and establishes HSV-1 as a model system for studying transcription termination. KW - herpes simplex virus KW - RNA polymerase II KW - gene expression KW - alpha-globin KW - motif discovery KW - regulatory protein ICP27 KW - poly(A) site usage KW - pre-messenger RNA KW - splicing inhibition KW - type 1 ICP27 Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-148643 VL - 6 IS - 7126 ER - TY - JOUR A1 - Seher, Axel A1 - Lagler, Charlotte A1 - Stühmer, Thorsten A1 - Müller-Richter, Urs Dietmar Achim A1 - Kübler, Alexander Christian A1 - Sebald, Walter A1 - Müller, Thomas Dieter A1 - Nickel, Joachim T1 - Utilizing BMP-2 muteins for treatment of multiple myeloma JF - PLoS ONE N2 - Multiple myeloma (MM) represents a haematological cancer characterized by the pathological hyper proliferation of antibody-producing B-lymphocytes. Patients typically suffer from kidney malfunction and skeletal disorders. In the context of MM, the transforming growth factor β (TGFβ) member Activin A was recently identified as a promoter of both accompanying symptoms. Because studies have shown that bone morphogenetic protein (BMP)-2-mediated activities are counteracted by Activin A, we analysed whether BMP2, which also binds to the Activin A receptors ActRII and ActRIIB but activates the alternative SMAD-1/5/8 pathway, can be used to antagonize Activin A activities, such as in the context of MM. Therefore three BMP2 derivatives were generated with modified binding activities for the type II (ActRIIB) and/or type I receptor (BMPRIA) showing either increased or decreased BMP2 activity. In the context of MM these BMP2 muteins show two functionalities since they act as a) an anti-proliferative/apoptotic agent against neoplastic B-cells, b) as a bone-formation promoting growth factor. The molecular basis of both activities was shown in two different cellular models to clearly rely on the properties of the investigated BMP2 muteins to compete for the binding of Activin A to the Activin type II receptors. The experimental outcome suggests new therapeutic strategies using BMP2 variants in the treatment of MM-related pathologies. KW - multiple myeloma KW - signaling KW - cell proliferation KW - cell binding KW - membrane receptor signaling KW - BMP KW - gene expression KW - B cell receptors KW - B cells Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-158144 VL - 12 IS - 5 ER - TY - THES A1 - Wu, Rongxue T1 - Treatment with integrin alpha v inhibitor abolishes compensatory cardiac hypertrophy due to altered signal transduction and ECM gene expression T1 - xxx N2 - Integrine sind Transmembranrezeptoren, welche mechanische Signale von der extrazellulären Matrix (ECM) zum Zytoskelett übermitteln ("outside-in-signaling"). Viele molekulare Defekte in der Verbindung zwischen Zytoskelett und ECM erzeugen bekanntermaßen Kardiomyopathien. alpha v Integrin scheint eine Hauptrolle in verschiedenen Prozessen der kardialen Reorganisation zu spielen, wie z.B. Regulation der Zellproliferation, -migration und -differenzierung. Unsere Hypothese war, dass alpha v -Integrin-vermittelte Signale notwendig für die kompensatorische Hypertrophie nach Aortenkonstriktion sind und assoziiert mit der Modulation der Expression von ECM-Proteinen. Dazu wurden Mäuse mit einem spezifischen alpha v Integrin-Inhibitor behandelt und einer Aortenkonstriktion (AB) unterzogen. Nach zwei Tagen und nach sieben Tagen wurden die Mäuse echokardiographisch untersucht und eingehende hämodynamische Untersuchungen wurden durchgeführt. Die Behandlung mit dem alpha v -Integrin-Inhibitor führte zu einer dilatativen Kardiomyopathie und Herzinsuffizienz in den AB-Mäusen, gekennzeichnet durch einen dilatierten linken Ventrikel, schlechte linksventrikuläre Funktion und einer Lungenstauung, wohingegen die scheinbehandelten Tiere eine kompensatorische Hypertrophie des linken Ventrikels zeigten. Untersuchungen der beteiligten Signalwege zeigten eine Aktivierung des p38 MAP-Kinase-Signalwegs, von ERK 1 und -2, der Focal Adhesion Kinase FAK und Tyrosin-Phosphorylierung von c-Src in den Kontrollherzen, was in den Inhibitor-behandelten Herzen fehlte. mRNA-Expressionsanalysen für 96 Gene mittels "Micro-Arrays" ermittelten verschiedene genomische Ziele des alpha v -Integrin-aktivierten Signalwegs. 18 für ECM-Proteine codierende Gene wurden mehr als 2-fach hochreguliert, z.B. Kollagen (8,11-fach ± 2,2), Fibronectin (2,32 ± 094), SPARC (3,78 ± 0,12), ADAMTS-1 (3,51 ± 0,81) und TIMP2 (2,23 ± 0,98), wohingegen die Aktivierung dieser Gene in Inhibitor-behandelten Tieren aufgehoben war. Wir folgern daraus, dass Signalwege unterhalb von alpha v -Integrin, mediiert durch MAP-Kinasen, FAK und c-Src, zu einer verstärkten Expression von ECM-Komponenten führt, welche für die kompensatorische Antwort auf Druckbelastung nötig sind. N2 - Integrins are transmembrane receptors transmitting mechanical signals from the extracellular matrix (ECM) to the cytoskeleton (outside-in-signaling). Many molecular defects in the link between cytoskeleton and ECM are known to induce cardiomyopathies. alpha v integrin appears to play a major role in several processes relevant to remodeling, such as binding and activation of matrix metalloproteinases as well as regulation of cell proliferation, migration, and differentiation. We hypothesized that alpha v integrin-mediated signaling is required for the compensatory hypertrophy after aortic banding (AB) and associated with the modulation of ECM protein expression. Mice were treated in vivo with a specific integrin alpha v inhibitor or vehicle via osmotic minipumps starting 1 day prior to aortic banding (AB). At day 2 and day 7 following AB or sham-operation, the mice were examined by echocardiography and hemodynamic analyses were performed. Treatment of alpha v Integrin inhibitor led to a dilated cardiomyopathy and congestive heart failure in AB mice (dilated left ventricle, depressed LV function, and pulmonary congestion), but not to hypertrophy as observed in mice without inhibitor treatment. Investigation of downstream signaling revealed significant activation of the p38 Mitogen-Activated Protein Kinase (MAPK), the Extracellular signal-Regulated Kinases 1 and 2 (Erk 1/2), Focal Adhesion Kinase (FAK) and tyrosine-phosphorylation of c-Src in mice 7 days after AB. This response was blunted in mice treated with integrin alpha v inhibitor. Microarrays probing for a total of 96 cell adhesion and ECM genes identified various genomic targets of integrin alpha v mediated signalling. 7 days after AB 18 ECM genes were up-regulated more than 2-fold (n=6), e.g. collagen (8.11 ± 2.2), fibronectin (2.32 ± 0.94), secreted protein, acidic and rich in cysteine (SPARC, 3.78 ± 0.12), A disintegrin-like and metalloprotease (reprolysin type) with trombospondin type 1 (Adamts-1, 3.51 ± 0.81) and Tissue inhibitor of metalloproteinase 2 (TIMP2, 2.23 ± 0.98), whereas this up-regulation was abolished in mice that were treatd by integrin alpha v inhibitor via mini pumps. We conclude that signaling downstream of integrin alpha v is mediated by the MAPK, FAK and c-Src pathways leading to an up-regulation of extracelluar matrix components necessary for the compensatory response of the heart under a condition of pressure overload. KW - Antigen KW - integrin alpha v KW - cardiac hypertrophy KW - signal transduction KW - ECM KW - gene expression KW - integrin alpha v KW - cardiac hypertrophy KW - signal transduction KW - ECM KW - gene expression Y1 - 2007 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-21339 ER - TY - JOUR A1 - Brodehl, Andreas A1 - Belke, Darrell D. A1 - Garnett, Lauren A1 - Martens, Kristina A1 - Abdelfatah, Nelly A1 - Rodriguez, Marcela A1 - Diao, Catherine A1 - Chen, Yong-Xiang A1 - Gordon, Paul M. K. A1 - Nygren, Anders A1 - Gerull, Brenda T1 - Transgenic mice overexpressing desmocollin-2 (DSC2) develop cardiomyopathy associated with myocardial inflammation and fibrotic remodeling JF - PLoS ONE N2 - Background Arrhythmogenic cardiomyopathy is an inherited heart muscle disorder leading to ventricular arrhythmias and heart failure, mainly as a result of mutations in cardiac desmosomal genes. Desmosomes are cell-cell junctions mediating adhesion of cardiomyocytes; however, the molecular and cellular mechanisms underlying the disease remain widely unknown. Desmocollin-2 is a desmosomal cadherin serving as an anchor molecule required to reconstitute homeostatic intercellular adhesion with desmoglein-2. Cardiac specific lack of desmoglein-2 leads to severe cardiomyopathy, whereas overexpression does not. In contrast, the corresponding data for desmocollin-2 are incomplete, in particular from the view of protein overexpression. Therefore, we developed a mouse model overexpressing desmocollin-2 to determine its potential contribution to cardiomyopathy and intercellular adhesion pathology. Methods and results We generated transgenic mice overexpressing DSC2 in cardiac myocytes. Transgenic mice developed a severe cardiac dysfunction over 5 to 13 weeks as indicated by 2D-echocardiography measurements. Corresponding histology and immunohistochemistry demonstrated fibrosis, necrosis and calcification which were mainly localized in patches near the epi- and endocardium of both ventricles. Expressions of endogenous desmosomal proteins were markedly reduced in fibrotic areas but appear to be unchanged in non-fibrotic areas. Furthermore, gene expression data indicate an early up-regulation of inflammatory and fibrotic remodeling pathways between 2 to 3.5 weeks of age. Conclusion Cardiac specific overexpression of desmocollin-2 induces necrosis, acute inflammation and patchy cardiac fibrotic remodeling leading to fulminant biventricular cardiomyopathy. KW - heart KW - mouse models KW - gene expression KW - fibrosis KW - inflammation KW - gene expression KW - genetically modified animals KW - cardiomyopathies KW - hyperexpression techniques Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-171084 VL - 12 IS - 3 ER - TY - JOUR A1 - Hickey, Scott F. A1 - Sridhar, Malathy A1 - Westermann, Alexander J. A1 - Qin, Qian A1 - Vijayendra, Pooja A1 - Liou, Geoffrey A1 - Hammond, Ming C. T1 - Transgene regulation in plants by alternative splicing of a suicide exon JF - Nucleic Acids Research N2 - Compared to transcriptional activation, other mechanisms of gene regulation have not been widely exploited for the control of transgenes. One barrier to the general use and application of alternative splicing is that splicing-regulated transgenes have not been shown to be reliably and simply designed. Here, we demonstrate that a cassette bearing a suicide exon can be inserted into a variety of open reading frames (ORFs), generating transgenes whose expression is activated by exon skipping in response to a specific protein inducer. The surprisingly minimal sequence requirements for the maintenance of splicing fidelity and regulation indicate that this splicing cassette can be used to regulate any ORF containing one of the amino acids Glu, Gln or Lys. Furthermore, a single copy of the splicing cassette was optimized by rational design to confer robust gene activation with no background expression in plants. Thus, conditional splicing has the potential to be generally useful for transgene regulation. KW - kingdom KW - pre-messenger RNA KW - gene expression KW - elements KW - decay KW - arabidopsis KW - eukaryotes KW - mechanisms Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-134724 VL - 40 IS - 10 ER - TY - JOUR A1 - Böhm, Jennifer A1 - Scherzer, Sönke A1 - Krol, Elzbieta A1 - Kreuzer, Ines A1 - von Meyer, Katharina A1 - Lorey, Christian A1 - Mueller, Thomas D. A1 - Shabala, Lana A1 - Monte, Isabel A1 - Solano, Roberto A1 - Al-Rasheid, Khaled A. S. A1 - Rennenberg, Heinz A1 - Shabala, Sergey A1 - Neher, Erwin A1 - Hedrich, Rainer T1 - The Venus flytrap Dionaea muscipula counts prey-induced action potentials to induce sodium uptake JF - Current Biology N2 - Carnivorous plants, such as the Venus flytrap (Dionaea muscipula), depend on an animal diet when grown in nutrient-poor soils. When an insect visits the trap and tilts the mechanosensors on the inner surface, action potentials (APs) are fired. After a moving object elicits two APs, the trap snaps shut, encaging the victim. Panicking preys repeatedly touch the trigger hairs over the subsequent hours, leading to a hermetically closed trap, which via the gland-based endocrine system is flooded by a prey-decomposing acidic enzyme cocktail. Here, we asked the question as to how many times trigger hairs have to be stimulated (e.g., now many APs are required) for the flytrap to recognize an encaged object as potential food, thus making it worthwhile activating the glands. By applying a series of trigger-hair stimulations, we found that the touch hormone jasmonic acid (JA) signaling pathway is activated after the second stimulus, while more than three APs are required to trigger an expression of genes encoding prey-degrading hydrolases, and that this expression is proportional to the number of mechanical stimulations. A decomposing animal contains a sodium load, and we have found that these sodium ions enter the capture organ via glands. We identified a flytrap sodium channel DmHKT1 as responsible for this sodium acquisition, with the number of transcripts expressed being dependent on the number of mechano-electric stimulations. Hence, the number of APs a victim triggers while trying to break out of the trap identifies the moving prey as a struggling Na\(^+\)-rich animal and nutrition for the plant. KW - jasmonic acid biosynthesis KW - gene expression KW - signal transduction KW - transporters KW - Arabidopsis Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-190870 VL - 26 IS - 3 ER - TY - JOUR A1 - Sander, Brigitta A1 - de Jong, Daphne A1 - Rosenwald, Andreas A1 - Xie, Wanling A1 - Balagué, Olga A1 - Calaminici, Maria A1 - Carreras, Joaquim A1 - Gaulard, Philippe A1 - Gribben, John A1 - Hagenbeek, Anton A1 - Kersten, Marie José A1 - Molina, Thierry Jo A1 - Lee, Abigail A1 - Montes-Moreno, Santiago A1 - Ott, German A1 - Raemaekers, John A1 - Salles, Gilles A1 - Sehn, Laurie A1 - Thorns, Christoph A1 - Wahlin, Bjorn E. A1 - Gascoyne, Randy D. A1 - Weller, Edie T1 - The reliability of immunohistochemical analysis of the tumor microenvironment in follicular lymphoma: a validation study from the Lunenburg Lymphoma Biomarker Consortium JF - Haematologica N2 - The cellular microenvironment in follicular lymphoma is of biological and clinical importance. Studies on the clinical significance of non-malignant cell populations have generated conflicting results, which may partly be influenced by poor reproducibility in immunohistochemical marker quantification. In this study, the reproducibility of manual scoring and automated microscopy based on a tissue microarray of 25 follicular lymphomas as compared to flow cytometry is evaluated. The agreement between manual scoring and flow cytometry was moderate for CD3, low for CD4, and moderate to high for CD8, with some laboratories scoring closer to the flow cytometry results. Agreement in manual quantification across the 7 laboratories was low to moderate for CD3, CD4, CD8 and FOXP3 frequencies, moderate for CD21, low for MIB1 and CD68, and high for CD10. Manual scoring of the architectural distribution resulted in moderate agreement for CD3, CD4 and CD8, and low agreement for FOXP3 and CD68. Comparing manual scoring to automated microscopy demonstrated that manual scoring increased the variability in the low and high frequency interval with some laboratories showing a better agreement with automated scores. Manual scoring reliably identified rare architectural patterns of T-cell infiltrates. Automated microscopy analyses for T-cell markers by two different instruments were highly reproducible and provided acceptable agreement with flow cytometry. These validation results provide explanations for the heterogeneous findings on the prognostic value of the microenvironment in follicular lymphoma. We recommend a more objective measurement, such as computer-assisted scoring, in future studies of the prognostic impact of microenvironment in follicular lymphoma patients. KW - CD/metabolism KW - flow cytometry KW - antigens KW - regulatory T-cells KW - independent predictor KW - gene expression KW - high numbers KW - CD40 ligand KW - Riutximab KW - survival KW - marcophages KW - transformation KW - in-vitro Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-116875 SN - 1592-8721 VL - 99 IS - 4 ER - TY - THES A1 - Zabka, Vanessa T1 - The Plasticity of Barley (Hordeum vulgare) Leaf Wax Characteristics and their Effects on Early Events in the Powdery Mildew Fungus (Blumeria graminis f.sp. hordei): Interactive Adaptations at the Physiological and the Molecular Level T1 - Die Plastizität von Blattwachsen der Gerste (Hordeum vulgare) und deren Effekte auf initiale Ereignisse der Mehltaukrankheit (Blumeria graminis f.sp. hordei): wechselseitige Anpassungen auf physiologischer und molekularer Ebene N2 - In order to test the effects of environmental factors on different characteristics of plant leaf waxes, barley plants (Hordeum vulgare) were abiotically stress treated (exposure to darkness, heavy metal, high salt concentrations and drought), and biotically stressed by the infection with powdery mildew (Blumeria graminis f.sp. hordei; Bgh). Different wax parameters like amount, chemical composition, and micromorphology of epicuticular wax crystals, were investigated. Etiolated leaves of barley showed distinctly reduced wax amounts and modifications in their relative composition. The alterations of these wax parameters might be a result of a developmental delay, which could have been caused by a decreased availability of energy for cellular processes, due to lack of light. Cadmium exposure led to a 1.5-fold increase of wax amount, while chemical composition was unaffected. In drought- and salt-stressed plants, all investigated leaf wax parameters remained unaltered. In each of the abiotic treatments, the microstructure of epicuticular wax crystals, formed as typical platelets, was not modified. Even after 6d infection with powdery mildew (Bgh), neither locally nor systemically enforced modifications of wax features were revealed. The analyzed leave surfaces, resulting from these four abiotic and the biotic treatment (phenotypic approach), were compared to altered leaf surfaces’ characteristics of 18 analyzed eceriferum (cer-) wax mutants (genotypic approach). Within the screening, 5 mutants were selected which distinctly differed from the wild-type in wax amount, portions of epi- and intracuticular wax fraction, relative chemical composition, crystal morphology, and surface wettability (hydrophobicity). Apart from quantitative and qualitative effects on the leaf waxes, environmentally enforced modifications in cuticular waxes might be reflected in molecular processes of wax biogenesis. Therefore, a barley wax-microarray was established. 254 genes were selected, which are putatively involved in processes of de novo fatty acid biosynthesis, fatty acid elongation, and modification, and which are supposed to take part in lipid-trafficking between cell compartments, and transport of wax components to the outer cell surface. The regulations within the expression pattern evoked by the respective treatments were correlated with the corresponding analytical wax data, and the observed molecular effects of a 3d powdery mildew infection were compared with succeeding fungal morphogenesis. Etiolation and cadmium exposition pointed to transcriptional modifications in the de novo fatty acid synthesis, and in the screened, transport-related mechanisms, which correlate with respective alterations in surface wax characteristics. Moderate changes in the gene expression pattern, evoked by drought- and salinity-stress, might give hints for evolved adaptations in barley to such common habitat stresses. Theinvasion of powdery mildew into the epidermal host cells was reflected in the regulation of several genes. Beside other functions, these genes take part in pathogen defense, and intracellular component transport, or they encode transcription factors. The different modifications within the molecular responses evoked by the investigated abiotic treatments, and the effects of powdery mildew infection representing a biotic stressor, were compared between the different treatments. In order to test the potential impact of different wax parameters on Bgh, conidia germination and differentiation was comparably investigated on leaf surfaces of abiotically stressed wild-type and cer-mutants, isolated cuticles, and further artificial surfaces. The rates of conidial development were similar on each of the leaf surfaces resulting from the abiotic treatments, while a significant reduction of the germination and differentiation success was revealed for the wax mutant cer-yp.949. Compared to the wild-type, developmental rates on isolated cuticles and extracted leaf waxes of the mutant cer-yp.949 indicated a modified embedding of cuticular waxes, and a possibly changed three-dimensional structure of the cer-yp.949 cuticle, which might explain the reduced conidial developmental rates on leaf surfaces of this particular mutant. Experiments with Bgh conidia on mechanically de-waxed leaf surfaces (selective mechanical removal of the epicuticular leaf waxes with glue-like gum arabic, followed by an extraction of the intracuticular wax portion with chloroform) demonstrated the importance of the wax coverage for the germination and differentiation of the fungal conidia. On all dewaxed leaf surfaces, except those of cer-yp.949, the differentiation success of the germlings was significantly reduced, by about 20% (“wax-effect”). This result was verified through an artificial system with increased conidia developmental rates on glass slides covered with extracted leaf waxes. Further comparative tests with the major components of barley leaf wax, hexacosanol and hexacosanal, showed that the germination and differentiation of powdery mildew conidia not only depends on the different chemistry, but is also influenced by the respective surface hydrophobicity. Compared to hexacosanol, on hexacosanal coated glass surfaces, higher germination and differentiation rates were achieved, which correlated with increased levels of surface hydrophobicity. Developmental rates of conidia on hydrophobic foils demonstrated that hydrophobicity, as a sole surface factor, may stimulate the conidial germination and differentiation processes. Moreover, the survival of conidia on artificial surfaces is determined by additional surface derived factors, e.g. the availability of water, and a pervadable matrix. N2 - Abiotische und biotische Umweltfaktoren können sowohl die Struktur als auch die chemischen Eigenschaften pflanzlicher Oberflächenwachse beeinflussen. In der vorliegenden Studie wurde vergleichend untersucht, inwiefern sich verschiedene Parameter von Gersten (Hordeum vulgare) Blattwachsen, wie deren Menge, chemische Zusammensetzung und die Morphologie epikutikulärer Wachskristalle unter dem Einfluss unterschiedlicher abiotischer Stressoren (Wachstum in Dunkelheit, Schwermetallbelastung, erhöhte Salzkonzentrationen, Trockenheit) und eines biotischen Stressors, dem Befall von Gerstenmehltau (Blumeria graminis fsp. hordei; Bgh), verändern können. Die Aufzucht ohne natürliches Licht führte zu etiolierten Blättern, die deutlich reduzierte Wachsmengen und quantitative Veränderungen in der Zusammensetzung einzelner Wachskomponenten zeigten. Die Veränderung dieser Wachscharakteristika könnte das Resultat einer pflanzlichen Entwicklungsverzögerung darstellen, die auf den Mangel an Licht, und damit einem Mangel an Energie für die zelluläre Triebkraft zurückzuführen ist. Cadmium-Belastung führte zu einer 1.5-fach erhöhten Wachsauflage der Versuchspflanzen bei unveränderter Chemie. Unter Trocken- und Salzstress zeigten sich keine Veränderungen der untersuchten Wachsparameter. Die plättchenförmige Kristallstruktur der epikutikulären Wachse blieb in jeder der untersuchten abiotischen Behandlungen unverändert. Um Auswirkungen von biotischem Stress auf die Wachsauflage zu testen, wurde eine Infektion mit Gerstenmehltau (Bgh) vorgenommen. Nach sechstägiger Pilzinfektion konnten hierbei weder lokale, noch systemische Veränderungen der unterschiedlichen Wachsparameter der Gerstenblätter detektiert werden. Zusätzlich zu solchen Blattoberflächen, die aus den vier abiotischen und der biotischen Behandlung resultierten (phänotypischer Ansatz), wurden die Oberflächenwachse von 18 cer-Wachsmutanten untersucht (genotypischer Ansatz). Hieraus wurden diejenigen fünf Mutanten ausgewählt, die die stärksten Abweichungen an Wachsmengen, Mengenverteilung zwischen epi- und intrakutikulärer Wachsfraktion und/ oder Anteilen der Einzelkomponenten, der Morphologie der epikutikulären Wachskristalle, und somit auch in der davon abhängenden Oberflächenbenetzbarkeit (Hydrophobizität) gegenüber dem Wildtyp aufwiesen. Um zu überprüfen, inwiefern sich die Modifizierung der Oberflächenwachse durch Umweltfaktoren in den zugrunde liegenden molekularen Prozessen der Wachsbiosynthese widerspiegelt, wurde ein Gerstenwachs-Microarray etabliert. Eine Auswahl von 254 Genen wurde zusammengestellt, denen potentiell Funktionen in der Fettsäurebiosynthese, Kettenverlängerung von Fettsäuren und deren Modifikation zu Wachskomponenten, sowie im Transport von Lipid- und Wachskomponenten zwischen den Zellkompartimenten zukommen. Die Veränderung der Expression einzelner Gene während der abiotischen Stress-Behandlungen wurde mit den Daten der Wachsanalyse dieser Behandlungen korreliert, sowie der Einfluss einer dreitägigen Mehltauinfektion auf molekulare Prozesse der Wirtspflanze mit der Pilzmorphogenese kombiniert. Hinweise auf transkriptionelle Veränderungen in der de novo Fettsäuresynthese und den untersuchten Transportmechanismen, die mit den Veränderungen der Oberflächenwachse korrelieren, waren insbesondere unter Cadmiumstress und durch Etiolierung zu verzeichnen. Die durch Trocken- und Salzstress verursachten, moderaten Veränderungen im Expressionsmuster untersuchter Gene könnten auf eine erworbene Toleranz von Gerste gegenüber solcher Art von Umweltstress hinweisen. Das Eindringen des Pilzes in die Epidermis spiegelte sich in zahlreichen Genregulierungen wider, die besonders der Pathogenabwehr und dem intrazellulären Komponententransport dienen, oder Transkriptionsfaktoren codieren. Der Einfluss der untersuchten abiotischen Faktoren und der Pilzbefall als biotischer Stressor lösten unterschiedliche Modifikationen der molekularen Antworten aus, die miteinander verglichen wurden. Um zu klären welche Wachsparameter die Auskeimung und Differenzierung der Konidien von B. graminis beeinflussen, wurden alle analysierten Blattoberflächen (abiotisch gestresster Wildtyp und cer-Mutanten) und weitere artifizielle Oberflächen in Biotests eingesetzt. Auf allen Blattoberflächen des abiotisch behandelten Wildtyps war die Konidienentwicklung gleichermaßen erfolgreich, während sich innerhalb des genotypischen Ansatzes eine signifikante Reduktion des Keimungs- und Differenzierungserfolgs auf Blättern der Mutante cer-yp.949 zeigte. Durch vergleichende Untersuchungen mit isolierten Kutikeln und extrahierten Blattwachsen von Wildtyp und der Mutante cer-yp.949 konnte gezeigt werden, dass der herabgesetzte Entwicklungserfolg der Konidien auf Blättern der Mutante cer-yp.949 auf eine modifizierte Einbettung der Wachse und eine veränderte dreidimensionale Struktur der cer-yp.949 Kutikula zurückzuführen sein könnte. Untersuchungen zur Entwicklung von Konidien auf sukzessiv entwachsten Blattoberflächen von Wildtyp und Mutanten (zunächst mechanisches Abheben der epikutikulären Wachskristalle durch Gummi arabicum, gefolgt von einer Extraktion der intrakutikulären Wachse mit Chloroform) zeigte die Bedeutung des Vorhandenseins von Wachs für die Auskeimung und Differenzierung der Konidien. Mit Ausnahme der Mutante cer-yp.949 wurde der Differenzierungserfolg der Konidien auf allen Blattflächen durch Wachsextraktion signifikant um ca. 20% reduziert („Wachseffekt“). Durch die Beschichtung von Glasobjektträgern mit extrahierten Blattwachsen konnte dieses Ergebnis auf ein artifizielles System übertragen und bestätigt werden. Zusätzliche Tests mit den Hauptkomponenten der Gerstenwachse Hexacosanol und Hexacosanal zeigten, dass Auskeimung und Differenzierung von Mehltau-Konidien von der unterschiedlichen Chemie, und auch von der Hydrophobizität der Oberfläche beeinflusst werden. Im Vergleich mit Hexacosanol zeigten Hexacosanal beschichtete Glasoberflächen sowohl den größten Keimungs- und Differenzierungserfolg, als auch die höchste Hydrophobizität. Entwicklungsraten auf hydrophoben Folien bestätigten, dass allein die Hydrophobizität der Oberfläche die Auskeimung und die Differenzierung der Konidien stimulieren kann. Das Überleben der Konidien auf artifiziellen Oberflächen wird darüber hinaus durch weitere Faktoren wie Wasserverfügbarkeit und eine durchdringbare Matrix bestimmt. KW - Mehltau KW - Gerstenkrankheit KW - Konidie KW - Keimung KW - Morphogenese KW - Wachs KW - Microarray KW - Differentielle Genexpression KW - powdery mildew desease KW - conidial differentiation KW - leaf wax analysis KW - microarray KW - wax biosynthesis KW - gene expression Y1 - 2008 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-26402 ER - TY - JOUR A1 - Schmidt, Marianne A1 - Skaf, Josef A1 - Gavril, Georgiana A1 - Polednik, Christine A1 - Roller, Jeanette A1 - Kessler, Michael A1 - Holzgrabe, Ulrike T1 - The influence of Osmunda regalis root extract on head and neck cancer cell proliferation, invasion and gene expression JF - BMC Complementary and Alternative Medicine N2 - Background: According to only a handful of historical sources, Osmunda regalis, the royal fern, has been used already in the middle age as an anti-cancer remedy. To examine this ancient cancer cure, an ethanolic extract of the roots was prepared and analysed in vitro on its effectiveness against head and neck cancer cell lines. Methods: Proliferation inhibition was measured with the MTT assay. Invasion inhibition was tested in a spheroid-based 3-D migration assay on different extracellular matrix surfaces. Corresponding changes in gene expression were analysed by qRT-PCR array. Induction of apoptosis was measured by fluorescence activated cell sorting (FACS) with the Annexin V binding method. The plant extract was analysed by preliminary phytochemical tests, liquid chromatography/mass spectroscopy (LC-MS) and thin layer chromatography (TLC). Anti-angiogenetic activity was determined by the tube formation assay. Results: O. regalis extract revealed a growth inhibiting effect on the head and neck carcinoma cell lines HLaC78 and FaDu. The toxic effect seems to be partially modulated by p-glycoprotein, as the MDR-1 expressing HLaC79-Tax cells were less sensitive. O. regalis extract inhibited the invasion of cell lines on diverse extracellular matrix substrates significantly. Especially the dispersion of the highly motile cell line HlaC78 on laminin was almost completely abrogated. Motility inhibition on laminin was accompanied by differential gene regulation of a variety of genes involved in cell adhesion and metastasis. Furthermore, O. regalis extract triggered apoptosis in HNSCC cell lines and inhibited tube formation of endothelial cells. Preliminary phytochemical analysis proved the presence of tannins, glycosides, steroids and saponins. Liquid chromatography/mass spectroscopy (LC-MS) revealed a major peak of an unknown substance with a molecular mass of 864.15 Da, comprising about 50% of the total extract. Thin layer chromatography identified ferulic acid to be present in the extract. Conclusion: The presented results justify the use of royal fern extracts as an anti-cancer remedy in history and imply a further analysis of ingredients. KW - head and neck carcinoma KW - invasion KW - plant extract KW - proliferation KW - HNSCC KW - metastasis KW - gene expression KW - Osmunda regalis Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-158704 VL - 17 IS - 518 ER - TY - JOUR A1 - Hyun, Tae Kyung A1 - van der Graaff, Eric A1 - Albacete, Alfonso A1 - Eom, Seung Hee A1 - Grosskinsky, Dominik K. A1 - Böhm, Hannah A1 - Janschek, Ursula A1 - Rim, Yeonggil A1 - Ali, Walid Wahid A1 - Kim, Soo Young A1 - Roitsch, Thomas T1 - The Arabidopsis PLAT Domain Protein1 is Critically Involved in Abiotic Stress Tolerance JF - PLOS ONE N2 - Despite the completion of the Arabidopsis genome sequence, for only a relatively low percentage of the encoded proteins experimental evidence concerning their function is available. Plant proteins that harbour a single PLAT (Polycystin, Lipoxygenase, Alpha-toxin and Triacylglycerol lipase) domain and belong to the PLAT-plant-stress protein family are ubiquitously present in monocot and dicots. However, the function of PLAT-plant-stress proteins is still poorly understood. Therefore, we have assessed the function of the uncharacterised Arabidopsis PLAT-plant-stress family members through a combination of functional genetic and physiological approaches. PLAT1 overexpression conferred increased abiotic stress tolerance, including cold, drought and salt stress, while loss-of-function resulted in opposite effects on abiotic stress tolerance. Strikingly, PLAT1 promoted growth under non-stressed conditions. Abiotic stress treatments induced PLAT1 expression and caused expansion of its expression domain. The ABF/ABRE transcription factors, which are positive mediators of abscisic acid signalling, activate PLAT1 promoter activity in transactivation assays and directly bind to the ABRE elements located in this promoter in electrophoretic mobility shift assays. This suggests that PLAT1 represents a novel downstream target of the abscisic acid signalling pathway. Thus, we showed that PLAT1 critically functions as positive regulator of abiotic stress tolerance, but also is involved in regulating plant growth, and thereby assigned a function to this previously uncharacterised PLAT domain protein. The functional data obtained for PLAT1 support that PLAT-plant-stress proteins in general could be promising targets for improving abiotic stress tolerance without yield penalty. KW - salicylic acid KW - gene expression KW - signal transduction KW - cold stress KW - salt stress KW - abscisic acid KW - endoplasmatic reticulum KW - transcription factors KW - pseudomonas syringae KW - plants response Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-114648 VL - 9 IS - 11 ER - TY - JOUR A1 - Weiste, Christoph A1 - Pedrotti, Lorenzo A1 - Selvanayagam, Jebasingh A1 - Muralidhara, Prathibha A1 - Fröschel, Christian A1 - Novák, Ondřej A1 - Ljung, Karin A1 - Hanson, Johannes A1 - Dröge-Laser, Wolfgang T1 - The Arabidopsis bZIP11 transcription factor links low-energy signalling to auxin-mediated control of primary root growth JF - PLoS Genetics N2 - Plants have to tightly control their energy homeostasis to ensure survival and fitness under constantly changing environmental conditions. Thus, it is stringently required that energy-consuming stress-adaptation and growth-related processes are dynamically tuned according to the prevailing energy availability. The evolutionary conserved SUCROSE NON-FERMENTING1 RELATED KINASES1 (SnRK1) and the downstream group C/S\(_{1}\) basic leucine zipper (bZIP) transcription factors (TFs) are well-characterised central players in plants’ low-energy management. Nevertheless, mechanistic insights into plant growth control under energy deprived conditions remains largely elusive. In this work, we disclose the novel function of the low-energy activated group S\(_{1}\) bZIP11-related TFs as regulators of auxin-mediated primary root growth. Whereas transgenic gain-of-function approaches of these bZIPs interfere with the activity of the root apical meristem and result in root growth repression, root growth of loss-of-function plants show a pronounced insensitivity to low-energy conditions. Based on ensuing molecular and biochemical analyses, we propose a mechanistic model, in which bZIP11-related TFs gain control over the root meristem by directly activating IAA3/SHY2 transcription. IAA3/SHY2 is a pivotal negative regulator of root growth, which has been demonstrated to efficiently repress transcription of major auxin transport facilitators of the PIN-FORMED (PIN) gene family, thereby restricting polar auxin transport to the root tip and in consequence auxin-driven primary root growth. Taken together, our results disclose the central low-energy activated SnRK1-C/S\(_{1}\)-bZIP signalling module as gateway to integrate information on the plant’s energy status into root meristem control, thereby balancing plant growth and cellular energy resources. KW - root growth KW - sucrose KW - auxins KW - meristems KW - regulator genes KW - genetically modified plants KW - gene expression KW - plant growth and development Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-157742 VL - 13 IS - 2 ER - TY - JOUR A1 - Lagler, Charlotte A1 - El-Mesery, Mohamed A1 - Kübler, Alexander Christian A1 - Müller-Richter, Urs Dietmar Achim A1 - Stühmer, Thorsten A1 - Nickel, Joachim A1 - Müller, Thomas Dieter A1 - Wajant, Harald A1 - Seher, Axel T1 - The anti-myeloma activity of bone morphogenetic protein 2 predominantly relies on the induction of growth arrest and is apoptosis-independent JF - PLoS ONE N2 - Multiple myeloma (MM), a malignancy of the bone marrow, is characterized by a pathological increase in antibody-producing plasma cells and an increase in immunoglobulins (plasmacytosis). In recent years, bone morphogenetic proteins (BMPs) have been reported to be activators of apoptotic cell death in neoplastic B cells in MM. Here, we use bone morphogenetic protein 2 (BMP2) to show that the "apoptotic" effect of BMPs on human neoplastic B cells is dominated by anti-proliferative activities and cell cycle arrest and is apoptosis-independent. The anti-proliferative effect of BMP2 was analysed in the human cell lines KMS12-BM and L363 using WST-1 and a Coulter counter and was confirmed using CytoTox assays with established inhibitors of programmed cell death (zVAD-fmk and necrostatin-1). Furthermore, apoptotic activity was compared in both cell lines employing western blot analysis for caspase 3 and 8 in cells treated with BMP2 and FasL. Additionally, expression profiles of marker genes of different cell death pathways were analysed in both cell lines after stimulation with BMP2 for 48h using an RT-PCR-based array. In our experiments we observed that there was rather no reduction in absolute cell number, but cells stopped proliferating following treatment with BMP2 instead. The time frame (48–72 h) after BMP2 treatment at which a reduction in cell number is detectable is too long to indicate a directly BMP2-triggered apoptosis. Moreover, in comparison to robust apoptosis induced by the approved apoptotic factor FasL, BMP2 only marginally induced cell death. Consistently, neither the known inhibitor of apoptotic cell death zVAD-fmk nor the necroptosis inhibitor necrostatin-1 was able to rescue myeloma cell growth in the presence of BMP2. KW - apoptosis KW - gene expression KW - necrotic cell death KW - multiple myeloma KW - cell metabolism KW - cell cycle and cell division KW - B cells Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-158993 VL - 12 IS - 10 ER - TY - JOUR A1 - Bocuk, Derya A1 - Wolff, Alexander A1 - Krause, Petra A1 - Salinas, Gabriela A1 - Bleckmann, Annalen A1 - Hackl, Christina A1 - Beissbarth, Tim A1 - Koenig, Sarah T1 - The adaptation of colorectal cancer cells when forming metastases in the liver: expression of associated genes and pathways in a mouse model JF - BMC Cancer N2 - Background: Colorectal cancer (CRC) is the second leading cause of cancer-related death in men and women. Systemic disease with metastatic spread to distant sites such as the liver reduces the survival rate considerably. The aim of this study was to investigate the changes in gene expression that occur on invasion and expansion of CRC cells when forming metastases in the liver. Methods: The livers of syngeneic C57BL/6NCrl mice were inoculated with 1 million CRC cells (CMT-93) via the portal vein, leading to the stable formation of metastases within 4 weeks. RNA sequencing performed on the Illumina platform was employed to evaluate the expression profiles of more than 14,000 genes, utilizing the RNA of the cell line cells and liver metastases as well as from corresponding tumour-free liver. Results: A total of 3329 differentially expressed genes (DEGs) were identified when cultured CMT-93 cells propagated as metastases in the liver. Hierarchical clustering on heat maps demonstrated the clear changes in gene expression of CMT-93 cells on propagation in the liver. Gene ontology analysis determined inflammation, angiogenesis, and signal transduction as the top three relevant biological processes involved. Using a selection list, matrix metallopeptidases 2, 7, and 9, wnt inhibitory factor, and chemokine receptor 4 were the top five significantly dysregulated genes. Conclusion: Bioinformatics assists in elucidating the factors and processes involved in CRC liver metastasis. Our results support the notion of an invasion-metastasis cascade involving CRC cells forming metastases on successful invasion and expansion within the liver. Furthermore, we identified a gene expression signature correlating strongly with invasiveness and migration. Our findings may guide future research on novel therapeutic targets in the treatment of CRC liver metastasis. KW - colorectal cancer (CRC) KW - RNA-sequencing KW - gene expression KW - liver metastasis Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-170853 VL - 17 IS - 342 ER - TY - THES A1 - Langjahr [verh. Held], Melissa T1 - Systemische Expression von Zytokinen bei schmerzhaften und schmerzlosen Polyneuropathien T1 - Systemic expression of cytokines in painful and painless polyneuropathies N2 - Die Pathophysiologie der PNP wie auch die Entstehung der oft assoziierten neuropathischen Schmerzen ist unklar. Gleichzeitig gibt es bislang keine geeigneten Biomarker, die die oft komplizierte Differentialdiagnose vereinfachen können. Einige Tiermodelle und klinische Studien lieferten bereits Hinweise auf die entscheidende Rolle pro- und anti-inflammatorischer Zytokine in diesen Prozessen. Ziel unserer Studie war es, die systemische Genexpression pro- und anti-inflammatorischer Zytokine in einer großen Kohorte von Patienten mit PNP verschiedener Ätiologie zu charakterisieren. Insgesamt konnten 111 PNP-Patienten und 38 gesunde Kontrollpersonen prospektiv rekrutiert werden. Nach Isolation von PBMC aus Blutproben von 97 Patienten wurde die Genexpression der pro-inflammatorischen Zytokine TNF, IL1, IL2, IL6, IL8 und der anti-inflammatorischen Zytokine IL4 und IL10 mittels qRT-PCR bestimmt. Bei 47 Patienten und 12 Kontrollen wurde zudem die IL6-, IL-8- und TNF-Zytokinproduktion von PBMC in vitro nach Stimulation durch LPS mittels ELISA untersucht. Hauptbefund war ein pro-inflammatorisches Zytokinprofil der PNP-Patienten mit höherer Genexpression von IL1, IL2, IL8 und TNF im Vergleich zu den gesunden Kontrollen. Im Falle der entzündlichen Neuropathien konnte zudem eine niedrigere Genexpression von IL10 im Vergleich zu Gesunden nachgewiesen werden. Sowohl schmerzhafte als auch schmerzlose Verlaufsformen wiesen ein pro-inflammatorisches Zytokingenexpressionsprofil im Vergleich zu Gesunden auf, das bei schmerzhaften PNP deutlich mehr beteiligte pro-inflammatorische Zytokine umfasste; relevante Unterschiede zwischen den PNP-Patienten mit und ohne Schmerz sowie der diagnostischen Subgruppen fanden sich nicht. Eine niedrigere Stimulationsschwelle der PBMC lag bei PNP-Patienten im Vergleich zu Gesunden nicht vor. Insgesamt erscheint die Rolle einzelner Zytokine als systemische Biomarker für die Differenzierung verschiedener PNP-Formen bzw. bezüglich neuropathischen Schmerzes aufgrund einer niedrigen Spezifität deutlich eingeschränkt. Dennoch sprechen unsere Ergebnisse für eine mögliche Rolle eines pro-inflammatorischen Milieus bei der Entstehung bzw. des Verlaufes verschiedener entzündlicher und nicht-entzündlicher Neuropathien und neuropathischen Schmerzes. N2 - Distinct cytokine expression patterns have been reported in biomaterial of patients with polyneuropathies (PNP). We investigated gene expression profiles of pro- and anti-inflammatory cytokines in peripheral blood mononuclear cells (PBMC) of patients with neuropathies of different etiologies. We prospectively studied 111 patients with neuropathies and compared data between diagnostic subgroups and healthy controls. Gene expression of a panel of pro- and anti-inflammatory cytokines was analyzed (interleukin-1 [IL-1], IL-2, IL-6, IL-8, and tumor necrosis factor-alpha [TNF], IL-4 and IL-10) in PBMC samples of 97 patients and 38 healthy controls. Furthermore, protein levels of IL-6, IL-8, and TNF were measured in supernatant of PBMC stimulated with lipopolysaccharide (LPS). PNP were associated with higher PBMC gene expression of IL-1 (p<0.05), IL-2 (p<0.05), IL-8 (p<0.001), and TNF (p<0.01) compared to healthy controls. Inflammatory neuropathies were associated with higher gene expression of IL-8 (p<0.001) and TNF (p<0.05) and lower gene expression of IL-10 (p<0.05) compared to healthy controls. More pro-inflammatory cytokines were elevated in painful neuropathy (IL-1, IL-2 [p<0.05], IL-8 [p<0.001] and TNF [p<0.05]) than in painless neuropathy (IL-8 [p<0.01] and TNF [p<0.01]) compared to healthy controls. Disease duration positively correlated with IL-6 gene expression (p<0.01). Supernatant protein levels of IL-6, IL-8, and TNF did not differ between groups. Conclusion: Systemic gene expression of pro-inflammatory cytokines is increased in patients with neuropathies and may be influenced by the presence of neuropathic pain. KW - Polyneuropathie KW - Cytokine KW - Genexpression KW - peripheral neuropathy KW - neuropathic pain KW - cytokine KW - gene expression KW - peripheral blood mononuclear cells KW - Neuropathischer Schmerz KW - Zytokine KW - Periphere mononukleäre Zellen Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-154445 ER - TY - JOUR A1 - Schneider, Johannes A1 - Klein, Teresa A1 - Mielich-Süss, Benjamin A1 - Koch, Gudrun A1 - Franke, Christian A1 - Kuipers, Oskar P. A1 - Kovács, Ákos T. A1 - Sauer, Markus A1 - Lopez, Daniel T1 - Spatio-temporal Remodeling of Functional Membrane Microdomains Organizes the Signaling Networks of a Bacterium JF - PLoS Genetics N2 - Lipid rafts are membrane microdomains specialized in the regulation of numerous cellular processes related to membrane organization, as diverse as signal transduction, protein sorting, membrane trafficking or pathogen invasion. It has been proposed that this functional diversity would require a heterogeneous population of raft domains with varying compositions. However, a mechanism for such diversification is not known. We recently discovered that bacterial membranes organize their signal transduction pathways in functional membrane microdomains (FMMs) that are structurally and functionally similar to the eukaryotic lipid rafts. In this report, we took advantage of the tractability of the prokaryotic model Bacillus subtilis to provide evidence for the coexistence of two distinct families of FMMs in bacterial membranes, displaying a distinctive distribution of proteins specialized in different biological processes. One family of microdomains harbors the scaffolding flotillin protein FloA that selectively tethers proteins specialized in regulating cell envelope turnover and primary metabolism. A second population of microdomains containing the two scaffolding flotillins, FloA and FloT, arises exclusively at later stages of cell growth and specializes in adaptation of cells to stationary phase. Importantly, the diversification of membrane microdomains does not occur arbitrarily. We discovered that bacterial cells control the spatio-temporal remodeling of microdomains by restricting the activation of FloT expression to stationary phase. This regulation ensures a sequential assembly of functionally specialized membrane microdomains to strategically organize signaling networks at the right time during the lifespan of a bacterium. KW - membrane proteins KW - gene expression KW - bacillus subtilis KW - fluorescence microscopy KW - cell fusion KW - signal transduction KW - gene regulation KW - lipids Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-125577 VL - 11 IS - 4 ER - TY - THES A1 - Kriegebaum, Claudia T1 - Spatio-temporal Expression Patterns of the Serotonin Synthesis Enzymes TPH1 and TPH2 and Effects of Acute Stress T1 - Regional-zeitliche Expressionsmuster der beiden Serotoninsynthese-Enzyme TPH1 und TPH2 und Effekte durch akuten Stress N2 - Several lines of evidence implicate a dysregulation of tryptophan hydroxylase (TPH)-dependent serotonin (5-HT) synthesis in emotions and stress and point to their potential relevance to the etiology and pathogenesis of various neuropsychiatric disorders. However, the differential expression pattern of the two isoforms TPH1 and TPH2 which encode two forms of the rate-limiting enzyme of 5-HT synthesis is controversial. Here, a comprehensive spatio-temporal analysis clarifies TPH1 and TPH2 expression during pre- and postnatal development of the mouse brain and in adult human brain as well as in peripheral organs including the pineal gland. Four different methods (real time PCR, in situ hybridization, immunohistochemistry and Western blot analysis) were performed to systematically control for tissue-, species- and isoform-specific expression on both the pre- and posttranslational level. TPH2 expression was consistently detected in the raphe nuclei, as well as in fibres in the deep pineal gland and in the gastrointestinal tract. Although TPH1 expression was found in these peripheral tissues, no significant TPH1 expression was detected in the brain, neither during murine development, nor in mouse and human adult brain. Also under conditions like stress and clearing the tissue from blood cells, no changes in expression levels were detectable. Furthermore, the reuptake of 5-HT into the presynaptic neuron by the serotonin transporter (SERT) is the major mechanism terminating the neurotransmitter signal. Thus, mice with a deletion in the Sert gene (Sert KO mice) provide an adequate model for human affective disorders to study lifelong modified 5-HT homeostasis in interaction with stressful life events. To further explore the role of TPH isoforms, Tph1 and Tph2 expression was studied in the raphe nuclei of Sert deficient mice under normal conditions as well as following exposure to acute immobilization stress. Interestingly, no statistically significant changes in expression were detected. Moreover, in comparison to Tph2, no relevant Tph1 expression was detected in the brain independent from genotype, gender and treatment confirming expression in data from native animals. Raphe neurons of a brain-specific Tph2 conditional knockout (cKO) model were completely devoid of Tph2-positive neurons and consequently 5-HT in the brain, with no compensatory activation of Tph1 expression. In addition, a time-specific Tph2 inducible (i) KO mouse provides a brain-specific knockdown model during adult life, resulting in a highly reduced number of Tph2-positive cells and 5-HT in the brain. Intriguingly, expression studies detected no obvious alteration in expression of 5-HT system-associated genes in these brain-specific Tph2 knockout and knockdown models. The findings on the one hand confirm the specificity of Tph2 in brain 5-HT synthesis across the lifespan and on the other hand indicate that neither developmental nor adult Tph2-dependent 5-HT synthesis is required for normal formation of the serotonergic system, although Tph1 does not compensate for the lack of 5-HT in the brain of Tph2 KO models. A further aim of this thesis was to investigate the expression of the neuropeptide oxytocin, which is primarily produced in the hypothalamus and released for instance in response to stimulation of 5-HT and selective serotonin reuptake inhibitors (SSRIs). Oxytocin acts as a neuromodulator within the central nervous system (CNS) and is critically involved in mediating pain modulation, anxiolytic-like effects and decrease of stress response, thereby reducing the risk for emotional disorders. In this study, the expression levels of oxytocin in different brain regions of interest (cortex, hippocampus, amygdala, hypothalamus and raphe nuclei) from female and male wildtype (WT) and Sert KO mice with or without exposure to acute immobilization stress were investigated. Results showed significantly higher expression levels of oxytocin in brain regions which are involved in the regulation of emotional stimuli (amygdala and hippocampus) of stressed male WT mice, whereas male Sert KO as well as female WT and Sert KO mice lack these stress-induced changes. These findings are in accordance with the hypothesis of oxytocin being necessary for protection against stress, depressive mood and anxiety but suggest gender-dependent differences. The lack of altered oxytocin expression in Sert KO mice also indicates a modulation of the oxytocin response by the serotonergic system and provides novel research perspectives with respect to altered response of Sert KO mice to stress and anxiety inducing stimuli. N2 - Durch zahlreiche Untersuchungen ist belegt, dass eine gestörte Tryptophan-Hydroxylase (TPH)-abhängige Serotonin (5-HT)-Synthese an einer veränderten emotionalen Reaktion sowie einer veränderten Stress-Antwort beteiligt ist und damit auch in der Ätiologie und Pathogenese psychischer Erkrankungen eine Rolle spielt. Dennoch werden nach wie vor die unterschiedlichen Expressionsmuster der beiden Isoformen TPH1 und TPH2, die für zwei Formen des Schrittmacherenzyms der 5-HT-Synthese kodieren, kontrovers diskutiert. Zentrales Anliegen dieser Arbeit ist daher eine Klärung der TPH1- und TPH2-Expression während der prä- und postnatalen Entwicklung des murinen Gehirns, sowie im adulten humanen Gehirn und in einigen peripheren Organen und der Zirbeldrüse. Durch die Verwendung von vier verschiedenen Methoden (Real time-PCR, In situ-Hybridisierung, Immunhistochemie und Westernblot-Analysen) wurde systematisch die Gewebs- und Isoform-spezifische Expression in Maus und Mensch auf prä- und posttranslationaler Ebene nachgewiesen. TPH2-Expression wurde Spezies-übergreifend in den Raphe-Kernen des Hirnstamms wie auch in Fasern zur Zirbeldrüse und im Gastrointestinaltrakt detektiert. Auch TPH1 konnte in diesen peripheren Organen (die Zirbeldrüse eingeschlossen) nachgewiesen werden, jedoch fand sich keine signifikante TPH1-Expression im Gehirn, weder während der Entwicklung des Maus-Gehirns noch im humanen und murinen adulten Gehirn. Auch durch veränderte Bedingungen wie der Entfernung von Blutzellen aus dem Gewebe oder der Anwendung von akutem Immobilisierungsstress konnte keine Änderung der Expression gemessen werden. Sert Knockout-Mäuse, stellen ein geeignetes Tiermodell für affektive Erkrankungen dar, insbesondere um eine lebenslang veränderte 5-HT-Homöostase in Verbindung mit belastenden Lebensereignissen zu untersuchen. Um die Bedeutung der TPH-Isoformen und deren korrekte Expression weiter zu untersuchen, wurde die Tph1- und Tph2-Expression in den Raphe-Kernen von Sert Knockout (KO)-Mäusen unter normalen Bedingungen und nach akutem Stress getestet. Interessanterweise konnten keine statistisch signifikanten Expressionsänderungen entdeckt werden. Mehr noch, relativ zu Tph2 konnte unabhängig von Behandlung, Geschlecht oder Genotyp keine relevante Tph1-Expression im Gehirn gemessen werden, was wiederum die Expressionsdaten aus nativen Tieren unterstützt. Die Raphe-Neurone eines Gehirn-spezifischen konditionalen Tph2 KO-Modells zeigten weder Tph2-positive Zellen noch 5-HT, wiesen aber auch keine kompensatorische Aktivierung der Tph1-Expression im Gehirn auf. Zusätzlich repräsentiert eine zeit-spezifische, induzierbare KO-Maus ein Gehirn-spezifisches Tph2 Knockdown-Modell ab dem Erwachsenenalter, das eine stark reduzierte Anzahl an Tph2-positiven Zellen und 5-HT im Gehirn aufweist. Expressionsuntersuchungen zeigten interessanterweise, dass diese Gehirn-spezifischen Tph2 Knockout- und Knockdown-Modelle keine sichtliche Änderung in der Expression von 5-HT-System-assoziierten Genen aufweisen. Diese Ergebnisse bestätigen zum einen, dass die 5-HT-Synthese im murinen Gehirn während der kompletten Lebensspanne ausschließlich durch Tph2 katalysiert wird und weisen außerdem darauf hin, dass eine Tph2-abhängige 5-HT-Synthese weder während der Entwicklung noch im Erwachsenalter für die Ausbildung eines normalen serotonergen Systems benötigt wird, obwohl Tph1 den Verlust des 5-HT-Vorkommens im Gehirn der Tph2 KO-Mäuse nicht kompensiert. Weiterhin beschäftigt sich diese Arbeit mit der Expression von Oxytocin, das hauptsächlich im Hypothalamus produziert. Oxytocin ist maßgeblich bei Angst-lösenden Effekten sowie einer verringerten Stressantwort beteiligt. In dieser Studie wurde die Expression von Oxytocin in verschiedenen Gehirnregionen (Cortex, Hippocampus, Amygdala, Hypothalamus und Raphe Nuclei) von weiblichen und männlichen Wildtyp- (WT) und Sert KO-Mäusen getestet, die entweder unter normalen Bedingungen gehalten wurden oder eine Stunde lang akutem Immobilisierungsstress ausgesetzt waren. Die Ergebnisse zeigten eine signifikant höhere Oxytocin-Expression in Gehirnregionen, die für die emotionale Reizverarbeitung zuständig sind (Amygdala und Hippocampus) in gestressten männlichen WT-Mäusen, während männliche Sert KO-Mäuse sowie weibliche WT- und Sert KO-Mäuse diese Stress-bedingten Unterschiede nicht aufwiesen. Diese Befunde sind im Einklang mit der Hypothese, dass Oxytocin eine schützende Rolle bei Stress, depressiver Stimmung und Angst übernimmt, weisen jedoch auf einen Geschlechterunterschied hin. Ferner legt das Fehlen einer veränderten Oxytocin-Expression in Sert KO-Mäusen eine Modulation der Oxytocin-Expression durch das serotonerge System nahe, was neue Forschungsperspektiven über eine veränderte Reaktion auf Stress und Angst-auslösende Reize in Sert KO-Mäusen eröffnet. KW - Serotonin KW - Neurotransmitter KW - Chemische Synthese KW - Stress KW - Enzym KW - Genexpression KW - Maus KW - serotonin KW - mouse KW - acute stress KW - gene expression KW - enzymatic synthesis Y1 - 2009 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-40839 ER - TY - JOUR A1 - Hamann, Catharina S. A1 - Bankmann, Julian A1 - Mora Maza, Hanna A1 - Kornhuber, Johannes A1 - Zoicas, Iulia A1 - Schmitt-Böhrer, Angelika T1 - Social fear affects limbic system neuronal activity and gene expression JF - International Journal of Molecular Sciences N2 - Social anxiety disorder (SAD) is a highly prevalent and comorbid anxiety disorder with rather unclear underlying mechanisms. Here, we aimed to characterize neurobiological changes occurring in mice expressing symptoms of social fear and to identify possible therapeutic targets for SAD. Social fear was induced via social fear conditioning (SFC), a validated animal model of SAD. We assessed the expression levels of the immediate early genes (IEGs) cFos, Fosl2 and Arc as markers of neuronal activity and the expression levels of several genes of the GABAergic, serotoninergic, oxytocinergic, vasopressinergic and neuropeptide Y (NPY)-ergic systems in brain regions involved in social behavior or fear-related behavior in SFC+ and SFC− mice 2 h after exposure to a conspecific. SFC+ mice showed a decreased number and density of cFos-positive cells and decreased expression levels of IEGs in the dorsal hippocampus. SFC+ mice also showed alterations in the expression of NPY and serotonin system-related genes in the paraventricular nucleus of the hypothalamus, basolateral amygdala, septum and dorsal raphe nucleus, but not in the dorsal hippocampus. Our results describe neuronal alterations occurring during the expression of social fear and identify the NPY and serotonergic systems as possible targets in the treatment of SAD. KW - social anxiety KW - fear expression KW - social avoidance KW - gene expression KW - Npy KW - Npyr1 KW - Npyr2 KW - Htr1a KW - Htr2a KW - Htr2c Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-284274 SN - 1422-0067 VL - 23 IS - 15 ER - TY - JOUR A1 - Kaya-Zeeb, Sinan A1 - Delac, Saskia A1 - Wolf, Lena A1 - Marante, Ana Luiza A1 - Scherf-Clavel, Oliver A1 - Thamm, Markus T1 - Robustness of the honeybee neuro-muscular octopaminergic system in the face of cold stress JF - Frontiers in Physiology N2 - In recent decades, our planet has undergone dramatic environmental changes resulting in the loss of numerous species. This contrasts with species that can adapt quickly to rapidly changing ambient conditions, which require physiological plasticity and must occur rapidly. The Western honeybee (Apis mellifera) apparently meets this challenge with remarkable success, as this species is adapted to numerous climates, resulting in an almost worldwide distribution. Here, coordinated individual thermoregulatory activities ensure survival at the colony level and thus the transmission of genetic material. Recently, we showed that shivering thermogenesis, which is critical for honeybee thermoregulation, depends on octopamine signaling. In this study, we tested the hypothesis that the thoracic neuro-muscular octopaminergic system strives for a steady-state equilibrium under cold stress to maintain endogenous thermogenesis. We can show that this applies for both, octopamine provision by flight muscle innervating neurons and octopamine receptor expression in the flight muscles. Additionally, we discovered alternative splicing for AmOARβ2. At least the expression of one isoform is needed to survive cold stress conditions. We assume that the thoracic neuro-muscular octopaminergic system is finely tuned in order to contribute decisively to survival in a changing environment. KW - honeybees KW - thermogenesis KW - cold stress KW - octopamine KW - octopamine receptors KW - gene expression Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-288753 SN - 1664-042X VL - 13 ER - TY - JOUR A1 - Irmer, Henriette A1 - Tarazona, Sonia A1 - Sasse, Christoph A1 - Olbermann, Patrick A1 - Loeffler, Jürgen A1 - Krappmann, Sven A1 - Conesa, Ana A1 - Braus, Gerhard H. T1 - RNAseq analysis of Aspergillus fumigatus in blood reveals a just wait and see resting stage behavior JF - BMC Genomics N2 - Background: Invasive aspergillosis is started after germination of Aspergillus fumigatus conidia that are inhaled by susceptible individuals. Fungal hyphae can grow in the lung through the epithelial tissue and disseminate hematogenously to invade into other organs. Low fungaemia indicates that fungal elements do not reside in the bloodstream for long. Results: We analyzed whether blood represents a hostile environment to which the physiology of A. fumigatus has to adapt. An in vitro model of A. fumigatus infection was established by incubating mycelium in blood. Our model allowed to discern the changes of the gene expression profile of A. fumigatus at various stages of the infection. The majority of described virulence factors that are connected to pulmonary infections appeared not to be activated during the blood phase. Three active processes were identified that presumably help the fungus to survive the blood environment in an advanced phase of the infection: iron homeostasis, secondary metabolism, and the formation of detoxifying enzymes. Conclusions: We propose that A. fumigatus is hardly able to propagate in blood. After an early stage of sensing the environment, virtually all uptake mechanisms and energy-consuming metabolic pathways are shut-down. The fungus appears to adapt by trans-differentiation into a resting mycelial stage. This might reflect the harsh conditions in blood where A. fumigatus cannot take up sufficient nutrients to establish self-defense mechanisms combined with significant growth. KW - Saccharomyces cerevisiae KW - cerebral aspergillosis KW - gene expression KW - Aspergillus fumigatus KW - iron homeostasis KW - invasive pulmonary aspergillosis KW - Candida albicans KW - cell wall KW - lysine biosynthesis KW - human pathogen KW - murine model KW - virulence KW - mRNA-Seq KW - transcriptome KW - human pathogenic fungi KW - secondary metabolite gene cluster KW - detoxification Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-151390 VL - 16 IS - 640 ER - TY - JOUR A1 - Reynolds, David A1 - Cliffe, Laura A1 - Förstner, Konrad U. A1 - Hon, Chung-Chau A1 - Siegel, T. Nicolai A1 - Sabatini, Robert T1 - Regulation of transcription termination by glucosylated hydroxymethyluracil, base J, in Leishmania major and Trypanosoma brucei JF - Nucleic Acids Research N2 - Base J, beta-d-glucosyl-hydroxymethyluracil, is an epigenetic modification of thymine in the nuclear DNA of flagellated protozoa of the order Kinetoplastida. J is enriched at sites involved in RNA polymerase ( RNAP) II initiation and termination. Reduction of J in Leishmania tarentolae via growth in BrdU resulted in cell death and indicated a role of J in the regulation of RNAP II termination. To further explore J function in RNAP II termination among kinetoplastids and avoid indirect effects associated with BrdU toxicity and genetic deletions, we inhibited J synthesis in Leishmania major and Trypanosoma brucei using DMOG. Reduction of J in L. major resulted in genome-wide defects in transcription termination at the end of polycistronic gene clusters and the generation of antisense RNAs, without cell death. In contrast, loss of J in T. brucei did not lead to genome-wide termination defects; however, the loss of J at specific sites within polycistronic gene clusters led to altered transcription termination and increased expression of downstream genes. Thus, J regulation of RNAP II transcription termination genome-wide is restricted to Leishmania spp., while in T. brucei it regulates termination and gene expression at specific sites within polycistronic gene clusters. KW - RNA-polymerase-II KW - variant surface glycoprotein KW - SWI2/SNF2-like protein KW - messenger RNA KW - polycistronic transcription KW - DNA glycosation KW - hela cells KW - gene expression KW - genome KW - 5-bromodeoxyuridine Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-117863 VL - 42 IS - 15 ER - TY - JOUR A1 - Zhang, Yi A1 - Lee, Chil-Woo A1 - Wehner, Nora A1 - Imdahl, Fabian A1 - Svetlana, Veselova A1 - Weiste, Christoph A1 - Dröge-Laser, Wolfgang A1 - Deeken, Rosalia T1 - Regulation of Oncogene Expression in T-DNA-Transformed Host Plant Cells JF - PLoS Pathogens N2 - Virulent Agrobacterium tumefaciens strains integrate their T-DNA into the plant genome where the encoded agrobacterial oncogenes are expressed and cause crown gall disease. Essential for crown gall development are IaaH (indole-3-acetamide hydrolase), IaaM (tryptophan monooxygenase) and Ipt (isopentenyl transferase), which encode enzymes for the biosynthesis of auxin (IaaH, IaaM) and cytokinin (Ipt). Although these oncogenes are well studied as the tumor-inducing principle, nothing is known about the regulation of oncogene expression in plant cells. Our studies show that the intergenic regions (IGRs) between the coding sequences (CDS) of the three oncogenes function as promoters in plant cells. These promoters possess a eukaryotic sequence organization and cis-regulatory elements for the binding of plant transcription factors. WRKY18, WRKY40, WRKY60 and ARF5 were identified as activators of the Ipt promoter whereas IaaH and IaaM is constitutively expressed and no transcription factor further activates their promoters. Consistent with these results, the wrky triple mutant plants in particular, develops smaller crown galls than wild-type and exhibits a reduced Ipt transcription, despite the presence of an intact ARF5 gene. WRKY40 and WRKY60 gene expression is induced by A. tumefaciens within a few hours whereas the ARF5 gene is transcribed later during crown gall development. The WRKY proteins interact with ARF5 in the plant nucleus, but only WRKY40 together with ARF5 synergistically boosts the activation of the Ipt promoter in an auxin-dependent manner. From our data, we propose that A. tumefaciens initially induces WRKY40 gene expression as a pathogen defense response of the host cell. The WRKY protein is recruited to induce Ipt expression, which initiates cytokinin-dependent host cell division. With increasing auxin levels triggered by ubiquitous expression of IaaH and IaaM, ARF5 is activated and interacts with WRKY40 to potentiate Ipt expression and balance cytokinin and auxin levels for further cell proliferation. KW - luminescence KW - oncogenes KW - agrobacterium tumefaciens KW - transcription factors KW - auxins KW - gene expression KW - cytokinins KW - plant cells Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-125256 VL - 11 IS - 1 ER - TY - JOUR A1 - Nguyen, Tu N. A1 - Müller, Laura S. M. A1 - Park, Sung Hee A1 - Siegel, T. Nicolai A1 - Günzl, Arthur T1 - Promoter occupancy of the basal class I transcription factor A differs strongly between active and silent VSG expression sites in Trypanosoma brucei JF - Nucleic Acid Research N2 - Monoallelic expression within a gene family is found in pathogens exhibiting antigenic variation and in mammalian olfactory neurons. Trypanosoma brucei, a lethal parasite living in the human bloodstream, expresses variant surface glycoprotein (VSG) from 1 of 15 bloodstream expression sites (BESs) by virtue of a multifunctional RNA polymerase I. The active BES is transcribed in an extranucleolar compartment termed the expression site body (ESB), whereas silent BESs, located elsewhere within the nucleus, are repressed epigenetically. The regulatory mechanisms, however, are poorly understood. Here we show that two essential subunits of the basal class I transcription factor A (CITFA) predominantly occupied the promoter of the active BES relative to that of a silent BES, a phenotype that was maintained after switching BESs in situ. In these experiments, high promoter occupancy of CITFA was coupled to high levels of both promoter-proximal RNA abundance and RNA polymerase I occupancy. Accordingly, fluorescently tagged CITFA-7 was concentrated in the nucleolus and the ESB. Because a ChIP-seq analysis found that along the entire BES, CITFA-7 is specifically enriched only at the promoter, our data strongly indicate that monoallelic BES transcription is activated by a mechanism that functions at the level of transcription initiation. KW - RNA-polymerase-I KW - blood-stream forms KW - acrican trypanosomes KW - gene expression KW - antigenic variation KW - ribosomal RNA KW - plasmodium falciparum KW - virulence genes KW - subunit KW - complex Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-117232 SN - 1362-4962 VL - 42 IS - 5 ER - TY - JOUR A1 - Naseem, Muhammad A1 - Kunz, Meik A1 - Dandekar, Thomas T1 - Probing the unknowns in cytokinin-mediated immune defense in Arabidopsis with systems biology approaches JF - Bioinformatics and Biology Insights N2 - Plant hormones involving salicylic acid (SA), jasmonic acid (JA), ethylene (Et), and auxin, gibberellins, and abscisic acid (ABA) are known to regulate host immune responses. However, plant hormone cytokinin has the potential to modulate defense signaling including SA and JA. It promotes plant pathogen and herbivore resistance; underlying mechanisms are still unknown. Using systems biology approaches, we unravel hub points of immune interaction mediated by cytokinin signaling in Arabidopsis. High-confidence Arabidopsis protein-protein interactions (PPI) are coupled to changes in cytokinin-mediated gene expression. Nodes of the cellular interactome that are enriched in immune functions also reconstitute sub-networks. Topological analyses and their specific immunological relevance lead to the identification of functional hubs in cellular interactome. We discuss our identified immune hubs in light of an emerging model of cytokinin-mediated immune defense against pathogen infection in plants. KW - plant hormones KW - systems biology KW - interaction networks KW - gene expression KW - cytokinin Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-120199 SN - 1177-9322 VL - 8 ER - TY - JOUR A1 - Schwerk, Christian A1 - Papandreou, Thalia A1 - Schuhmann, Daniel A1 - Nickol, Laura A1 - Borkowski, Julia A1 - Steinmann, Ulrike A1 - Quednau, Natascha A1 - Stump, Carolin A1 - Weiss, Christel A1 - Berger, Jürgen A1 - Wolburg, Hartwig A1 - Claus, Heike A1 - Vogel, Ulrich A1 - Ishikawa, Hiroshi A1 - Tenenbaum, Tobias A1 - Schroten, Horst T1 - Polar Invasion and Translocation of Neisseria meningitidis and Streptococcus suis in a Novel Human Model of the Blood-Cerebrospinal Fluid Barrier JF - PLoS One N2 - Acute bacterial meningitis is a life-threatening disease in humans. Discussed as entry sites for pathogens into the brain are the blood-brain and the blood-cerebrospinal fluid barrier (BCSFB). Although human brain microvascular endothelial cells (HBMEC) constitute a well established human in vitro model for the blood-brain barrier, until now no reliable human system presenting the BCSFB has been developed. Here, we describe for the first time a functional human BCSFB model based on human choroid plexus papilloma cells (HIBCPP), which display typical hallmarks of a BCSFB as the expression of junctional proteins and formation of tight junctions, a high electrical resistance and minimal levels of macromolecular flux when grown on transwell filters. Importantly, when challenged with the zoonotic pathogen Streptococcus suis or the human pathogenic bacterium Neisseria meningitidis the HIBCPP show polar bacterial invasion only from the physiologically relevant basolateral side. Meningococcal invasion is attenuated by the presence of a capsule and translocated N. meningitidis form microcolonies on the apical side of HIBCPP opposite of sites of entry. As a functionally relevant human model of the BCSFB the HIBCPP offer a wide range of options for analysis of disease-related mechanisms at the choroid plexus epithelium, especially involving human pathogens. KW - gene expression KW - plexus epithelial-cells KW - central-nervous-system KW - microvascular endothelial-cells KW - choroid-plexus KW - in vitro KW - brain barrier KW - tight junctions KW - meningococcal disease KW - bacterial meningitis Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-131459 VL - 7 IS - 1 ER - TY - JOUR A1 - Waller, Frank A1 - Mueller, Martin J. A1 - Pedrotti, Lorenzo T1 - Piriformospora indica Root Colonization Triggers Local and Systemic Root Responses and Inhibits Secondary Colonization of Distal Roots JF - PLoS ONE N2 - Piriformospora indica is a basidiomycete fungus colonizing roots of a wide range of higher plants, including crop plants and the model plant Arabidopsis thaliana. Previous studies have shown that P. indica improves growth, and enhances systemic pathogen resistance in leaves of host plants. To investigate systemic effects within the root system, we established a hydroponic split-root cultivation system for Arabidopsis. Using quantitative real-time PCR, we show that initial P. indica colonization triggers a local, transient response of several defense-related transcripts, of which some were also induced in shoots and in distal, non-colonized roots of the same plant. Systemic effects on distal roots included the inhibition of secondary P. indica colonization. Faster and stronger induction of defense-related transcripts during secondary inoculation revealed that a P. indica pretreatment triggers root-wide priming of defense responses, which could cause the observed reduction of secondary colonization levels. Secondary P. indica colonization also induced defense responses in distant, already colonized parts of the root. Endophytic fungi therefore trigger a spatially specific response in directly colonized and in systemic root tissues of host plants. KW - Arabidopsis thaliana KW - flowering plants KW - fungal spores KW - fungi KW - gene expression KW - marker genes KW - plant defenses KW - plant signaling Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96493 ER - TY - JOUR A1 - Tsai, Yu-Chen A1 - Grimm, Stefan A1 - Chao, Ju-Lan A1 - Wang, Shih-Chin A1 - Hofmeyer, Kerstin A1 - Shen, Jie A1 - Eichinger, Fred A1 - Michalopoulou, Theoni A1 - Yao, Chi-Kuang A1 - Chang, Chih-Hsuan A1 - Lin, Shih-Han A1 - Sun, Y. Henry A1 - Pflugfelder, Gert O. T1 - Optomotor-blind negatively regulates Drosophila eye development by blocking Jak/STAT signaling JF - PLoS ONE N2 - Organ formation requires a delicate balance of positive and negative regulators. In Drosophila eye development, wingless (wg) is expressed at the lateral margins of the eye disc and serves to block retinal development. The T-box gene optomotor-blind (omb) is expressed in a similar pattern and is regulated by Wg. Omb mediates part of Wg activity in blocking eye development. Omb exerts its function primarily by blocking cell proliferation. These effects occur predominantly in the ventral margin. Our results suggest that the primary effect of Omb is the blocking of Jak/STAT signaling by repressing transcription of upd which encodes the Jak receptor ligand Unpaired. KW - morphogenetic furrow progression KW - cell fate KW - compartment boundary KW - reporter gene KW - compound eye KW - gene expression KW - retinal differentiation KW - acts downstream KW - imaginal disk KW - glial cells Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-143577 VL - 10 IS - 3 ER - TY - JOUR A1 - Wang, Huiqiang A1 - Chen, Nanhai G. A1 - Minev, Boris R. A1 - Szalay, Aladar A. T1 - Oncolytic vaccinia virus GLV-1h68 strain shows enhanced replication in human breast cancer stem-like cells in comparison to breast cancer cells JF - Journal of Translational Medicine N2 - Background: Recent data suggest that cancer stem cells (CSCs) play an important role in cancer, as these cells possess enhanced tumor-forming capabilities and are responsible for relapses after apparently curative therapies have been undertaken. Hence, novel cancer therapies will be needed to test for both tumor regression and CSC targeting. The use of oncolytic vaccinia virus (VACV) represents an attractive anti-tumor approach and is currently under evaluation in clinical trials. The purpose of this study was to demonstrate whether VACV does kill CSCs that are resistant to irradiation and chemotherapy. Methods: Cancer stem-like cells were identified and separated from the human breast cancer cell line GI-101A by virtue of increased aldehyde dehydrogenase 1 (ALDH1) activity as assessed by the ALDEFLUOR assay and cancer stem cell-like features such as chemo-resistance, irradiation-resistance and tumor-initiating were confirmed in cell culture and in animal models. VACV treatments were applied to both ALDEFLUOR-positive cells in cell culture and in xenograft tumors derived from these cells. Moreover, we identified and isolated CD44\(^+\)CD24\(^+\)ESA\(^+\) cells from GI-101A upon an epithelial-mesenchymal transition (EMT). These cells were similarly characterized both in cell culture and in animal models. Results: We demonstrated for the first time that the oncolytic VACV GLV-1h68 strain replicated more efficiently in cells with higher ALDH1 activity that possessed stem cell-like features than in cells with lower ALDH1 activity. GLV-1h68 selectively colonized and eventually eradicated xenograft tumors originating from cells with higher ALDH1 activity. Furthermore, GLV-1h68 also showed preferential replication in CD44\(^+\)CD24\(^+\)ESA\(^+\) cells derived from GI-101A upon an EMT induction as well as in xenograft tumors originating from these cells that were more tumorigenic than CD44\(^+\)CD24\(^-\)ESA\(^+\) cells. Conclusions: Taken together, our findings indicate that GLV-1h68 efficiently replicates and kills cancer stem-like cells. Thus, GLV-1h68 may become a promising agent for eradicating both primary and metastatic tumors, especially tumors harboring cancer stem-like cells that are resistant to chemo and/or radiotherapy and may be responsible for recurrence of tumors. KW - tumors KW - therapy KW - metastasis KW - identification KW - lines KW - gene expression KW - in-vitro propagation KW - acute myeloid leukemia KW - epithelial-mesenchymal transition KW - subpopulation Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-130019 VL - 10 IS - 167 ER - TY - JOUR A1 - Fetiva, Maria Camila A1 - Liss, Franziska A1 - Gertzmann, Dörthe A1 - Thomas, Julius A1 - Gantert, Benedikt A1 - Vogl, Magdalena A1 - Sira, Nataliia A1 - Weinstock, Grit A1 - Kneitz, Susanne A1 - Ade, Carsten P. A1 - Gaubatz, Stefan T1 - Oncogenic YAP mediates changes in chromatin accessibility and activity that drive cell cycle gene expression and cell migration JF - Nucleic Acids Research N2 - YAP, the key protein effector of the Hippo pathway, is a transcriptional co-activator that controls the expression of cell cycle genes, promotes cell growth and proliferation and regulates organ size. YAP modulates gene transcription by binding to distal enhancers, but the mechanisms of gene regulation by YAP-bound enhancers remain poorly understood. Here we show that constitutive active YAP5SA leads to widespread changes in chromatin accessibility in untransformed MCF10A cells. Newly accessible regions include YAP-bound enhancers that mediate activation of cycle genes regulated by the Myb-MuvB (MMB) complex. By CRISPR-interference we identify a role for YAP-bound enhancers in phosphorylation of Pol II at Ser5 at MMB-regulated promoters, extending previously published studies that suggested YAP primarily regulates the pause-release step and transcriptional elongation. YAP5SA also leads to less accessible ‘closed’ chromatin regions, which are not directly YAP-bound but which contain binding motifs for the p53 family of transcription factors. Diminished accessibility at these regions is, at least in part, a consequence of reduced expression and chromatin-binding of the p53 family member ΔNp63 resulting in downregulation of ΔNp63-target genes and promoting YAP-mediated cell migration. In summary, our studies uncover changes in chromatin accessibility and activity that contribute to the oncogenic activities of YAP. KW - oncogenic YAP KW - chromatin KW - cell cycle KW - gene expression KW - cell migration KW - YAP5SA Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-350218 VL - 51 IS - 9 ER - TY - JOUR A1 - Mueller, Kerstin A1 - Quandt, Jasmin A1 - Marienfeld, Ralf B. A1 - Weihrich, Petra A1 - Fiedler, Katja A1 - Claussnitzer, Melina A1 - Laumen, Helmut A1 - Vaeth, Martin A1 - Berberich-Siebelt, Frederike A1 - Serfling, Edgar A1 - Wirth, Thomas A1 - Brunner, Cornelia T1 - Octamer-dependent transcription in T cells is mediated by NFAT and \(NF-\kappa B\) JF - Nucleic Acids Research N2 - The transcriptional co-activator BOB.1/OBF.1 was originally identified in B cells and is constitutively expressed throughout B cell development. BOB.1/OBF.1 associates with the transcription factors Oct1 and Oct2, thereby enhancing octamer-dependent transcription. In contrast, in T cells, BOB.1/OBF.1 expression is inducible by treatment of cells with PMA/Ionomycin or by antigen receptor engagement, indicating a marked difference in the regulation of BOB.1/OBF.1 expression in B versus T cells. The molecular mechanisms underlying the differential expression of BOB.1/OBF.1 in T and B cells remain largely unknown. Therefore, the present study focuses on mechanisms controlling the transcriptional regulation of BOB.1/OBF.1 and Oct2 in T cells. We show that both calcineurin- and \(NF-\kappa B\)-inhibitors efficiently attenuate the expression of BOB.1/OBF.1 and Oct2 in T cells. In silico analyses of the BOB.1/OBF.1 promoter revealed the presence of previously unappreciated combined NFAT/\(NF-\kappa B\) sites. An array of genetic and biochemical analyses illustrates the involvement of the \(Ca^{2+}\)/calmodulin-dependent phosphatase calcineurin as well as NFAT and \(NF-\kappa B\) transcription factors in the transcriptional regulation of octamer-dependent transcription in T cells. Conclusively, impaired expression of BOB.1/OBF.1 and Oct2 and therefore a hampered octamer-dependent transcription may participate in T cell-mediated immunodeficiency caused by the deletion of NFAT or \(NF-\kappa B\) transcription factors. KW - germinal center formation KW - OBF-1 OCA-B KW - coactivator OBF-1 KW - gene expression KW - functional characterization KW - immunoglobulin promoters KW - OCT-1-deficient mice KW - embryonic lethality KW - endothelial cells KW - murine homolog Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-123280 SN - 1362-4962 VL - 41 IS - 4 ER - TY - JOUR A1 - Garcia, Tzintzuni I. A1 - Matos, Isa A1 - Shen, Yingjia A1 - Pabuwal, Vagmita A1 - Coelho, Maria Manuela A1 - Wakamatsu, Yuko A1 - Schartl, Manfred A1 - Walter, Ronald B. T1 - Novel Method for Analysis of Allele Specific Expression in Triploid Oryzias latipes Reveals Consistent Pattern of Allele Exclusion JF - PLOS ONE N2 - Assessing allele-specific gene expression (ASE) on a large scale continues to be a technically challenging problem. Certain biological phenomena, such as X chromosome inactivation and parental imprinting, affect ASE most drastically by completely shutting down the expression of a whole set of alleles. Other more subtle effects on ASE are likely to be much more complex and dependent on the genetic environment and are perhaps more important to understand since they may be responsible for a significant amount of biological diversity. Tools to assess ASE in a diploid biological system are becoming more reliable. Non-diploid systems are, however, not uncommon. In humans full or partial polyploid states are regularly found in both healthy (meiotic cells, polynucleated cell types) and diseased tissues (trisomies, non-disjunction events, cancerous tissues). In this work we have studied ASE in the medaka fish model system. We have developed a method for determining ASE in polyploid organisms from RNAseq data and we have implemented this method in a software tool set. As a biological model system we have used nuclear transplantation to experimentally produce artificial triploid medaka composed of three different haplomes. We measured ASE in RNA isolated from the livers of two adult, triploid medaka fish that showed a high degree of similarity. The majority of genes examined (82%) shared expression more or less evenly among the three alleles in both triploids. The rest of the genes (18%) displayed a wide range of ASE levels. Interestingly the majority of genes (78%) displayed generally consistent ASE levels in both triploid individuals. A large contingent of these genes had the same allele entirely suppressed in both triploids. When viewed in a chromosomal context, it is revealed that these genes are from large sections of 4 chromosomes and may be indicative of some broad scale suppression of gene expression. KW - RNA-SEQ data KW - copy-number alteration KW - squalius alburnoides KW - gene expression KW - medaka KW - variant detection KW - transplantation KW - genome KW - generation KW - evolution Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-116000 SN - 1932-6203 VL - 9 IS - 6 ER - TY - JOUR A1 - Scognamiglio, Roberta A1 - Cabezas-Wallscheid, Nina A1 - Thier, Marc Christian A1 - Altamura, Sandro A1 - Reyes, Alejandro A1 - Prendergast, Áine M. A1 - Baumgärtner, Daniel A1 - Carnevalli, Larissa S. A1 - Atzberger, Ann A1 - Haas, Simon A1 - von Paleske, Lisa A1 - Boroviak, Thorsten A1 - Wörsdörfer, Philipp A1 - Essers, Marieke A. G. A1 - Kloz, Ulrich A1 - Eisenman, Robert N. A1 - Edenhofer, Frank A1 - Bertone, Paul A1 - Huber, Wolfgang A1 - van der Hoeven, Franciscus A1 - Smith, Austin A1 - Trumpp, Andreas T1 - Myc depletion induces a pluripotent dormant state mimicking diapause JF - Cell N2 - Mouse embryonic stem cells (ESCs) are maintained in a naive ground state of pluripotency in the presence of MEK and GSK3 inhibitors. Here, we show that ground-state ESCs express low Myc levels. Deletion of both c-myc and N-myc (dKO) or pharmacological inhibition of Myc activity strongly decreases transcription, splicing, and protein synthesis, leading to proliferation arrest. This process is reversible and occurs without affecting pluripotency, suggesting that Myc-depleted stem cells enter a state of dormancy similar to embryonic diapause. Indeed, c-Myc is depleted in diapaused blastocysts, and the differential expression signatures of dKO ESCs and diapaused epiblasts are remarkably similar. Following Myc inhibition, pre-implantation blastocysts enter biosynthetic dormancy but can progress through their normal developmental program after transfer into pseudo-pregnant recipients. Our study shows that Myc controls the biosynthetic machinery of stem cells without affecting their potency, thus regulating their entry and exit from the dormant state. KW - hematopoietic stem cells KW - leukemia inhibitory factor KW - c-Myc KW - N-Myc KW - gene expression KW - embryonic stem cells KW - self-renewal KW - protein synthesis Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-190868 VL - 164 IS - 4 ER - TY - THES A1 - El-Barkani, Abdelmalic T1 - Molekulargenetische Charakterisierung des pH-regulierten Dimorphismus und der pH-abhängigen Genexpression von Candida albicans und Entwicklung eines Reportersystem für Candida glabrata T1 - Molecular genetic Characterisation of the pH Regulated Dimorphism and the pH Dependent Gene Expression of Candida albicans and Development of a Reporter System for Candida glabrata N2 - Candida albicans ist in der Lage seine Zellmorphologie in Abhängigkeit von Umweltfaktoren zu verändern (Odds, 1988). Dieser morphologische Formenwechsel ist ein wesentlicher Pathogenitätsfaktor von C. albicans. Der pH-Wert gehört zu den wichtigen Umweltfaktoren, welche die Zellmorphologie von C. albicans beeinflussen. Bei sauren pH-Werten wächst C. albicans als unizellulärer Sprosspilz, während bei neutralen pH-Werten und einer Umgebungstemperatur von 37°C die filamentöse Form dominiert (Buffo et al., 1984). C. albicans reagiert auf unterschiedliche pH-Werte mit der differentiellen Expression bestimmter Gene. Zu diesen gehören die funktional homologen Gene PHR1 und PHR2, deren Genprodukte an der Synthese der Pilzzellwand beteiligt sind. PHR1 wird im neutralen Milieu induziert, während PHR2 im sauren Milieu exprimiert wird. Die Deletion von PHR1 oder PHR2 führt zu pH-abhängigen Defekten des Wachstums, der Zellmorphologie und der Virulenz (Saporito-Irwin et al., 1995; Mühlschlegel und Fonzi, 1997; De Bernardis et al., 1998). Im Rahmen der vorliegenden Arbeit wurde anhand der Isolierung von phr2D-Revertanten der Zusammenhang der molekularen Regulation des morphologischen Formenwechsels und der pH-regulierten Expression von Genen, die eine wichtige Funktion bei der Zellwandsynthese besitzen, untersucht. Die phr2D-Revertanten waren in der Lage bei einem pH-Wert von 4 zu wachsen und zu filamentieren. Das irreguläre Wachstum der Revertanten war auf eine konstitutive Expression des PHR1-Gens zurückzuführen. Dagegen spielte das bei sauren pH-Werten exprimierte PHR1 keine Rolle für das atypische Filamentierungsverhalten der Revertanten. Die molekulargenetische Untersuchung unabhängiger phr2D-Revertanten zeigte, dass eine heterozygote dominant-aktive Mutation im RIM101-Lokus für den Phänotyp der Revertanten verantwortlich war. RIM101 ist demnach das Schlüsselelement des pH-regulierten Dimorphismus. Diese Ergebnisse zeigten zudem, dass der in Aspergillus nidulans und anderen Pilzen beschriebene molekulare Mechanismus der pH-abhängigen Genexpression auch in C. albicans konserviert ist. Die Expression multipler wildtypischer oder mutierter RIM101-Kopien führte zur Suppression des Temperatursignals, welches für das pH-abhängige filamentöse Wachstum notwendig ist. Demnach konvergieren die Umweltsignale pH-Wert und Temperatur auf gemeinsame Zielgene. RIM101 von C. albicans scheint seine eigene Expression zu induzieren. Konstitutiv aktive RIM101-Allele verursachen eine starke Expression von RIM101 bei pH 4. Im Wildtyp dagegen wird RIM101 bei sauren pH-Werten nur schwach exprimiert. Die Inaktivierung der MAP Kinase Kaskade und der cAMP-abhängigen Kaskade durch Deletion der beiden Gene CPH1 und EFG1 führt zur Blockade der morphologischen Flexibilität von C. albicans (Lo et al., 1997). Mit Hilfe eines dominant–aktiven RIM101-Allels wurde eine mögliche Wechselwirkung von RIM101 mit diesen Filamentierungskaskaden untersucht. Diese Untersuchungen ergaben, dass der pH-regulierte Dimorphismus von EFG1 abhängig war. Dagegen war die pH-regulierte Genexpression unabhängig von EFG1. C. albicans und Candida glabrata sind als opportunistische Krankheitserreger in der Lage diverse Gewebe und Organe zu besiedeln und zu infizieren. Das Überleben in den unterschiedlichen Wirtsnischen erfordert daher eine hohe Anpassungsfähigkeit. Auf unterschiedliche Umweltbedingungen reagiert C. albicans, wie oben beschrieben, mit der Expression bestimmter Gene, wie z. B. PHR1, PHR2 und RIM101. Während die Genregulation in C. albicans in den letzten Jahren intensiv erforscht wurde, ist über die differentielle Genexpression in der klinisch zunehmend wichtigen Spezies C. glabrata kaum etwas bekannt. Im Rahmen dieser Arbeit wurde die Etablierung eines geeigneten Reportersystems für C. glabrata angestrebt, welches zur Untersuchung der Genregulation und der Identifizierung differentiell exprimierter Gene eingesetzt werden kann. Das lacZ-Gen wurde als Reporter für die Genexpression in C. glabrata getestet. Die Resultate zeigten die Funktionalität des bakteriellen lacZ-Gens als Reporter für die Genexpression in C. glabrata. Zu dem wurden C. glabrata / E. coli Shuttle-Vektoren entwickelt, die für translationelle Genfusionen zum lacZ verwendet werden können. N2 - Morphological development of the fungal pathogen C. albicans is profoundly affected by environmental signals. This morphological flexibility is considered an essential factor for pathogenicity of C. albicans. One of the important signals that regulates morphology of C. albicans is the ambient pH. Acidic pH restricts growth to the yeast form, whereas neutral pH permits development of the filamentous form. Superimposed on the pH restriction is a temperature requirement of approximately 37°C for filamentation. C. albicans responds to changes in environmental pH by differential expression of several genes including PHR1 and PHR2. PHR2 is an acid expressed gene that is not expressed at detectable levels above pH 6.5. Mutants lacking PHR2 are unable to grow at acidic pH and exhibit morphological defects. PHR1 is an alkaline expressed gene with the inverse pattern of expression. PHR1 and PHR2 encode functionally homologous proteins involved in cell wall biosynthesis, which is pivotal in determining cell shape changes during morphogenesis. The role of pH in development was investigated in this work by selecting revertants of phr2D mutants that had gained the ability to grow at acid pH. The extragenic suppressors in two independent revertants were identified as nonsense mutations in the pH response regulator RIM101 that resulted in a carboxy-terminal truncation of the open reading frame. These dominant active alleles conferred the ability to filament at acidic pH, to express PHR1, an alkaline expressed gene, at acidic pH and to repress the acid expressed gene PHR2. This indicates that RIM101 is a key regulator of the pH-dependent dimorphism in C. albicans. Furthermore these results suggest that the molecular mechanisms which control pH-dependent gene expression in Aspergillus nidulans and other fungi are also conserved in C. albicans. It was also observed that both the wild type and mutant alleles could act as multicopy suppressors of the temperature restriction on filamentation, allowing extensive filamentation at 29°C. This observation suggests that two environmental signals, pH and temperature, converge on common molecular targets. The ability of the activated alleles to promote filamentation was dependent upon the developmental regulator EFG1. The results suggest that RIM101 is responsible for the pH-dependence of hyphal development. C. albicans and C. glabrata are opportunistic pathogens which are able to colonize and infect many tissues and organs. This indicates that these organisms are well adapted for survival within the diverse environmental niches of the human host. C. albicans responds to different environmental signals, as described above, with the expression of certain genes, e.g. PHR1, PHR2 and RIM101. In contrast to C. albicans the gene regulation in the emerging pathogen C. glabrata is poorly understood. In order to develop a reporter system allowing studies on regulated gene expression in C. glabrata the functionality of the E. coli lacZ gene as a reporter of gene expression in C. glabrata was investigated. C. glabrata shuttle vectors suitable for the construction of translational fusions of a gene of interest to the E. coli lacZ reporter were generated. By fusing different promoters to the lacZ gene it could be shown that the E. coli lacZ gene provides a sensitive and inducible reporter displaying b-galactosidase activity in C. glabrata. KW - Candida albicans KW - Wasserstoffionenkonzentration KW - Genexpression KW - Torulopsis glabrata KW - Markierungsgen KW - Candida albicans KW - pH KW - Dimorphismus KW - Genexpression KW - RIM101 KW - Candida glabrata KW - Reportergen KW - Candida albicans KW - pH KW - dimorphism KW - gene expression KW - RIM101 KW - Candida glabrata KW - reporter gene Y1 - 2000 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-1125 ER - TY - JOUR A1 - De Giorgi, Valeria A1 - Buonaguro, Luigi A1 - Worschech, Andrea A1 - Tornesello, Maria Lina A1 - Izzo, Francesco A1 - Marincola, Francesco M. A1 - Wang, Ena A1 - Buonaguro, Franco M. T1 - Molecular Signatures Associated with HCV-Induced Hepatocellular Carcinoma and Liver Metastasis JF - PLoS ONE N2 - Hepatocellular carcinomas (HCCs) are a heterogeneous group of tumors that differ in risk factors and genetic alterations. In Italy, particularly Southern Italy, chronic hepatitis C virus (HCV) infection represents the main cause of HCC. Using high-density oligoarrays, we identified consistent differences in gene-expression between HCC and normal liver tissue. Expression patterns in HCC were also readily distinguishable from those associated with liver metastases. To characterize molecular events relevant to hepatocarcinogenesis and identify biomarkers for early HCC detection, gene expression profiling of 71 liver biopsies from HCV-related primary HCC and corresponding HCV-positive non-HCC hepatic tissue, as well as gastrointestinal liver metastases paired with the apparently normal peri-tumoral liver tissue, were compared to 6 liver biopsies from healthy individuals. Characteristic gene signatures were identified when normal tissue was compared with HCV-related primary HCC, corresponding HCV-positive non-HCC as well as gastrointestinal liver metastases. Pathway analysis classified the cellular and biological functions of the genes differentially expressed as related to regulation of gene expression and post-translational modification in HCV-related primary HCC; cellular Growth and Proliferation, and Cell-To-Cell Signaling and Interaction in HCV-related non HCC samples; Cellular Growth and Proliferation and Cell Cycle in metastasis. Also characteristic gene signatures were identified of HCV-HCC progression for early HCC diagnosis. Conclusions: A diagnostic molecular signature complementing conventional pathologic assessment was identified. KW - identification KW - hepatitis C virus KW - United States KW - gene expression KW - class I KW - endoplasmic reticulum KW - motile phenotype KW - bladder cancer KW - up-regulation KW - target Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-131155 VL - 8 IS - 2 ER - TY - JOUR A1 - Sanz-Moreno, Adrian A1 - Fuhrmann, David A1 - Wolf, Elmar A1 - von Eyss, Björn A1 - Eilers, Martin A1 - Elsässer, Hans-Peter T1 - Miz1 Deficiency in the Mammary Gland Causes a Lactation Defect by Attenuated Stat5 Expression and Phosphorylation JF - PLOS ONE N2 - Miz1 is a zinc finger transcription factor with an N-terminal POZ domain. Complexes with Myc, Bcl-6 or Gfi-1 repress expression of genes like Cdkn2b (p15(Ink4)) or Cd-kn1a (p21(Cip1)). The role of Miz1 in normal mammary gland development has not been addressed so far. Conditional knockout of the Miz1 POZ domain in luminal cells during pregnancy caused a lactation defect with a transient reduction of glandular tissue, reduced proliferation and attenuated differentiation. This was recapitulated in vitro using mouse mammary gland derived HC11 cells. Further analysis revealed decreased Stat5 activity in Miz1 Delta POZ mammary glands and an attenuated expression of Stat5 targets. Gene expression of the Prolactin receptor (PrlR) and ErbB4, both critical for Stat5 phosphorylation (pStat5) or pStat5 nuclear translocation, was decreased in Miz1 Delta POZ females. Microarray, ChIP-Seq and gene set enrichment analysis revealed a down-regulation of Miz1 target genes being involved in vesicular transport processes. Our data suggest that deranged intracellular transport and localization of PrlR and ErbB4 disrupt the Stat5 signalling pathway in mutant glands and cause the observed lactation phenotype. KW - C-MYC KW - transcription factor MIZ-1 KW - breast-cancer cells KW - gene expression KW - epithelial cells KW - prolactin KW - transgenic mice KW - growth KW - differentiation KW - proliferation Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-117286 VL - 9 IS - 2 ER - TY - THES A1 - Hirschmann, Anna T1 - microRNA-Genexpressionsprofile in Blut-, Haut- und Nervenproben von Patienten mit Polyneuropathien T1 - microRNA gene expression profiles in blood, skin and nerve samples of patients with polyneuropathy N2 - Die Polyneuropathie (PNP) ist die häufigste Störung des peripheren Nervensystems bei Erwachsenen. Die Suche nach der Ursache bleibt in vielen Fällen erfolglos, ist aber unverzichtbar, da die Therapiewahl von der Ätiologie der Erkrankung abhängt. Geeignete Biomarker könnten die Differentialdiagnose unter Umständen erleichtern. microRNAs (miRNAs) sind in dieser Hinsicht vielversprechend, da in vielen Studien bei Nervende- und regenerationsprozessen sowie in neuropathischen Schmerzmodellen eine Dysregulation beschrieben wurde. In dieser Studie wurde die Expression zweier miRNAs, miR-103a und miR-let-7d, sowie eines Zielmoleküls der miR-103a, des Kalziumkanals Cav1,2, in einer großen Kohorte von PNP-Patienten unterschiedlicher Ätiologie in Blut, Haut- und Nervenbiopsien untersucht. Insgesamt wurden 116 Patienten und 22 Kontroll-probanden in die Studie eingeschlossen. Nach der Isolation von RNA aus weißen Blutzellen (WBC), Haut- und Nervenbiopsien folgte die Expressionsbestimmung mittels qRT-PCR. Während sich jeweils Unterschiede zwischen PNP-Patienten und Kontrollen und zwischen Patienten mit entzündlicher und solchen mit nicht-entzündlicher PNP zeigten, wurden keine Unterschiede in der Expression zwischen den ätiologischen Subgruppen oder zwischen Patienten mit schmerzhafter und schmerzloser PNP festgestellt. In den Nervenbiopsien der Patientenkohorte ergab sich eine inverse Korrelation der miR-103a und ihrem Zielgen Cacna1c, die darauf hinweisen könnte, dass Cacna1c von der miR-103a negativ reguliert wird. Da in unserer Patientenkohorte keine Unterschiede zwischen den PNP-Subgruppen auftraten, scheint der Einsatz der miR-103a und miR-let-7d als diagnostische Biomarker zur ätiologischen Einordnung einer PNP nicht gerechtfertigt. Dennoch deuten unsere Ergebnisse auf eine mögliche Rolle der untersuchten miRNAs bei Entstehung und Verlauf von PNP hin. Für ein tieferes pathophysiologisches Verständnis der miRNAs vor allem bei entzündlichen Neuropathien, könnte die Untersuchung von weiteren miRNAs und Zielgenen Aufschluss geben. N2 - Polyneuropathies (PNP) are the most frequent disorder of the peripheral nervous system in adults. Since the choice of therapy depends on it, the etiological diagnostic is essential but often remains without results so far. The differential diagnosis could be facilitated by a suitable biomarker. In this respect, microRNA (miRNA) are promising because their dysregulation has been described in processes of nerve degeneration and regeneration as well as in neuropathic pain models. This study investigated the expression of two miRNA, miR-103a and miR-let-7d, and the calcium channel Cav1.2, a target of miR-103a, in a large cohort of PNP patients with different etiology in blood, skin and nerve samples. Altogether, 116 patients and 22 controls have been included in the study. Expressional analysis via qRT-PCR succeeded the isolation of RNA out of white blood cells (WBC), skin and nerve biopsies. Differences have been found between PNP patients and controls and between patients with inflammatory and non-inflammatory PNP. No differences have been recorded between the etiological subgroups or between painful and painless PNP. miR-103a and its target Cacna1c correlated inversely in nerve which could be an indication for Cacna1c being negatively regulated by miR-103a. miR-103a and miR-let-7d do not seem to be appropriate diagnostic biomarkers for the etiological classification of PNP as there have not been found any differences between the PNP subgroups. Nevertheless, our results suggest that miRNA may play a part in the development and the progression of PNP. The investigation of further miRNA and targets could provide insight into a deeper pathophysiological understanding of miRNA, especially in inflammatory neuropathies. KW - miRNS KW - Polyneuropathie KW - Genexpression KW - microRNA KW - miRNA KW - PNP KW - Neuropathischer Schmerz KW - neuropathic pain KW - gene expression Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-217010 ER - TY - JOUR A1 - Correia Santos, Sara A1 - Bischler, Thorsten A1 - Westermann, Alexander J. A1 - Vogel, Jörg T1 - MAPS integrates regulation of actin-targeting effector SteC into the virulence control network of Salmonella small RNA PinT JF - Cell Reports N2 - A full understanding of the contribution of small RNAs (sRNAs) to bacterial virulence demands knowledge of their target suites under infection-relevant conditions. Here, we take an integrative approach to capturing targets of the Hfq-associated sRNA PinT, a known post-transcriptional timer of the two major virulence programs of Salmonella enterica. Using MS2 affinity purification and RNA sequencing (MAPS), we identify PinT ligands in bacteria under in vitro conditions mimicking specific stages of the infection cycle and in bacteria growing inside macrophages. This reveals PinT-mediated translational inhibition of the secreted effector kinase SteC, which had gone unnoticed in previous target searches. Using genetic, biochemical, and microscopic assays, we provide evidence for PinT-mediated repression of steC mRNA, eventually delaying actin rearrangements in infected host cells. Our findings support the role of PinT as a central post-transcriptional regulator in Salmonella virulence and illustrate the need for complementary methods to reveal the full target suites of sRNAs. KW - gene expression KW - nondocing RNA KW - chaperone HFQ KW - soluble-RNA KW - SEQ KW - interactome KW - repression KW - secretion KW - infection KW - biology Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-259134 VL - 34 IS - 5 ER - TY - JOUR A1 - Üçeyler, Nurcan A1 - Valet, Michael A1 - Kafke, Waldemar A1 - Tölle, Thomas R. A1 - Sommer, Claudia T1 - Local and Systemic Cytokine Expression in Patients with Postherpetic Neuralgia N2 - Background Postherpetic neuralgia (PHN) is the painful complication of a varicella zoster virus reactivation. We investigated the systemic and local gene expression of pro- and anti-inflammatory cytokine expression in patients with PHN. Methods Thirteen patients with PHN at the torso (Th4-S1) were recruited. Skin punch biopsies were obtained from the painful and the contralateral painless body area for intraepidermal nerve fiber density (IENFD) and cytokine profiling. Additionally, blood was withdrawn for systemic cytokine expression and compared to blood values of healthy controls. We analyzed the gene expression of selected pro- and anti-inflammatory cytokines (tumor necrosis factor-alpha [TNF] and interleukins [IL]-1β, IL-2, and IL-8). Results IENFD was lower in affected skin compared to unaffected skin (p<0.05), while local gene expression of pro- and anti-inflammatory cytokines did not differ except for two patients who had 7fold higher IL-6 and 10fold higher IL-10 gene expression in the affected skin compared to the contralateral unaffected skin sample. Also, the systemic expression of cytokines in patients with PHN and in healthy controls was similar. Conclusion While the systemic and local expression of the investigated pro- and anti-inflammatory cytokines was not different from controls, this may have been influenced by study limitations like the low number of patients and different disease durations. Furthermore, other cytokines or pain mediators need to be considered. KW - neuropathic pain KW - cytokines KW - pain sensation KW - gene expression KW - nerve fibres KW - RNA extraction KW - shingles KW - skin tumors Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-113041 ER - TY - JOUR A1 - Gaubatz, Stefan A1 - Esterlechner, Jasmina A1 - Reichert, Nina A1 - Iltzsche, Fabian A1 - Krause, Michael A1 - Finkernagel, Florian T1 - LIN9, a Subunit of the DREAM Complex, Regulates Mitotic Gene Expression and Proliferation of Embryonic Stem Cells JF - PLoS ONE N2 - The DREAM complex plays an important role in regulation of gene expression during the cell cycle. We have previously shown that the DREAM subunit LIN9 is required for early embryonic development and for the maintenance of the inner cell mass in vitro. In this study we examined the effect of knocking down LIN9 on ESCs. We demonstrate that depletion of LIN9 alters the cell cycle distribution of ESCs and results in an accumulation of cells in G2 and M and in an increase of polyploid cells. Genome-wide expression studies showed that the depletion of LIN9 results in downregulation of mitotic genes and in upregulation of differentiation-specific genes. ChIP-on chip experiments showed that mitotic genes are direct targets of LIN9 while lineage specific markers are regulated indirectly. Importantly, depletion of LIN9 does not alter the expression of pluripotency markers SOX2, OCT4 and Nanog and LIN9 depleted ESCs retain alkaline phosphatase activity. We conclude that LIN9 is essential for proliferation and genome stability of ESCs by activating genes with important functions in mitosis and cytokinesis. KW - cell cycle KW - cell division KW - cell differentation KW - DNA-binding proteins KW - gene expression KW - gene regulation KW - gene targeting KW - microarrays KW - pluripotency Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96922 ER - TY - JOUR A1 - Zannas, Anthony S. A1 - Arloth, Janine A1 - Carrillo-Roa, Tania A1 - Iurato, Stella A1 - Röh, Simone A1 - Ressler, Kerry J. A1 - Nemeroff, Charles B. A1 - Smith, Alicia K. A1 - Bradley, Bekh A1 - Heim, Christine A1 - Menke, Andreas A1 - Lange, Jennifer F. A1 - Brückl, Tanja A1 - Ising, Marcus A1 - Wray, Naomi R. A1 - Erhardt, Angelika A1 - Binder, Elisabeth B. A1 - Mehta, Divya T1 - Lifetime stress accelerates epigenetic aging in an urban, African American cohort: relevance of glucocorticoid signaling JF - Genome Biology N2 - Background Chronic psychological stress is associated with accelerated aging and increased risk for aging-related diseases, but the underlying molecular mechanisms are unclear. Results We examined the effect of lifetime stressors on a DNA methylation-based age predictor, epigenetic clock. After controlling for blood cell-type composition and lifestyle parameters, cumulative lifetime stress, but not childhood maltreatment or current stress alone, predicted accelerated epigenetic aging in an urban, African American cohort (n = 392). This effect was primarily driven by personal life stressors, was more pronounced with advancing age, and was blunted in individuals with higher childhood abuse exposure. Hypothesizing that these epigenetic effects could be mediated by glucocorticoid signaling, we found that a high number (n = 85) of epigenetic clock CpG sites were located within glucocorticoid response elements. We further examined the functional effects of glucocorticoids on epigenetic clock CpGs in an independent sample with genome-wide DNA methylation (n = 124) and gene expression data (n = 297) before and after exposure to the glucocorticoid receptor agonist dexamethasone. Dexamethasone induced dynamic changes in methylation in 31.2 % (110/353) of these CpGs and transcription in 81.7 % (139/170) of genes neighboring epigenetic clock CpGs. Disease enrichment analysis of these dexamethasone-regulated genes showed enriched association for aging-related diseases, including coronary artery disease, arteriosclerosis, and leukemias. Conclusions Cumulative lifetime stress may accelerate epigenetic aging, an effect that could be driven by glucocorticoid-induced epigenetic changes. These findings contribute to our understanding of mechanisms linking chronic stress with accelerated aging and heightened disease risk. KW - aging KW - DNA methylation KW - gene expression KW - glucocorticoids KW - psychological stress KW - aging-related disease KW - epigenetics Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-149865 VL - 16 IS - 266 ER - TY - THES A1 - Wu, Rongxue T1 - Integrins and SPARC : potential implications for cardiac remodeling N2 - Der enorme Umbau des Herzgewebes, wie man ihn nach Drucküberlastung des Ventrikels oder MyokardInfarkt beobachten kann, gilt als eine der kausalen Ursachen des Herzversagens. Die Veränderungen in der Architektur des Herzens beeinflussen die mechanischen Eigenschaften des Herzmuskels, begründet sind sie jedoch in Anpassungsprozessen auf der zellulären Ebene vor allem in einer Modulation der Expression bestimmter Gene. Gemeinsam mit Integrinen, den Transmembran-Rezeptoren, welche die extrazelluläre Umgebung mit dem intrazellulären Zytoskelett verbinden, gehören Proteine der extrazellulären Matrix (ECM) und matrizelluläre Proteine zu den Schlüsselkomponenten, die den Umbauprozess im Herzen steuern. Aus diesen Gründen hatte diese Doktorarbeit zum Ziel, die Rolle der Integrine für die Regulation der Genexpression und die Leistungsfähigkeit des Herzmuskels während der durch Drucküberlastung oder myokardialen Infarkt (MI) hervorgerufenen Wundheilungsprozesse zu analysieren. Um die Beteiligung von Integrin Beta 1 zu untersuchen, wurde ein experimentelles Modell der Drucküberlastung im Mausherzen (aortic banding; Konstriktion der Aorta; AB) eingesetzt, wobei Mäuse mit einer konditionalen, Herz-spezifischen Deletion des Integrin Beta 1 Gens untersucht wurden. Ein besonderes Augenmerk wurde dabei auf die physiologischen Unterschiede und eine veränderte Genexpression im gestressten Herzen in An- oder Abwesenheit von Integrin Beta 1 gelegt. Interessanterweise wurden die Mäuse, welche eine Kombination aus Integrin knock-out Allel und dem Kardiomyozyten-spezifischen konditionalen knock-out Allel von Integrin Beta 1 aufwiesen im normalen Mendelschen Verhältnis geboren und wuchsen normal auf. Obwohl diese Tiere immer noch geringe Mengen von Integrin Beta 1 in ihrem Herzen aufwiesen (exprimiert von nicht-Myozyten), besaßen diese Mäuse eine veränderte Herzfunktion und waren sehr sensitiv gegenüber AB. Im Gegensatz zu der kompensatorischen hypertrophischen Reaktion, die in Wildtyp Mäusen zu beobachten war, zeigte sich in den Integrin Beta 1–defizienten Mausherzen kein Gewebeumbau. Auch die erhöhte Expression von verschiedenen ECM Proteinen, insbesondere die verstärkte Expression des matrizellulären Proteins SPARC, unterblieb nach AB in den Integrin Beta 1–defizienten Tieren. Interessanterweise konnte auch eine transiente Erhöhung der SPARC mRNA während der Umbauprozesse im Herzen in Folge von myokardialem Infarkt (MI) mittels cDNA Makroarrays festgestellt werden. In der Tat fanden sich größere Mengen von SPARC bereits 2 Tage (~2,5-fach erhöht), 7 Tage (~4-fach erhöht) und 1 Monat (~2-fach erhöht) nach MI, während ein spezifischer Inhibitor der Integrin alpha v Untereinheit diese Hochregulation von SPARC in vivo verhinderte. Immunfluoreszenz Untersuchungen von Herzgewebe verdeutlichten, dass sich die erhöhte Expression von SPARC auf das Infarktareal beschränkte, dass die Expression von SPARC nach einer anfänglichen Erhöhung im Verlauf von 1 Monaten wieder auf das Anfangsniveau zurückging und dass die verstärkte Expression von der Einwanderung von Fibroblasten in das ischämische Herzgewebe begleitet war. In vitro stimulierten die Wachstumsfaktoren TGF-Beta 1 und PDGF-BB die Expression von SPARC durch Fibroblasten. Wie sich an Hand von ELISA und Western Blot Untersuchungen feststellen ließ, war die Inhibition von Integrin Beta v nicht in der Lage, die durch TGF-Beta 1 oder PDGF induzierte Sekretion von SPARC zu beeinflussen. Jedoch zeigte sich, dass Vitronektin, ein Ligand von Integrin alpha v, sowohl die Sekretion von TGF-Beta 1 als auch von PDGF-BB durch Kardiomyozyten induzierte und diese Reaktion wurde durch den Integrin alpha v Inhibitor komplett unterdrückt. In funktioneller Hinsicht wirkte SPARC auf die durch ECM Proteine induzierte Migration von Fibroblasten ein, so dass man davon ausgehen kann, dass die lokale Freisetzung von SPARC nach myokardialem Infarkt zur Wundheilung im Herzen beiträgt. Zusammenfassend läßt die Kombination der in vivo und in vitro erhobenen experimentellen Daten den Schluss zu, dass mehrere Integrin Untereinheiten eine entscheidende Rolle während der Gewebeumbildung im Herzen spielen. Integrin-abhängige Genexpressionsereignisse wie beispielsweise die erhöhte Expression von SPARC nach MI sind entscheidend an der Koordination der Wundheilung beteiligt. Diese Prozesse scheinen auf einer komplexen Wechselwirkung und Kommunikation zwischen verschiedenen Zelltypen wie Kardiomyozyten und Fibroblasten zu beruhen, um lokal begrenzt eine Heilung und Vernarbung des verletzten Gewebes zu regulieren. Die Aufklärung des fein abgestimmten Wechselspiels zwischen Integrinen matrizellulären Proteinen wie SPARC und Wachstumsfaktoren wird sicherlich zu einem besseren und klinisch nutzbarem Verständnis der molekularen Mechanismen des Gewebeumbaus im Herzen beitragen. N2 - The massive remodeling of the heart tissue, as observed in response to pressure overload or myocardial infarction, is considered to play a causative role in the development of heart failure. Alterations in the heart architecture clearly affect the mechanical properties of the heart muscle, but they are rooted in changes at the cellular level including modulation of gene expression. Together with integrins, the transmembrane receptors linking the extracellular environment to the cytoskeleton, extracellular matrix (ECM) proteins and matricellular proteins are key components of the remodeling process in the heart. Therefore, this thesis was aimed at analysing the role of integrins in the regulation of gene expression and heart muscle performance during cardiac wound repair induced by pressure overload or myocardial infarction (MI). To investigate the contribution of integrin Beta 1, we characterised the response of mice with a conditional, cardiac-specific deletion of the integrin Beta 1 gene in an experimental model of pressure overload by aortic banding (AB). In particular, we measured physiological alterations and gene expression events in the stressed heart in the presence or absence of integrin Beta 1. Interestingly, mice containing a knock-out allele and the ventricular myocyte-specific conditional allele of the integrin Beta 1 gene were born and grew up to adulthood. Though these animals still exhibited minor amounts of integrin Beta1 in the heart (expressed by non-myocytes), these mice displayed abnormal cardiac function and were highly sensitive to AB. Whereas a compensatory hypertrophic response to pressure overload was observed in wildtype mice, the integrin Beta 1-deficient mice were not able to undergo heart tissue remodeling. Furthermore, ECM gene expression was altered and, in particular, the increased expression of the matricellular protein SPARC after AB was abolished in integrin Beta 1–deficient mice. Interestingly, we also found a transient upregulation of SPARC mRNA during heart remodeling after MI using cDNA macroarrays. Indeed, increased SPARC protein levels were observed starting at day 2 (2.55±0.21fold, p<0.01), day 7 (3.72±0.28 fold, p<0.01) and 1 month (1.9±0.16 fold, p<0.01) after MI, which could be abolished by using an integrin alpha v inhibitor in vivo. Immunofluorescence analysis of heart tissue demonstrated that the increased SPARC expression was confined to the infarcted area and occurred together with the influx of fibroblasts into the heart. In vitro, either TGF-Beta 1 or PDGF-BB stimulated SPARC expression by fibroblasts. Inhibition of integrin alpha v did not interfere with TGF-Beta1 or PDGF induced SPARC secretion as determined by ELISA assays or Western blot. However, secretion of TGF-Beta1 and PDGF-BB by cardiomyocytes was induced by vitronectin, a ligand of integrin alpha v, and this response was blocked by the integrin alpga v inhibitor. Functionally, SPARC modulated the migratory response of fibroblasts towards ECM proteins suggesting that the local deposition of SPARC following MI contributes to scar formation. Taken together, our combined in vivo and in vitro data demonstrate that several integrin subunits play critical roles during tissue remodeling in the injured heart. Integrin-dependent gene expression events such as the upregulation of SPARC following MI are critical to orchestrate the healing response. These processes appear to involve complex cross-talk between different cell types such as cardiomyocytes and fibroblasts to allow for locally confined scar formation. The elucidation of the sophisticated interplay between integrins, matricellular proteins such as SPARC, and growth factors will undoubtedly provide us with a better and clinically useful understanding of the molecular mechanisms governing heart remodeling. KW - Integrine KW - Genexpression KW - Herzmuskel KW - Grundsubstanz KW - Extracellular matrix KW - gene expression KW - cardiac remodeling KW - migration Y1 - 2006 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-17531 ER - TY - JOUR A1 - Berghoff, Bork A. A1 - Konzer, Anne A1 - Mank, Nils N. A1 - Looso, Mario A1 - Rische, Tom A1 - Förstner, Konrad U. A1 - Krüger, Marcus A1 - Klug, Gabriele T1 - Integrative "Omics"-Approach Discovers Dynamic and Regulatory Features of Bacterial Stress Responses JF - PLOS Genetics N2 - Bacteria constantly face stress conditions and therefore mount specific responses to ensure adaptation and survival. Stress responses were believed to be predominantly regulated at the transcriptional level. In the phototrophic bacterium Rhodobacter sphaeroides the response to singlet oxygen is initiated by alternative sigma factors. Further adaptive mechanisms include post-transcriptional and post-translational events, which have to be considered to gain a deeper understanding of how sophisticated regulation networks operate. To address this issue, we integrated three layers of regulation: (1) total mRNA levels at different time-points revealed dynamics of the transcriptome, (2) mRNAs in polysome fractions reported on translational regulation (translatome), and (3) SILAC-based mass spectrometry was used to quantify protein abundances (proteome). The singlet oxygen stress response exhibited highly dynamic features regarding short-term effects and late adaptation, which could in part be assigned to the sigma factors RpoE and RpoH2 generating distinct expression kinetics of corresponding regulons. The occurrence of polar expression patterns of genes within stress-inducible operons pointed to an alternative of dynamic fine-tuning upon stress. In addition to transcriptional activation, we observed significant induction of genes at the post-transcriptional level (translatome), which identified new putative regulators and assigned genes of quorum sensing to the singlet oxygen stress response. Intriguingly, the SILAC approach explored the stress-dependent decline of photosynthetic proteins, but also identified 19 new open reading frames, which were partly validated by RNA-seq. We propose that comparative approaches as presented here will help to create multi-layered expression maps on the system level ("expressome"). Finally, intense mass spectrometry combined with RNA-seq might be the future tool of choice to re-annotate genomes in various organisms and will help to understand how they adapt to alternating conditions. KW - singlet oxygen stress KW - genome-wide analysis KW - anti-sigma factor KW - rhodobacter sphaeroides KW - gene expression KW - quanititative proteomics KW - photooxidative stress KW - in-vivo KW - photosynthesis genes KW - mass spectrometry Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-127587 SN - 1553-7404 VL - 9 IS - 6 ER - TY - JOUR A1 - Üçeyler, Nurcan A1 - Topuzoğlu, Tengü A1 - Schießer, Peter A1 - Hahnenkamp, Saskia A1 - Sommer, Claudia T1 - IL-4 Deficiency Is Associated with Mechanical Hypersensitivity in Mice JF - PLoS One N2 - Interleukin-4 (IL-4) is an anti-inflammatory and analgesic cytokine that induces opioid receptor transcription. We investigated IL-4 knockout (ko) mice to characterize their pain behavior before and after chronic constriction injury (CCI) of the sciatic nerve as a model for neuropathic pain. We investigated opioid responsivity and measured cytokine and opioid receptor gene expression in the peripheral and central nervous system (PNS, CNS) of IL-4 ko mice in comparison with wildtype (wt) mice. Naïve IL-4 ko mice displayed tactile allodynia (wt: 0.45 g; ko: 0.18 g; p<0.001), while responses to heat and cold stimuli and to muscle pressure were not different. No compensatory changes in the gene expression of tumor necrosis factor-alpha (TNF), IL-1β, IL-10, and IL-13 were found in the PNS and CNS of naïve IL-4 ko mice. However, IL-1β gene expression was stronger in the sciatic nerve of IL-4 ko mice (p<0.001) 28 days after CCI and only IL-4 ko mice had elevated IL-10 gene expression (p = 0.014). Remarkably, CCI induced TNF (p<0.01), IL-1β (p<0.05), IL-10 (p<0.05), and IL-13 (p<0.001) gene expression exclusively in the ipsilateral spinal cord of IL-4 ko mice. The compensatory overexpression of the anti-inflammatory and analgesic cytokines IL-10 and IL-13 in the spinal cord of IL-4 ko mice may explain the lack of genotype differences for pain behavior after CCI. Additionally, CCI induced gene expression of μ, κ, and δ opioid receptors in the contralateral cortex and thalamus of IL-4 ko mice, paralleled by fast onset of morphine analgesia, but not in wt mice. We conclude that a lack of IL-4 leads to mechanical sensitivity; the compensatory hyperexpression of analgesic cytokines and opioid receptors after CCI, in turn, protects IL-4 ko mice from enhanced pain behavior after nerve lesion. KW - mouse models KW - animal behavior KW - sciatic nerves KW - spinal cord KW - opioids KW - cytokines KW - gene expression KW - mice Y1 - 2011 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-137924 VL - 6 IS - 12 ER - TY - JOUR A1 - Buchner, Erich A1 - Blanco Redondo, Beatriz A1 - Bunz, Melanie A1 - Halder, Partho A1 - Sadanandappa, Madhumala K. A1 - Mühlbauer, Barbara A1 - Erwin, Felix A1 - Hofbauer, Alois A1 - Rodrigues, Veronica A1 - VijayRaghavan, K. A1 - Ramaswami, Mani A1 - Rieger, Dirk A1 - Wegener, Christian A1 - Förster, Charlotte T1 - Identification and Structural Characterization of Interneurons of the Drosophila Brain by Monoclonal Antibodies of the Würzburg Hybridoma Library JF - PLoS ONE N2 - Several novel synaptic proteins have been identified by monoclonal antibodies (mAbs) of the Würzburg hybridoma library generated against homogenized Drosophila brains, e.g. cysteine string protein, synapse-associated protein of 47 kDa, and Bruchpilot. However, at present no routine technique exists to identify the antigens of mAbs of our library that label only a small number of cells in the brain. Yet these antibodies can be used to reproducibly label and thereby identify these cells by immunohistochemical staining. Here we describe the staining patterns in the Drosophila brain for ten mAbs of the Würzburg hybridoma library. Besides revealing the neuroanatomical structure and distribution of ten different sets of cells we compare the staining patterns with those of antibodies against known antigens and GFP expression patterns driven by selected Gal4 lines employing regulatory sequences of neuronal genes. We present examples where our antibodies apparently stain the same cells in different Gal4 lines suggesting that the corresponding regulatory sequences can be exploited by the split-Gal4 technique for transgene expression exclusively in these cells. The detection of Gal4 expression in cells labeled by mAbs may also help in the identification of the antigens recognized by the antibodies which then in addition to their value for neuroanatomy will represent important tools for the characterization of the antigens. Implications and future strategies for the identification of the antigens are discussed. KW - cell staining KW - drosophila melanogaster KW - gene expression KW - hybridomas KW - immune serum KW - library screening KW - monoclonal antibodies KW - neurons Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-97109 ER - TY - JOUR A1 - Pfeiffer, Susanne A1 - Krüger, Jacqueline A1 - Maierhofer, Anna A1 - Böttcher, Yvonne A1 - Klöting, Nora A1 - El Hajj, Nady A1 - Schleinitz, Dorit A1 - Schön, Michael R. A1 - Dietrich, Arne A1 - Fasshauer, Mathias A1 - Lohmann, Tobias A1 - Dreßler, Miriam A1 - Stumvoll, Michael A1 - Haaf, Thomas A1 - Blüher, Matthias A1 - Kovacs, Peter T1 - Hypoxia-inducible factor 3A gene expression and methylation in adipose tissue is related to adipose tissue dysfunction JF - Scientific Reports N2 - Recently, a genome-wide analysis identified DNA methylation of the HIF3A (hypoxia-inducible factor 3A) as strongest correlate of BMI. Here we tested the hypothesis that HIF3A mRNA expression and CpG-sites methylation in adipose tissue (AT) and genetic variants in HIF3A are related to parameters of AT distribution and function. In paired samples of subcutaneous AT (SAT) and visceral AT (VAT) from 603 individuals, we measured HIF3A mRNA expression and analyzed its correlation with obesity and related traits. In subgroups of individuals, we investigated the effects on HIF3A genetic variants on its AT expression (N = 603) and methylation of CpG-sites (N = 87). HIF3A expression was significantly higher in SAT compared to VAT and correlated with obesity and parameters of AT dysfunction (including CRP and leucocytes count). HIF3A methylation at cg22891070 was significantly higher in VAT compared to SAT and correlated with BMI, abdominal SAT and VAT area. Rs8102595 showed a nominal significant association with AT HIF3A methylation levels as well as with obesity and fat distribution. HIF3A expression and methylation in AT are fat depot specific, related to obesity and AT dysfunction. Our data support the hypothesis that HIF pathways may play an important role in the development of AT dysfunction in obesity. KW - gene expression KW - adipose KW - hypoxia-inducible factor 3A KW - adipose tissue dysfunction KW - obesity Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-167662 VL - 6 IS - 27969 ER - TY - JOUR A1 - Hennig, Thomas A1 - Michalski, Marco A1 - Rutkowski, Andrzej J. A1 - Djakovic, Lara A1 - Whisnant, Adam W. A1 - Friedl, Marie-Sophie A1 - Jha, Bhaskar Anand A1 - Baptista, Marisa A. P. A1 - L'Hernault, Anne A1 - Erhard, Florian A1 - Dölken, Lars A1 - Friedel, Caroline C. T1 - HSV-1-induced disruption of transcription termination resembles a cellular stress response but selectively increases chromatin accessibility downstream of genes JF - PLoS Pathogens N2 - Lytic herpes simplex virus 1 (HSV-1) infection triggers disruption of transcription termination (DoTT) of most cellular genes, resulting in extensive intergenic transcription. Similarly, cellular stress responses lead to gene-specific transcription downstream of genes (DoG). In this study, we performed a detailed comparison of DoTT/DoG transcription between HSV-1 infection, salt and heat stress in primary human fibroblasts using 4sU-seq and ATAC-seq. Although DoTT at late times of HSV-1 infection was substantially more prominent than DoG transcription in salt and heat stress, poly(A) read-through due to DoTT/DoG transcription and affected genes were significantly correlated between all three conditions, in particular at earlier times of infection. We speculate that HSV-1 either directly usurps a cellular stress response or disrupts the transcription termination machinery in other ways but with similar consequences. In contrast to previous reports, we found that inhibition of Ca\(^{2+}\) signaling by BAPTA-AM did not specifically inhibit DoG transcription but globally impaired transcription. Most importantly, HSV-1-induced DoTT, but not stress-induced DoG transcription, was accompanied by a strong increase in open chromatin downstream of the affected poly(A) sites. In its extent and kinetics, downstream open chromatin essentially matched the poly(A) read-through transcription. We show that this does not cause but rather requires DoTT as well as high levels of transcription into the genomic regions downstream of genes. This raises intriguing new questions regarding the role of histone repositioning in the wake of RNA Polymerase II passage downstream of impaired poly(A) site recognition. KW - DNA transcription KW - dogs KW - thermal stresses KW - chromatin KW - histones KW - gene expression KW - cellular stress responses KW - transcriptional termination Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-176350 VL - 14 IS - 3 ER - TY - JOUR A1 - Schulz, Herbert A1 - Ruppert, Ann-Kathrin A1 - Herms, Stefan A1 - Wolf, Christiane A1 - Mirza-Schreiber, Nazanin A1 - Stegle, Oliver A1 - Czamara, Darina A1 - Forstner, Andreas J. A1 - Sivalingam, Sugirthan A1 - Schoch, Susanne A1 - Moebus, Susanne A1 - Pütz, Benno A1 - Hillmer, Axel A1 - Fricker, Nadine A1 - Vatter, Hartmut A1 - Müller-Myhsok, Bertram A1 - Nöthen, Markus M. A1 - Becker, Albert J. A1 - Hoffmann, Per A1 - Sander, Thomas A1 - Cichon, Sven T1 - Genome-wide mapping of genetic determinants influencing DNA methylation and gene expression in human hippocampus JF - Nature Communications N2 - Emerging evidence emphasizes the strong impact of regulatory genomic elements in neurodevelopmental processes and the complex pathways of brain disorders. The present genome-wide quantitative trait loci analyses explore the \(cis\)-regulatory effects of single-nucleotide polymorphisms (SNPs) on DNA methylation (meQTL) and gene expression (eQTL) in 110 human hippocampal biopsies. We identify \(cis\)-meQTLs at 14,118 CpG methylation sites and \(cis\)-eQTLs for 302 3′-mRNA transcripts of 288 genes. Hippocampal \(cis\)-meQTL-CpGs are enriched in flanking regions of active promoters, CpG island shores, binding sites of the transcription factor CTCF and brain eQTLs. \(Cis\)-acting SNPs of hippocampal meQTLs and eQTLs significantly overlap schizophrenia-associated SNPs. Correlations of CpG methylation and RNA expression are found for 34 genes. Our comprehensive maps of \(cis\)-acting hippocampal meQTLs and eQTLs provide a link between disease-associated SNPs and the regulatory genome that will improve the functional interpretation of non-coding genetic variants in the molecular genetic dissection of brain disorders. KW - psychiatry KW - epigenetics in the nervous system KW - epigenomics KW - gene expression KW - neurological disorders Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-173168 VL - 8 ER - TY - JOUR A1 - Leal, Andrea Zurita A1 - Schwebs, Marie A1 - Briggs, Emma A1 - Weisert, Nadine A1 - Reis, Helena A1 - Lemgruber, Leondro A1 - Luko, Katarina A1 - Wilkes, Jonathan A1 - Butter, Falk A1 - McCulloch, Richard A1 - Janzen, Christian J. T1 - Genome maintenance functions of a putative Trypanosoma brucei translesion DNA polymerase include telomere association and a role in antigenic variation JF - Nucleic Acids Research N2 - Maintenance of genome integrity is critical to guarantee transfer of an intact genome from parent to off-spring during cell division. DNA polymerases (Pols) provide roles in both replication of the genome and the repair of a wide range of lesions. Amongst replicative DNA Pols, translesion DNA Pols play a particular role: replication to bypass DNA damage. All cells express a range of translesion Pols, but little work has examined their function in parasites, including whether the enzymes might contribute to host-parasite interactions. Here, we describe a dual function of one putative translesion Pol in African trypanosomes, which we now name TbPolIE. Previously, we demonstrated that TbPolIE is associated with telomeric sequences and here we show that RNAi-mediated depletion of TbPolIE transcripts results in slowed growth, altered DNA content, changes in cell morphology, and increased sensitivity to DNA damaging agents. We also show that TbPolIE displays pronounced localization at the nuclear periphery, and that its depletion leads to chromosome segregation defects and increased levels of endogenous DNA damage. Finally, we demonstrate that TbPolIE depletion leads to deregulation of telomeric variant surface glycoprotein genes, linking the function of this putative translesion DNA polymerase to host immune evasion by antigenic variation. KW - cross-link repair KW - cell cycle KW - gene expression KW - low fidelity KW - replication KW - bypass KW - theta KW - reveals KW - binding Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-230579 VL - 48 IS - 17 ER - TY - THES A1 - Weniger, Markus T1 - Genome Expression Pathway Analysis Tool - Analyse und Visualisierung von Microarray Genexpressionsdaten unter genomischen, proteomischen und metabolischen Gesichtspunkten T1 - Genom Expression Pathway Analysis Tool - Analysis and visualization of microarray gene expression data under genomic, proteomic and metabolic context N2 - Die Messung der Genexpression ist für viele Bereiche der Biologie und Medizin wichtig geworden und unterstützt Studien über Behandlung, Krankheiten und Entwicklungsstadien. Microarrays können verwendet werden, um die Expression von tausenden mRNA-Molekülen gleichzeitig zu messen und ermöglichen so einen Einblick und einen Vergleich der verschiedenen zellulären Bedingungen. Die Daten, die durch Microarray-Experimente gewonnen werden, sind hochdimensional und verrauscht, eine Interpretation der Daten ist deswegen nicht einfach. Obwohl Programme für die statistische Auswertung von Microarraydaten existieren, fehlt vielen eine Integration der Analyseergebnisse mit einer automatischen Interpretationsmöglichkeit. In dieser Arbeit wurde GEPAT, Genome Expression Pathway Analysis Tool, entwickelt, das eine Analyse der Genexpression unter dem Gesichtspunkten der Genomik, Proteomik und Metabolik ermöglicht. GEPAT integriert statistische Methoden zum Datenimport und -analyse mit biologischer Interpretation für Genmengen oder einzelne Gene, die auf dem Microarray gemessen werden. Verschiedene Typen von Oligonukleotid- und cDNAMicroarrays können importiert werden, unterschiedliche Normalisierungsmethoden können auf diese Daten angewandt werden, anschließend wird eine Datenannotation durchgeführt. Nach dem Import können mit GEPAT verschiedene statische Datenanalysemethoden wie hierarchisches, k-means und PCA-Clustern, ein auf einem linearen Modell basierender t-Test, oder ein Vergleich chromosomaler Profile durchgeführt werden. Die Ergebnisse der Analysen können auf Häufungen biologischer Begriffe und Vorkommen in Stoffwechselwegen oder Interaktionsnetzwerken untersucht werden. Verschiedene biologische Datenbanken wurden integriert, um zu jeder Gensonde auf dem Array Informationen zur Verfügung stellen zu können. GEPAT bietet keinen linearen Arbeitsablauf, sondern erlaubt die Benutzung von beliebigen Teilmengen von Genen oder biologischen Proben als Startpunkt einer neuen Analyse oder Interpretation. Dabei verlässt es sich auf bewährte Datenanalyse-Pakete, bietet einen modularen Ansatz zur einfachen Erweiterung und kann auf einem verteilten Computernetzwerk installiert werden, um eine große Zahl an Benutzern zu unterstützen. Es ist unter der LGPL Open-Source Lizenz frei verfügbar und kann unter http://gepat.sourceforge.net heruntergeladen werden. N2 - The measurement of gene expression data is relevant to many areas of biology and medicine, in the study of treatments, diseases, and developmental stages. Microarrays can be used to measure the expression level of thousands of mRNAs at the same time, allowing insight into or comparison of different cellular conditions. The data derived out of microarray experiments is highly dimensional and noisy, and interpretation of the results can get tricky. Although programs for the statistical analysis of microarray data exist, most of them lack an integration of analysis results and biological interpretation. In this work GEPAT, Genome Expression Pathway Analysis Tool, was developed, offering an analysis of gene expression data under genomic, proteomic and metabolic context. GEPAT integrates statistical methods for data import and data analysis together with an biological interpretation for subset of genes or single genes measured on the chip. GEPAT imports various types of oligonucleotide and cDNA array data formats. Different normalization methods can be applied to the data, afterwards data annotation is performed. After import, GEPAT offers various statistical data analysis methods, as hierarchical, k-means and PCA clustering, a linear model based t-Test or chromosomal profile comparison. The results of the analysis can be interpreted by enrichment of biological terms, pathway analysis or interaction networks. Different biological databases are included, to give various informations for each probe on the chip. GEPAT offers no linear work flow, but allows the usage of any subset of probes and samples as start for a new data analysis or interpretation. GEPAT relies on established data analysis packages, offers a modular approach for an easy extension, and can be run on a computer grid to allow a large number of users. It is freely available under the LGPL open source license for academic and commercial users at http://gepat.sourceforge.net. KW - Microarray KW - Genexpression KW - Datenanalyse KW - Explorative Datenanalyse KW - microarray KW - gene expression KW - data analysis KW - explorative data analysis Y1 - 2007 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-25392 ER - TY - THES A1 - Cremer, Nicole T1 - Genexpression bei der Alzheimer Demenz und dem Morbus Parkinson T1 - Gene expression in Alzheimer Dementia and Parkinson Diseasse N2 - Die Alzheimer Demenz und der Morbus Parkinson als häufigste neurodegenerative Erkrankungen führen zu schwerer Behinderung, zu Pflegebedürftigkeit und meist über Komplikationen zum Tod. Ihr langer Verlauf stellt für Betroffene, Angehörige sowie für das Gesundheitssystem eine enorme Belastung dar. Da die Ätiologie der Alzheimer Demenz und des Morbus Parkinson sowie der meisten neurodegenerativen Krankheiten im Einzelnen nicht bekannt sind und phänotypische Überschneidungen auftreten, sind die Möglichkeiten der eindeutigen Diagnosestellung häufig eingeschränkt oder erst postmortal möglich. Um eine Therapie bei Auftreten der ersten klinischen Symptome zu beginnen oder eine Voraussage der Erkrankungen zu ermöglichen, ist eine sensitive und validierte Frühdiagnostik nötig. Ziel der vorliegenden Arbeit war deshalb, auf der Genebene potentielle pathogenetische Verbindungen, mögliche diagnostische Markerproteine sowie Zusammenhänge zum zeitlichen Verlauf beider Krankheiten zu identifizieren. Dafür wurde mit der Real-Time Polymerasekettenreaktion die Expression von 44 Genen anhand von post mortem Gehirngewebe von Patienten mit Alzheimer Demenz, Morbus Parkionson im Vergleich zu Gesunden aus den vier Hirnregionen Hippocampus, Gyrus frontalis medialis, Gyrus temporalis medialis und Kleinhirn untersucht. Im Resultat zeigen die Gene mit einer statistisch signifikant veränderten Expression, z. B. Glutamattransporter, olfaktorische Rezeptoren oder vakuoläre Sortierungsproteine, bei beiden Erkrankungen gehäuft gleichsinnige Änderungen. Anhand dieser Ergebnisse ist eine kausale Verknüpfung des veränderten Genmetabolismus mit der ablaufenden Neurodegeneration zu vermuten. Zusätzlich wird die Hypothese gemeinsamer pathogenetischer Mechanismen beider Erkrankungen untermauert. Zusammenhänge der Genexpression zum zeitlichen Verlauf der Erkrankungen werden nur vereinzelt belegt, bekräftigten dann aber die Annahme einer Assoziation zu den degenerativen Prozessen. Die Identifizierung eines spezifischen Biomarkers für eine der beiden Erkrankungen war ein Ziel der vorliegenden Arbeit. Aufgrund seiner Expressionsänderung im Hippocampus bei Patienten mit Alzheimer Demenz könnte das BACE1-Gen (Beta site APP cleaving enzyme 1), das dort eine signifikante Expressionsabnahme zeigt, als solcher für dieses Patientenkollektiv diskutiert werden. Die häufig in dieser Arbeit im Hippocampus detektierten, signifikanten Expressionsänderungen, weisen zudem auf eine besondere Affektion dieser Hirnregion bei der Alzheimer Demenz als auch beim Morbus Parkinson hin. Des Weiteren werden in der vorliegenden Arbeit im Kleinhirn, einer Hirnregion, in der bei beiden Erkrankungen scheinbar kaum oder keine pathologischen Prozesse ablaufen, gehäuft und dann ähnliche Änderungen der Genexpression gemessen, die für eine Beteiligung des Kleinhirns bei beiden Krankheiten sprechen, deren Bedeutung bislang unklar ist. N2 - Alzheimer dementia and Parkinson disease are the most common neurodegenerative diseases. They lead to severe disability and mostly cause death through secondary complications. Their long latency is a big burden for the patients, their families and the health care system. The etiology of the most neurodegenerative diseases including Alzheimer dementia and Parkinson disease is largely unknown and there are phenotypical overlaps that limit the diagnostic options. Sensitive and validated diagnostic tools are necessary to start the appropriate therapy early and to make meaningful predictions. This thesis aims to find genes which can act as diagnostic marker proteins, show pathogenetic commonalities and potential correlations to the chronological sequence of the described diseases. 44 genes were analysed with real time polymerase chain reaction of post mortal tissue of the temporal and frontal cortex, the hippocampus and cerebellum from patients with Alzheimer dementia and Parkinson disease compared to a control group. Genes with statistical significant changes in expression between test subjects and controls as the olfactory receptor gene, the glutamate transporter gene or the vacuolar sorting protein gene often show similar changes in both diseases. These results show a connection between the changed gene expression and the progress of the neurodegenerative process in both diseases. In addition these results support the theory of common pathogenetic pathways in both diseases. Correlations to the chronological sequence of both diseases were confirmed just in individual cases but corroborate the connection to the ongoing neurodegenerative process. Furthermore this thesis aims to identify a diagnostic biological marker. Due to the expression profile of the BACE1 gene in the hippocampus of patients with Alzheimer dementia this gene can be seen as a potential biological marker for this group of patients. The frequently measured changes of gene expression profiles in the hippocampus show the particular significance of this brain region in the Alzheimer dementia and Parkinson disease. Furthermore this thesis shows numerous and similar changes of gene expression profiles for both diseases in the cerebellum, a region which demonstrates nearly no pathological processes in Alzheimer dementia and Parkinson disease. The significance of the findings is yet unknown and requires further research. KW - Alzheimer KW - Demenz KW - Parkinson KW - Genexpression KW - Alzheimer-Krankheit KW - Demenz KW - Parkinson-Krankheit KW - Differentielle Genexpression KW - Genanalyse KW - Gen KW - Alzheimer KW - dementia KW - Parkinson KW - gene KW - gene expression KW - gene analysis KW - Parkinson disease KW - Alzheimer disease Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-76748 ER - TY - THES A1 - Altrock, Stefanie T1 - Genetische Organisation und Transkription eines Virulenz-assoziierten, instabilen Chromosomenabschnitts von Listeria ivanovii T1 - Genetic organisation and transcription of a virulence-associated, instable chromosomal region of Listeria ivanovii N2 - Unter den sechs Arten der Gattung Listeria finden sich nur zwei pathogene Spezies. L. monocytogenes ist pathogen für Mensch und Tier, L. ivanovii nur tierpathogen. Beide Arten besitzen ein Virulenzgencluster, das auch als Pathogenitätsinsel LIPI-1 bezeichnet wird. Pathogenitätsinseln (PAIs) sind bei gram-negativen Bakterien weit verbreitet, wurden bei gram-positiven Pathogenen bisher jedoch nur selten beschrieben. In L. ivanovii wurde nun ein weiterer Virulenz-assoziierter, instabiler Chromosomenabschnitt entdeckt, der in einem Teilbereich Eigenschaften einer Pathogenitätsinsel besitzt. Ausgehend von einem spontanen, aber reproduzierbaren Deletionsereignis eines großen Genomabschnitts, der einige schon bekannte Virulenz-assoziierte Gene umfasst (i-inlE, i-inlF, smcL), wurden in Zusammenarbeit mit den Kooperationspartnern an der "Universidad Complutense de Madrid", insbesondere mit G. Domínguez-Bernal die komplette deletierte Region sowie flankierende Genombereiche genauer analysiert. Im Rahmen dieser Arbeit konnten rechts von dem bereits charakterisierten Gen smcL 13 neue Open Reading Frames (ORFs) bzw. Gene (ydeI, rnaH, norA) von L. ivanovii identifiziert werden, die größtenteils in der Deletionsmutante L. ivanovii GD-3 deletiert waren. Für die meisten Open Reading Frames konnten Homologien zu ORFs in den Genomsequenzen von L. monocytogenes und der apathogenen Art L. innocua gefunden werden. Eigene experimentelle Analysen zeigten zudem, dass diese ORFs in ähnlicher Anordnung auch in den apathogenen Arten L. seeligeri und L. welshimeri vorhanden sind, was wahrscheinlich macht, dass sie nicht an der Virulenz von Listerien beteiligt sind. G. Domínguez-Bernal fand im links von smcL liegenden Bereich eine Reihe neuer Internalingene, die alle spezifisch für L. ivanovii sind. Für die Gene i-inlE, i-inlF und smcL ist bereits bekannt, dass diese Virulenz-assoziiert sind. Dies führte zur Definition einer neuen, LIPI-2 genannten Pathogenitätsinsel in L. ivanovii, die außer smcL und i-inlFE alle neu gefundenen Internalingene umfasst. In dieser Arbeit durchgeführte Untersuchungen der LIPI-2 flankierenden Bereiche zeigten, dass diese in L. monocytogenes und auch den apathogenen Arten L. innocua, L. seeligeri und L. welshimeri bemerkenswert konserviert sind. Durch Transkriptionsuntersuchungen mittels RT-PCR wurde die Expression der neu identifizierten Gene analysiert. Hierbei wurden verschiedene Kulturbedingungen untersucht sowie die Transkription nach Infektion mehrerer Zelllinien bestimmt. Bei der Sequenzanalyse wurde für fast alle Internalingene eine PrfA-Box identifiziert und es bestätigte sich in dieser Arbeit, dass die meisten der Internalingene PrfA-abhängig exprimiert werden. Allerdings wiesen die einzelnen Gene kein einheitliches Transkriptionsprofil unter verschiedenen in vitro-Bedingungen auf. Eine Analyse der Genexpression nach Infektion verschiedener Zelllinien zeigte schließlich, dass die Internalingene während einer Infektion differentiell transkribiert werden und möglicherweise am Infektionsgeschehen beteiligt sind. Das Expressionsmuster der zu LIPI-2 benachbarten Open Reading Frames bestätigte, dass diese Gene PrfA-unabhängig und unter verschiedenen Bedingungen konstitutiv exprimiert werden. Das Expressionsmuster dieser Gene läßt den Schluss zu, dass sie vermutlich nicht zur Virulenz von L. ivanovii beitragen. Die Untersuchung der Virulenzclustergene in LIPI-1 schließlich zeigte eine deutliche PrfA-Abhängigkeit der Genexpression. Es konnte bestätigt werden, dass deren Transkription unter PrfA-induzierenden Bedingungen verstärkt wird. Zudem fand sich auch nach Infektion eine deutliche Expression dieser Gene. N2 - Among the six species of Listeria only two are pathogenic. Whereas L. monocytogenes is pathogenic for men and animals, L. ivanovii only causes Listeriosis in animals. Both pathogenic species possess a virulence gene cluster, which is also designated as pathogenicity island LIPI-1. Pathogenicity islands (PAIs) are widespread among gram-negative bacteria, but so far have rarely been described for gram-positive pathogens. In L. ivanovii, an additional virulence-associated unstable part of the chromosome has recently been discovered, parts of which have some characteristics of a pathogenicity island. Starting from a spontaneous but reproducible deletion event of a big part of the genome which carries some known virulence associated genes (i-inlE, i-inlF, smcL), the complete deleted area plus flanking regions were analyzed in co-operation with G. Domínguez-Bernal from the "Universidad Complutense de Madrid". Within this work 13 new open reading frames (ORFs) resp. genes (ydeI, rnaH, norA) on the right side of the smcL gene could be identified in L. ivanovii. Most of them were deleted in the deletion mutant L ivanovii GD-3. Most of the open reading frames show homologies to ORFs also found in the genome sequences of L. monocytogenes and the apathogenic species L. innocua. Own experimental analyses showed, that the genes identified in this work are also present in the apathogenic species L. seeligeri and L. welshimeri. From this it can be concluded that they presumably are not involved in L. ivanovii virulence. G. Domínguez-Bernal discovered several new internalin genes on the left side of the smcL gene. All these genes are specific for L. ivanovii. For i-inlE, i-inlF and smcL it has already been shown that they are virulence associated. This lead to the definition of a new pathogenicity island (LIPI-2) in L. ivanovii, which, in addition to smcL and i-inlFE, comprises all newly found internalin genes. Study of the regions flanking LIPI-2 showed that these are considerably conserved in L. monocytogenes as well as in the apathogenic species L. innocua, L. seeligeri and L. welshimeri. By means of RT-PCR the expression of the new identified genes was analyzed. For this, different culture conditions and transcription after infection of several cell lines were examined. By sequence analysis, a PrfA-box has been identified in front of almost all internalin genes. This work confirmed, that the expression of most internalin genes is PrfA-dependent. However, the transcription pattern was not uniform under different in vitro conditions. Finally, the analysis of gene expression after infection of several cell lines showed, that the internalin genes are transcribed differentially during infection. From this it can be concluded that they may have a role in the infection process. The expression pattern of the open reading frames flanking LIPI-2 confirmed, that these genes are transcribed PrfA independently and constitutively in vitro. This suggests that they do not contribute to virulence of L. ivanovii. Examination of the virulence cluster genes finally showed, that there is a strong PrfA dependency in gene expression. It could be confirmed, that the transcription of these genes is increased under PrfA inducing conditions. In addition, after infection also a strong expression could be detected. KW - Listeria ivanovii KW - Virulenz KW - Molekulargenetik KW - Listeria KW - Listeria ivanovii KW - LIPI-2 KW - Pathogenitätsinsel KW - Internaline KW - ydeI KW - rnaH KW - norA KW - Genexpression KW - Listeria KW - Listeria ivanovii KW - LIPI-2 KW - pathogenicity island KW - internalins KW - ydeI KW - rnaH KW - norA KW - gene expression Y1 - 2002 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-3303 ER - TY - JOUR A1 - Morton, Charles Oliver A1 - Fliesser, Mirjam A1 - Dittrich, Marcus A1 - Müller, Tobias A1 - Bauer, Ruth A1 - Kneitz, Susanne A1 - Hope, William A1 - Rogers, Thomas Richard A1 - Einsele, Hermann A1 - Löffler, Jürgen T1 - Gene Expression Profiles of Human Dendritic Cells Interacting with Aspergillus fumigatus in a Bilayer Model of the Alveolar Epithelium/Endothelium Interface N2 - The initial stages of the interaction between the host and Aspergillus fumigatus at the alveolar surface of the human lung are critical in the establishment of aspergillosis. Using an in vitro bilayer model of the alveolus, including both the epithelium (human lung adenocarcinoma epithelial cell line, A549) and endothelium (human pulmonary artery epithelial cells, HPAEC) on transwell membranes, it was possible to closely replicate the in vivo conditions. Two distinct sub-groups of dendritic cells (DC), monocyte-derived DC (moDC) and myeloid DC (mDC), were included in the model to examine immune responses to fungal infection at the alveolar surface. RNA in high quantity and quality was extracted from the cell layers on the transwell membrane to allow gene expression analysis using tailored custom-made microarrays, containing probes for 117 immune-relevant genes. This microarray data indicated minimal induction of immune gene expression in A549 alveolar epithelial cells in response to germ tubes of A. fumigatus. In contrast, the addition of DC to the system greatly increased the number of differentially expressed immune genes. moDC exhibited increased expression of genes including CLEC7A, CD209 and CCL18 in the absence of A. fumigatus compared to mDC. In the presence of A. fumigatus, both DC subgroups exhibited up-regulation of genes identified in previous studies as being associated with the exposure of DC to A. fumigatus and exhibiting chemotactic properties for neutrophils, including CXCL2, CXCL5, CCL20, and IL1B. This model closely approximated the human alveolus allowing for an analysis of the host pathogen interface that complements existing animal models of IA. KW - aspergillus fumigatus KW - gene expression KW - immune receptors KW - immune response KW - denritic cells KW - B cell receptors KW - gene regulation KW - RNA extraction Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-112893 ER - TY - THES A1 - Körner, Ulrich T1 - Funktionelle Rolle von HMGN-Proteinen während der Embryonalentwicklung von Xenopus laevis T1 - The functional role of the HMGN proteins during embryogenesis of Xenopus laevis N2 - HMGN Proteine sind Architekturelemente des Chromatins und besitzen die Fähigkeit, Chromatin aufzulockern. Sie ermöglichen anderen Proteinen den Zugang zu Nukleosomen und unterstützen DNA-abhängige Prozesse wie Replikation, Transkription und DNA-Reparatur. In dieser Arbeit wurde die funktionelle Rolle der HMGN Proteine während der Embryogenese am Beispiel des südafrikanischen Krallenfroschs Xenopus laevis untersucht. Dabei wurde entdeckt, dass sowohl die Expression als auch die zelluläre Verteilung der HMGN Proteine entwicklungsspezifisch reguliert ist. Eine Manipulation der HMGN Proteinmengen während der Embryonalentwicklung führte zu schweren Fehlentwicklungen in Postblastula Embryonen. In der Oogenese waren sowohl Xenopus HMGN mRNAs als auch Xenopus HMGN Proteine in allen Oozytenstadien nachweisbar. Interessanterweise waren HMGN Proteine in späteren Oozytenstadien nur im Zytoplasma zu finden und nicht mit Lampenbürstenchromosomen assoziiert. Im Zuge der Maturation der Oozyten zu Eiern verschwinden die Proteine gänzlich. Während der Embryogenese waren HMGN Proteine dann erst wieder ab der Blastula detektierbar, zeitgleich mit der transkriptionellen Aktivierung des embryonalen Genoms. Gleichzeitig wiesen ihre Expressionsmuster, zumindest auf mRNA-Ebene, auf Gewebspezifität hin. Whole mount in situ-Hybridisierungen und RT-PCR-Analysen zeigten eine erhöhte mRNA-Menge in mesodermalen und neuroektodermalen Geweben von Schwanzknospenstadien. Nach Injektion rekombinanter HMGN Proteine (Überexpression) oder Morpholino-Antisense-Oligonukleotiden (knock-down) in die Zygote entwickelten sich Embryonen mit offenen Rücken, stark verkürzten und gebogenen Körperachsen und deformierten Kopfstrukturen als Hauptmerkmale. Histologische Analysen und insbesondere die Magnetresonanz Bildgebung deuteten auf Fehler in der Mesodermdifferenzierung hin. Die Analysen zeigen, dass eine bestimmte kritische zelluläre HMGN Proteinmenge für eine korrekte Embryonalentwicklung von Xenopus laevis notwendig ist. Durch „animal cap assays“ und RT-PCR-Expressionsanalysen Mesoderm-spezifischer Gene konnte schließlich gezeigt werden, dass HMGN Proteine die Regulation Mesoderm-spezifischer Gene beeinflussen. Die Ergebnisse lassen vermuten, dass auch die HMGN-Genexpression während der Mesodermdifferenzierung reguliert wird. Durch eine Analyse des Expressionsbeginns entwicklungsrelevanter Gene während der Midblastula Transition konnte gezeigt werden, dass veränderte HMGN Proteinmengen den Expressionsbeginn spezifischer Gene wie Xbra und chordin beeinflussen. Damit konnte zum ersten Mal ein Einfluss dieser ubiquitären Chromatinproteine auf die Expression spezifischer Gene gefunden werden. Die durch HMGN Proteine verursachte fehlerhafte Expression von Xbra und chordin als Schlüsselgene der Mesodermdifferenzierung kann die Fehlentwicklungen mesodermaler Strukturen erklären. N2 - HMGN proteins are architectural chromatin proteins that reduce the compaction of the chromatin fiber, facilitate access to nucleosomes and modulate DNA-dependent processes such as replication, transcription and DNA repair. In this work the functional role of the HMGN proteins during embryogenesis was analyzed using the African clawed frog Xenopus laevis as a model system. The expression and cellular location of the HMGN proteins was found to be developmentally regulated. Experimental manipulations of the HMGN protein amounts led to gross developmental defects in postblastula embryos. HMGN transcripts and proteins were present throughout oogenesis. Interestingly, the HMGN proteins were stored in the cytoplasm of later oocyte stages and excluded from the oocytes nuclei and lampbrush chromosomes. Upon maturation of oocytes into eggs, HMGN proteins were no longer detectable. During embryogenesis, HMGN proteins were first detected in blastula stage embryos, coinciding with the transcriptional activation of the embryonic genome. At least at the mRNA level the expression pattern showed a tissue specific pattern, with relatively high levels of mRNAs in the mesodermal and neuroectodermal regions of early tailbud embryos as shown by whole mount in-situ hybridization and RT-PCR-analyses. After microinjection of recombinant HMGN proteins (overexpression) or morpholino-antisense oligonucleotides (knock-down) the embryos displayed typical phenotypes with imperfect closure of the blastopore, distorted body axis and abnormal head structures. Histological analyses and magnetic resonance imaging indicated that mesoderm differentiation was particularly affected by aberrant HMGN protein levels. The results demonstrate that proper embryonic development of Xenopus laevis requires precisely regulated levels of HMGN proteins. “Animal cap assays” and RT-PCR-analyses of the expression of mesodermal genes indicated that HMGN proteins are involved in the regulation of mesoderm specific genes. These experiments also indicated that the HMGN expression itself is regulated during mesoderm differentiation. Moreover, by studying the expression pattern of developmentally relevant genes during midblastula transition it became evident that altered HMGN protein levels influence the onset of the expression of specific genes such as Xbra and chordin. The results show, for the first time, that these ubiquitous chromatin proteins modulate the expression of specific genes. The HMGN-induced misexpression of Xbra and chordin as key regulatory genes during mesoderm differentiation may explain the observed malformations of mesodermal structures. KW - Glatter Krallenfrosch KW - HMG-Proteine KW - Genexpression KW - Embryonalentwicklung KW - HMGN Proteine KW - Xenopus laevis KW - Genexpression KW - Chromatin KW - Embryonalentwicklung KW - HMGN proteins KW - Xenopus laevis KW - chromatin KW - gene expression KW - early development Y1 - 2004 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-9166 ER - TY - THES A1 - Stoll, Sascha T1 - Funktionelle Analyse von Blochmannia floridanus, dem primären Endosymbionten der Rossameise Camponotus floridanus T1 - Functional analysis of Blochmannia floridanus, the primary endosymbiont of the carpenter ant Camponotus floridanus N2 - Ameisen der Gattung Camponotus beherbergen bakterielle Symbionten der Gattung Blochmannia in spezialisierten Zellen des Mitteldarms (Blochmann, 1882; Buchner, 1965; Sauer, 2000; Schröder et al., 1996). Die Genomsequenzierung dieser Symbionten zeigte, dass Blochmannia, ähnlich den Symbionten von Blattläusen, hauptsächlich Gene der Aminosäurebiosynthese beibehalten hat (Degnan et al., 2005; Gil et al., 2003). Die Relevanz dieser nahrungsaufwertenden Funktion konnte experimentell bestätigt werden (Feldhaar et al., 2007). Ein Schwerpunkt der vorliegenden Arbeit war die Aufklärung der dynamischen Interaktion der beiden Partner während des komplexen Lebenszyklus des holometabolen Wirtes. Frühere Studien deuteten darauf hin, dass die Symbiose vor allem während der Larven- und Puppenphasen von Bedeutung sein könnte (Feldhaar et al., 2007; Wolschin et al., 2004; Zientz et al., 2006). Mit fluoreszenter in situ Hybridisierung (FISH) und konfokaler Laserscanning Mikroskopie konnte in der vorliegenden Arbeit die Lokalisierung von B. floridanus während der wichtigsten Entwicklungsstadien aufgeklärt werden. Hierbei konnte gezeigt werden, dass die Symbionten schon im ersten Larvenstadium in spezialisierten Zellen um den Darm angeordnet sind, aber in späteren Stadien nicht, wie bisher angenommen, auf diese Bakteriozyten beschränkt sind, sondern bis zum Schlupf der jungen Arbeiterinnen massiv andere Darmzellen infizieren. Übereinstimmend mit Bestimmungen der Zellzahl in den verschiedenen Wirtsstadien ist die Anzahl der Symbionten gegen Ende der Metamorphose am höchsten. Die Symbiose degeneriert in sehr alten Arbeiterinnen, gut gefüllte Bakteriozyten werden jedoch noch monatelang beibehalten. Mit Macroarray- und qRT- PCR- basierten Transkriptomanalysen wurde die Expression der bakteriellen Gene in charakteristischen Entwicklungsstadien des Wirtes untersucht. Allgemein zeigen vor allem Gene für molekulare Chaperons und bestimmte bakterielle Grundfunktionen eine hohe Expression. Aber auch viele Gene, die möglicherweise wichtige Funktionen in der Symbiose besitzen, wie die Biosynthese essentieller Aminosäuren und das Recycling von Stickstoffverbindungen, zeigen ein hohes absolutes Transkriptlevel. Zudem besteht eine positive Korrelation zwischen dem Expressionsniveau und dem GC- Gehalt der Gene, die in dem höheren Selektionsdruck und damit einer geringeren Mutationsrate der essentiellen Gene begründet liegt (Schaber et al., 2005). Durch Proteinanalysen konnte bestätigt werden, dass die Faktoren mit der höchsten absoluten Transkription die dominanten Proteine der Symbionten darstellen. In den unterschiedlichen Entwicklungsstadien zeigen viele Gene eine deutliche Dynamik, deren Ausmaß aber, verglichen mit freilebenden Bakterien, gering ist. Aus den Expressionsprofilen aufeinanderfolgender Gene lassen sich mögliche Transkriptionseinheiten ableiten, die teilweise auch experimentell bestätigt wurden. Oftmals zeigen auch Gene, die nicht in Transkriptionseinheiten angeordnet sind, aber verwandten Stoffwechselwegen angehören, ähnliche Muster. Dies deutet auf das Vorhandensein grundlegender Genregulations-mechanismen hin, obwohl im Genom von B. floridanus nur noch sehr wenige Transkriptionsfaktoren codiert sind (Gil et al., 2003). Auf übergeordneter Ebene zeigt sich, dass bei Symbionten aus späten Puppenstadien viele symbioserelevante Gene im Vergleich zu Genen des Grundmetabolismus eine erhöhte Expression zeigen. Dies betrifft besonders die Biosynthese aromatischer und verzweigter Aminosäuren, die in diesen Stadien vom Wirt in hoher Menge benötigt werden, während die internen Reserven gleichzeitig zur Neige gehen. Dies äußert sich auch im deutlichen Abfallen der Speicherproteinmenge des Wirts gegen Ende der Puppenphase. Die festgestellte Veränderung der Symbiontenzahl übertrifft das geringe Ausmaß der Genregulation um ein Vielfaches. Die Bakterien liegen in jedem Stadium polyploid mit bis zu 100 Genomkopien vor, dieser Polyploidiegrad bleibt jedoch während der gesamten Wirtsentwicklung weitestgehend konstant. Somit scheint die Kontrolle des Wirts über die bakterielle Vermehrung der entscheidende Faktor dieser Symbiose zu sein. Die verbleibenden regulatorischen Fähigkeiten der Bakterien stellen möglicherweise eine Feinjustierung von optimierten Produktionseinheiten dar, deren Anzahl nach den Bedürfnissen des Wirtes verändert wird. Insgesamt konnten in der vorliegenden Arbeit neue Einblicke in das komplexe Zusammenleben von Blochmannia und Camponotus gewonnen werden, die zu einem besseren Verständnis der biologischen Funktion und der grundlegenden Mechanismen dieser Symbiose führen. Eine der wichtigsten Fragestellungen nach dem Sinn einer nahrungsaufwertenden Symbiose für einen Nahrungsgeneralisten konnte mit starken Hinweisen auf eine stadienabhängige Relevanz der Symbiose beantwortet werden, die den enormen evolutionären Erfolg dieser Ameisengattung erklären könnte.  N2 - Ants of the genus Camponotus harbor bacterial endosymbionts of the genus Blochmannia in specialized cells of their midgut (Blochmann, 1882; Buchner, 1965; Sauer, 2000; Schröder et al., 1996). The complete sequencing of the symbiont’s genome revealed, that Blochmannia, comparable to the symbionts of aphids, mainly retained genes involved in the biosynthesis of essential amino acids (Degnan et al., 2005; Gil et al., 2003). The biological relevance of a nutritional upgrading by Blochmannia could be confirmed experimentally (Feldhaar et al., 2007). One focus of this thesis was the elucidation of the dynamic interactions between the two partners during the complex life cycle of the holometabolic host animal. Previous studies pointed towards a temporal relevance of this symbiosis especially during larval and pupal development (Feldhaar et al., 2007; Wolschin et al., 2004; Zientz et al., 2006). In this thesis the localization of B. floridanus could be documented throughout all life stages of the host by fluorescent in situ hybridization (FISH) and confocal laser scanning microscopy. A layer of densely filled bacteriocytes surrounding the gut could already be identified in first instar larvae. In contrast to previous assumptions, the bacteria are not restricted to these cells in later stages, as until the eclosion of the young adult workers bacteria massively infect other midgut cells. Concordant with previous findings, bacterial load is highest at the end of metamorphosis and symbiont numbers decrease in older workers, yet densely filled bacteriocytes are still visible after several months. The expression of the bacterial genes during characteristic life stages of the C. floridanus was assessed by macroarray and qRT- PCR- based experiments. In general, especially molecular chaperones, central basic metabolism and may putative symbiosis related factors like pathways leading to essential amino acids or nitrogen recycling show highest absolute expression levels. A positive correlation between expression level and GC- content of the genes can be observed, which is caused by a higher selection pressure and lower mutation rate of these essential factors (Schaber et al., 2005). Protein analyses confirmed the correlation between gene expression and translation of the most abundant factors. Many B. floridanus genes exhibit a dynamic expression during the different host stages but the extent of this gene regulation is modest as compared to free living bacteria. Expression profiles of genes located next to each other on the genome allow proposal of local transcription units, which were confirmed experimentally in several cases. Often genes that are not clustered locally but belong to related metabolic functions also exhibit similar expression patterns. This indicates the existence of basic mechanisms of gene regulation despite the low number of transcription factors annotated in the B. floridanus genome (Gil et al., 2003). In late pupal stages symbiosis related genes often show a higher expression compared to basic metabolic functions. This especially includes biosynthetic pathways for aromatic and branched amino acids, which are needed by the host at this stage in increased amounts, while internal storages are depleted. This could be demonstrated by the significant decrease in storage proteins of the host at the end of the pupal phase. The observed change in bacterial numbers per host exceeds the extent of bacterial gene regulation by far. The symbionts are polyploid in each host stage with up to 100 genome copies per cell. The degree of polyploidy is largely constant during host development. Thus the control over bacterial reproduction seems to be the decisive factor in this symbiosis. The residual regulatory capacities of the symbionts might represent a mechanism of fine tuning of a production unit that has been streamlined by evolution and whose numbers are adjusted according to the host’s needs. In conclusion, this thesis delivers new insights into the complex symbiosis of Blochmannia and Camponotus leading to a better understanding of its biological function and the underlying mechanisms. One of the central mysteries concerning the need of a symbiont for nutritional upgrading for an omnivorous host could be explained by a temporal, stage- dependent relevance of this symbiosis, possibly being the reason for the enormous evolutionary success of this ant genus. KW - Intrazelluläre Symbiose KW - Symbiose KW - Ameisen KW - Mikrobiologie KW - Gram-negative Bakterien KW - Bakterien KW - Differentielle Genexpression KW - Genexpression KW - Entwicklung KW - Blochmannia KW - Camponotus KW - symbiosis KW - endosymbiosis KW - ants KW - bacteria KW - gene expression Y1 - 2009 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-37238 ER - TY - THES A1 - Schäfer, Ingo T1 - Fremdgenexpression in humanen Mitochondrien T1 - Artificial gene expression in human mitochondria N2 - Bei einer Vielzahl neuromuskulärer und neurodegenerativer Erkrankungen spielen Fehlfunktionen der Mitochondrien eine wichtige Rolle. Da die Proteine der Atmungsketten-komplexe sowohl durch die mitochondriale DNA als auch durch das Kerngenom codiert werden, können Mutationen in beiden Genomen die Auslöser dieser Erkrankungen darstellen. Veränderungen der mitochondrialen DNA lassen sich - im Gegensatz zum Kerngenom - bisher nicht korrigieren, weshalb bei einem großen Teil der Erkrankungen nur die Symptome und nicht die Auslöser behandelt werden können. Das grundlegende Problem stellt dabei der Transport der DNA in die Mitochondrien dar. Ziel dieser Arbeit war es, mit Hilfe von physikalischen Transfektionsmethoden exogene DNA in die Mitochondrien menschlicher Kulturzellen einzubringen. Dazu wurden unterschiedliche Vektoren hergestellt, die in Mitochondrien das an die Mitochondrien angepasste grün fluoreszierende mtEGFP exprimieren sollen. Die Expressionsfähigkeit und Prozessierung dieser Konstrukte konnte in in-vitro-Assays mit einem Mitochondrienextrakt nachgewiesen werden. Bei Transfektionsversuchen mit der Gene Gun gelang es erstmals, exogene Plasmid-DNA in die Mitochondrien menschlicher Zellen einzubringen. Das durch die transfizierten Vektoren exprimierte mtEGFP konnte am Fluoreszenzmikroskop eindeutig in den Mitochondrien der Zellen lokalisiert werden. Eine Transfektion mit Hilfe magnetischer Partikel erwies sich jedoch nicht als zielführend, da die die Partikel eine Eigenfluoreszenz aufwiesen, die eine Detektion der mtEGFP-Expression verhinderten. Eine wichtige Voraussetzung für die Transfektion von Mitochondrien durch mechanische Methoden wie die Mikroinjektion ist die reversible Induktion von Megamitochondrien, da sie erst in diesem Zustand penetriert werden können. Durch eine Ansäuerung des Kulturmediums mit Natriumacetat bzw. Essigsäure konnten Mitochondrien erzeugt werden, die beinahe die Größe des Zellkerns aufwiesen und somit ideale Bedingungen für die Mikroinjektion darstellen. Bei den anschließenden Mikroinjektionsversuchen mit den hergestellten mitochondrialen Expressionsvektoren wurden wiederum Zellen mit eindeutig grün fluoreszierenden Mitochondrien gefunden. Zusammenfassend wurden im Rahmen dieser Arbeit erstmalig menschliche Mitochondrien mit exogener DNA transfiziert. Dies stellt einen grundlegenden Schritt für die Entwicklung neuer Therapieformen bei mitochondrialen Myopathien dar. Zuvor müssen die Transfektionsmethoden jedoch noch weiter optimiert werden, um eine höhere Transfektionseffizienz zu erreichen. N2 - Mitochondrial dysfunctions play an important role in a variety of neuromuscular and neurodegenerative diseases. As the proteins of the respiratory chain complexes are encoded by the mitochondrial DNA as well as the nuclear genome, mutations in both could trigger solely the diseases. Up to now, changes of the mitochondrial DNA could not be corrected, hence, therapies were designed to decrease symptoms in patients. In this context, the limiting factor to cure these disease relies on the DNA transport into the mitochondria. The aim of this work was to insert exogenous DNA into the mitochondria of human cultured cells by physical transfection methods. A variety of different vectors was constructed to express the mitochondrially adapted green fluorescent mtEGFP within mitochondria. The ability of these constructs to be expressed and processed was proved by in vitro assays using a mitochrondrial extract. In the transfection experiments using the gene gun, we succeeded for the first time to introduce exogenous plasmid DNA into human mitochondria. The mtEGFP expressed by the transfected vectors could definitely be localized to the mitochondria of the cells. Transfections using magnetic particles as mediator could not be used, because the particles exhibit an autofluorescence which prevents a detection of the mtEGFP expression. An essential prerequisite for the transfection of mitochondria by mechanical methods like microinjection is the reversible induction of megamitochondria, since they could not be penetrated as small regular organelles. Acidification of the culture medium with sodium acetate or acetic acid led to mitochondria exhibiting almost the size of the nucleus, thus giving ideal conditions for microinjection. In the applied microinjection experiments using the mitochondrial expression vectors, cells displayed mitochondria with distinct green fluorescence. In summary, human mitochondria were transfected successfully for the first time with mitochondrial expression vectors. This is a fundamental step in the development of new therapies targeting mitochondrial myopathies. However, the transfection methods have to be optimized to achieve higher transfection efficiencies. KW - Mitochondrium KW - Heterologe Genexpression KW - Mitochondrien KW - mitochondria KW - gene expression KW - Transfektion KW - Mensch KW - Genexpression Y1 - 2011 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-85202 ER - TY - JOUR A1 - Fehrholz, Markus A1 - Seidenspinner, Silvia A1 - Kunzmann, Steffen T1 - Expression of surfactant protein B is dependent on cell density in H441 lung epithelial cells JF - PLoS ONE N2 - Background Expression of surfactant protein (SP)-B, which assures the structural stability of the pulmonary surfactant film, is influenced by various stimuli, including glucocorticoids; however, the role that cell-cell contact plays in SP-B transcription remains unknown. The aim of the current study was to investigate the impact of cell-cell contact on SP-B mRNA and mature SP-B expression in the lung epithelial cell line H441. Methods Different quantities of H441 cells per growth area were either left untreated or incubated with dexamethasone. The expression of SP-B, SP-B transcription factors, and tight junction proteins were determined by qPCR and immunoblotting. The influence of cell density on SP-B mRNA stability was investigated using the transcription inhibitor actinomycin D. Results SP-B mRNA and mature SP-B expression levels were significantly elevated in untreated and dexamethasone-treated H441 cells with increasing cell density. High cell density as a sole stimulus was found to barely have an impact on SP-B transcription factor and tight junction mRNA levels, while its stimulatory ability on SP-B mRNA expression could be mimicked using SP-B-negative cells. SP-B mRNA stability was significantly increased in high-density cells, but not by dexamethasone alone. Conclusion SP-B expression in H441 cells is dependent on cell-cell contact, which increases mRNA stability and thereby potentiates the glucocorticoid-mediated induction of transcription. Loss of cell integrity might contribute to reduced SP-B secretion in damaged lung cells via downregulation of SP-B transcription. Cell density-mediated effects should thus receive greater attention in future cell culture-based research. KW - messenger RNA KW - surfactants KW - epithelial cells KW - transcription factors KW - gene expression KW - tight junctions KW - adenocarcinoma of the lung KW - immunoblotting Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-158291 VL - 12 IS - 9 ER - TY - JOUR A1 - Nono, Justin Komguep A1 - Pletinckx, Katrien A1 - Lutz, Manfred B. A1 - Brehm, Klaus T1 - Excretory/Secretory-Products of Echinococcus multilocularis Larvae Induce Apoptosis and Tolerogenic Properties in Dendritic Cells In Vitro JF - PLoS Neglected Tropical Diseases N2 - Background: Alveolar echinococcosis, caused by Echinococcus multilocularis larvae, is a chronic disease associated with considerable modulation of the host immune response. Dendritic cells (DC) are key effectors in shaping the immune response and among the first cells encountered by the parasite during an infection. Although it is assumed that E. multilocularis, by excretory/secretory (E/S)-products, specifically affects DC to deviate immune responses, little information is available on the molecular nature of respective E/S-products and their mode of action. Methodology/Principal Findings: We established cultivation systems for exposing DC to live material from early (oncosphere), chronic (metacestode) and late (protoscolex) infectious stages. When co-incubated with Echinococcus primary cells, representing the invading oncosphere, or metacestode vesicles, a significant proportion of DC underwent apoptosis and the surviving DC failed to mature. In contrast, DC exposed to protoscoleces upregulated maturation markers and did not undergo apoptosis. After pre-incubation with primary cells and metacestode vesicles, DC showed a strongly impaired ability to be activated by the TLR ligand LPS, which was not observed in DC pre-treated with protoscolex E/S-products. While none of the larvae induced the secretion of pro-inflammatory IL-12p70, the production of immunosuppressive IL-10 was elevated in response to primary cell E/S-products. Finally, upon incubation with DC and naive T-cells, E/S-products from metacestode vesicles led to a significant expansion of Foxp3+ T cells in vitro. Conclusions: This is the first report on the induction of apoptosis in DC by cestode E/S-products. Our data indicate that the early infective stage of E. multilocularis is a strong inducer of tolerance in DC, which is most probably important for generating an immunosuppressive environment at an infection phase in which the parasite is highly vulnerable to host attacks. The induction of CD4+CD25+Foxp3+ T cells through metacestode E/S-products suggests that these cells fulfill an important role for parasite persistence during chronic echinococcosis. KW - granulosus KW - hydatid disease KW - metacestode vesicles KW - antigen-B KW - alveoar echinococcosis KW - TGF-BETA KW - regulatory T cells KW - gene expression KW - Brugia Malayi KW - TNF-alpha Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-134280 VL - 6 IS - 2 ER - TY - THES A1 - Brambrink, Tobias T1 - Entwicklung und Evaluierung eines Verfahrens zur Genexpressionsanalyse bei individuellen präimplantatorischen Säugerembryonen über die cDNA-Array-Technologie T1 - Development and evaluation of a methodology for cDNA-array gene expression profiling in individual mammalian preimplantation embryos N2 - Untersuchungen der Transkriptionsebene individueller präimplantatorischer Embryonalstadien können wertvolle Informationen über den physiologischen Status der betrachteten Embryonen, die z.B. zur Verbesserung der Systeme zur In vitro-Produktion von Embryonen genutzt werden können, liefern. Bisher fehlte es jedoch an einer geeigneten Technologie, um eine große Anzahl von Transkripten in einzelnen Embryonen zu erfassen. Zielsetzung der vorliegenden Arbeit war es, ein Verfahren zur globalen Amplifikation embryonaler mRNA-Präparationen zu entwickeln, das die Analyse der Transkriptionsebene einzelner präimplantatorischer Embryonalstadien über die cDNA-Array-Technologie ermöglicht. Dazu wurde die Strategie gewählt, zwei bereits etablierte Amplifikationsverfahren, Polymerasekettenreaktion und In vitro-Transkription, zu kombinieren, um so synergistische Effekte beider Verfahren zu nutzen. Die Evaluierung des entwickelten Verfahrens zeigte eine hohe Reproduzierbarkeit der erhaltenen Genexpressionsdaten und belegte, dass die relativen Mengenverhältnisse einzelner mRNA-Spezies zueinander während der globalen mRNA-Amplifikation nur unwesentlich verändert wurden. Die entwickelte Methodik ist somit geeignet, komplexe Genexpressionsprofile einzelner Blastozysten zu erstellen und Unterschiede in der Expressionsstärke einzelner Transkripte zu detektieren. Es konnte weiterhin gezeigt werden, dass es möglich ist, über heterologe Hybridisierung Genexpressionsprofile boviner Blastozysten mit cDNA-Arrays, die murine Probensequenzen enthalten, reproduzierbar darzustellen. Neben der Detektion individueller Unterschiede in den Genexpressionsprofilen diverser muriner Embryonalstadien und boviner Blastozysten lag ein Schwerpunkt dieser Arbeit in der Untersuchung der Auswirkungen verschiedener in vitro-Produktionssysteme auf die embryonale Genexpression. Die erhaltenen cDNA-Array Expressionsdaten muriner Oozyten, Zweizeller und Blastozysten befanden sich dabei in Übereinstimmung mit Daten früherer Publikationen anderer Arbeitsgruppen. Genexpressionsprofile in vitro fertilisierter boviner Blastozysten ließen eine Beurteilung der Auswirkungen unterschiedlicher Proteinsupplemente des Kulturmediums auf die embryonale Genexpression zu. Im Rahmen dieser Arbeit wurden zum ersten Mal Genexpressionsprofile einzelner präimplantatorischer Säugerembryonen über cDNA-Array-Analyse erstellt. Die entwickelte Technologie ermöglicht es -bei Verwendung entsprechender cDNA-Array-Systeme-, eine theoretisch unbegrenzte Zahl von Transkripten in individuellen Säugerembryonen semiquantitativ zu erfassen. Dies ist ein wichtiger Schritt hin zu einem besseren Verständnis komplexer Regulationsabläufe während der frühen Embryonalentwicklung und einer besseren Beurteilung der Lebensfähigkeit und Entwicklungskompetenz in vitro produzierter Embryonen, was für die Verbesserung von In vitro-Produktionssystemen für Embryonen sowohl bei Tieren als auch beim Menschen unerlässlich ist. N2 - Transcript expression profiling in single mammalian embryos can provide valuable information about their physiological status and developmental competence that can be exploited to improve systems for embryo in vitro production. Conventional methodologies such as RT-PCR limit the number of transcripts that can be quantitatively screened in a single embryo to only a few. The purpose of this study was to develop and evaluate a methodology for the global amplification of mRNA that permits cDNA-array analysis of individual preimplantation embryos. For this purpose, two conventional amplification procedures – polymerase chain reaction and in vitro transcription – were combined to a global amplification procedure. Evaluation of methodology developed revealed that data produced were high reproducible and that the relative transcript levels found in the original (non-amplified) sample were maintained throughout the amplification process. Thus, this method is suitable to generate complex gene expression profiles and to detect differentially expressed transcripts in individual mammalian embryos. Furthermore, this study demonstrates that expression profiles can reproducibly be produced from bovine embryos using arrays consisting of murine cDNA-probes by heterologous hybridization. The focus of this study was to establish a methodology to detect differentially expressed genes in different murine developmental stages and in bovine embryos derived from different in vitro production systems. The data obtained from murine oocyte, 2-cell stage and blastocyst expression profiles were in agreement with data previously published by other groups. Expression profiles from bovine in vitro fertilized embryos cultured in different media revealed effects of different media protein supplementation on embryonic gene expression. In this study, for the first time, gene expression profiles were generated from single mammalian preimplantation embryos via model cDNA-arrays. Using state-of-the-art cDNA-arrays this technology features the quantitative screening of a virtually unlimited number of transcripts in individual blastocysts and cleavage stages. Complex expression profiles of preimplantation embryos will contribute to the understanding of the molecular mechanisms essential for embryogenesis. This is crucial for the improvement of systems for in vitro production of mammalian embryos. KW - Embryo KW - Säugetiere KW - Array-Technologie KW - Messenger-RNS KW - Genexpression KW - Embryo KW - Genexpression KW - cDNA-Arrays KW - mRNA-Amplifikation KW - embryo KW - gene expression KW - cDNA-arrays KW - mRNA-amplification Y1 - 2002 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-1787 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 - THES A1 - Heintel, Timo Michael T1 - Einfluss von Stickstoffmonoxid auf die Genexpression humaner artikulärer Chondrozyten während Expansion und Redifferenzierung in einem in-vitro-Modell T1 - Influence of nitric oxide on the gene expression of human articular chondrocytes during expansion and redifferentiation in an in vitro-modell N2 - Bei der Kultivierung humaner artikulärer Chondrozyten für eine mögliche therapeutische Anwendung gilt es, deren besondere zellphysiologische Eigenschaften zu berücksichtigen, um ein zell- und molekularbiologisch hochwertiges Transplantat erzielen zu können. Stickstoffmonoxid (NO) gilt als ein wichtiger Faktor für die Homöostase der chondrogenen Extrazellulärmatrix, der für die Funktion des hyalinen Gelenkknorpels entscheidenden Gewebekomponente. Es stellt bisherigen Untersuchungen nach einen wichtigen Regulator im sensiblen Gleichgewicht zwischen der Synthese knorpelspezifischer Matrixproteine und dem Matrixabbau dar. Trotz dieser Bedeutung ist das Wissen über die Expression der NO-generierenden Enzyme in humanen artikulären Chondrozyten, insbesondere unter Kulturbedingungen, sehr begrenzt. Des Weiteren fehlen Erkenntnisse über den Einfluss von NO auf den Differenzierungsstatus dieser Zellen. Ziel der vorliegenden Arbeit war daher die Charakterisierung der Genexpression adulter Gelenkknorpelzellen während deren Expansion und anschließender Redifferenzierung in einem in vitro-Modell. Das Hauptaugenmerk wurde hierbei auf die 3 NOS-Isoformen sowie die beiden Matrixproteine Kollagen Typ II und Aggrecan gelegt. In Zusatzversuchen wurde die Bedeutung von NO für den Metabolismus sowie für Differenzierungsvorgänge humaner artikulärer Chondrozyten untersucht. Hierbei sollten funktionelle Zusammenhänge aufgezeigt und regulative Abhängigkeiten auf der Ebene der Transkription identifiziert werden. Humane artikuläre Chondrozyten wurden hierfür unter standardisierten Bedingungen enzymatisch aus Knorpelgewebe von Femurköpfen isoliert. Nach Expansion der Zellen in zweidimensionaler Monolayerkultur wurden die amplifizierten Zellen in Form dreidimensionaler Zellaggregate in einem chondrogenen Differenzierungsmedium rekultiviert. Veränderungen des zellulären Phänotyps wurden morphologisch, histochemisch, immunhistochemisch und mittels RT-PCR auf Genexpressionsebene verfolgt. Im Verlauf der Expansion konnte eine funktionelle und morphologische Dedifferenzierung der Chondrozyten dokumentiert werden. Durch 21tägige Rekultivierung in einem definierten chondrogenen Differenzierungsmedium konnten die Zellen ihre, zuvor verloren gegangenen knorpelspezifischen Eigenschaften wieder ausbilden (Redifferenzierung). Die Analyse der Genexpression der NOS-Isoformen humaner artikulärer Chondrozyten auf RNA-Ebene ergab neben der, in der Literatur bereits beschriebenen induzierbaren NOS die Expression zweier weiterer Isoformen, der neuronalen und der endothelialen NOS. In weiteren Versuchen wurde der Effekt verschiedener Mediatoren auf die Genexpression der Gelenkknorpelzellen beobachtet. So wurden Zellaggregate während verschiedener Phasen der Redifferenzierung mit rhIL-1 beta bzw. rhTNF alpha stimuliert. Die Chondrozyten reagierten darauf mit einer starker Induktion der induzierbaren NOS sowie mit einem konsekutiven Anstieg der NO-Freisetzung. Die eNOS-Expression wurde negativ reguliert. Auf die Konzentration der nNOS-Transkripte hatten beide Zytokine keinen messbaren Einfluss. Zudem konnte auf diesen Reiz hin eine drastische Reduktion der Kollagen Typ II und Aggrecan-Expression festgestellt werden. In Zusatzversuchen, bei denen u.a. ein NO-Donor und ein NOS-Inhibitor zum Einsatz kamen wurde dieser Effekt genauer erforscht. Aus den gewonnenen Ergebnissen kann geschlossen werden, dass der Effekt von IL-1 beta und TNF alpha auf die Synthese der beiden wichtigen Matrixproteine Kollagen Typ II und Aggrecan zumindest teilweise über NO vermittelt wird. In mehren Versuchsreihen gelang es des Weiteren die besondere Bedeutung von NO für die Zelldifferenzierung zu belegen. Die Modifikation des verwendeten chondrogenen Differenzierungsmediums durch Zusatz des NOS-Inhibitors NG-Amino-L-Arginin (L-NAA) führte zu einer deutlich früheren bzw. stärkeren Expression der beiden chondrogenen Markergene Kollagen Typ II und Aggrecan. N2 - Wird nachgereicht! KW - Chondrozyten KW - Stickstoffmonoxid KW - Genexpression KW - Expansion KW - Redifferenzierung KW - chondrocytes KW - nitric oxide KW - gene expression KW - expansion KW - redifferentiation Y1 - 2006 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-20456 ER - TY - JOUR A1 - Ceteci, Fatih A1 - Ceteci, Semra A1 - Zanucco, Emanuele A1 - Thakur, Chitra A1 - Becker, Matthias A1 - El-Nikhely, Nefertiti A1 - Fink, Ludger A1 - Seeger, Werner A1 - Savai, Rajkumar A1 - Rapp, Ulf R. T1 - E-Cadherin Controls Bronchiolar Progenitor Cells and Onset of Preneoplastic Lesions in Mice JF - Neoplasia N2 - Although progenitor cells of the conducting airway have been spatially localized and some insights have been gained regarding their molecular phenotype, relatively little is known about the mechanisms regulating their maintenance, activation, and differentiation. This study investigates the potential roles of E-cadherin in mouse Clara cells, as these cells were shown to represent the progenitor/stem cells of the conducting airways and have been implicated as the cell of origin of human non-small cell lung cancer. Postnatal inactivation of E-cadherin affected Clara cell differentiation and compromised airway regeneration under injury conditions. In steady-state adult lung, overexpression of the dominant negative E-cadherin led to an expansion of the bronchiolar stem cells and decreased differentiation concomitant with canonical Wnt signaling activation. Expansion of the bronchiolar stem cell pool was associated with an incessant proliferation of neuroepithelial body-associated Clara cells that ultimately gave rise to bronchiolar hyperplasia. Despite progressive hyperplasia, only a minority of the mice developed pulmonary solid tumors, suggesting that the loss of E-cadherin function leads to tumor formation when additional mutations are sustained. The present study reveals that E-cadherin plays a critical role in the regulation of proliferation and homeostasis of the epithelial cells lining the conducting airways. KW - injury KW - lung cancer KW - stem cells KW - clara cell KW - gene expression KW - basal cell KW - in vivo KW - epithelium KW - airway KW - renewal Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-135407 VL - 14 IS - 12 ER - TY - JOUR A1 - Afonso-Grunz, Fabian A1 - Hoffmeier, Klaus A1 - Müller, Sören A1 - Westermann, Alexander J. A1 - Rotter, Björn A1 - Vogel, Jörg A1 - Winter, Peter A1 - Kahl, Günter T1 - Dual 3'Seq using deepSuperSAGE uncovers transcriptomes of interacting Salmonella enterica Typhimurium and human host cells JF - BMC Genomics N2 - Background: The interaction of eukaryotic host and prokaryotic pathogen cells is linked to specific changes in the cellular proteome, and consequently to infection-related gene expression patterns of the involved cells. To simultaneously assess the transcriptomes of both organisms during their interaction we developed dual 3'Seq, a tag-based sequencing protocol that allows for exact quantification of differentially expressed transcripts in interacting pro-and eukaryotic cells without prior fixation or physical disruption of the interaction. Results: Human epithelial cells were infected with Salmonella enterica Typhimurium as a model system for invasion of the intestinal epithelium, and the transcriptional response of the infected host cells together with the differential expression of invading and intracellular pathogen cells was determined by dual 3'Seq coupled with the next-generation sequencing-based transcriptome profiling technique deepSuperSAGE (deep Serial Analysis of Gene Expression). Annotation to reference transcriptomes comprising the operon structure of the employed S. enterica Typhimurium strain allowed for in silico separation of the interacting cells including quantification of polycistronic RNAs. Eighty-nine percent of the known loci are found to be transcribed in prokaryotic cells prior or subsequent to infection of the host, while 75% of all protein-coding loci are represented in the polyadenylated transcriptomes of human host cells. Conclusions: Dual 3'Seq was alternatively coupled to MACE (Massive Analysis of cDNA ends) to assess the advantages and drawbacks of a library preparation procedure that allows for sequencing of longer fragments. Additionally, the identified expression patterns of both organisms were validated by qRT-PCR using three independent biological replicates, which confirmed that RELB along with NFKB1 and NFKB2 are involved in the initial immune response of epithelial cells after infection with S. enterica Typhimurium. KW - complete genome sequence KW - secretion systems KW - RNA-Seq KW - deepSuperSAGE KW - transcriptome KW - gene expression KW - serovar Typhimurium KW - human macrophages KW - epithelial cells KW - infection KW - SuperSAGE KW - receptors KW - Dual 3'seq KW - MACE KW - tag based KW - simultaneous KW - genome wide KW - gene expression profiling KW - host pathogen interaction KW - Salmonella enterica Typhimurium strain SL1344 Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-143230 VL - 16 IS - 323 ER - TY - JOUR A1 - Fan, Ben A1 - Li, Lei A1 - Chao, Yanjie A1 - Förstner, Konrad A1 - Vogel, Jörg A1 - Borriss, Rainer A1 - Wu, Xiao-Qin T1 - dRNA-Seq Reveals Genomewide TSSs and Noncoding RNAs of Plant Beneficial Rhizobacterium Bacillus amyloliquefaciens FZB42 JF - PLoS One N2 - Bacillus amyloliquefaciens subsp. plantarum FZB42 is a representative of Gram-positive plant-growth-promoting rhizobacteria (PGPR) that inhabit plant root environments. In order to better understand the molecular mechanisms of bacteria-plant symbiosis, we have systematically analyzed the primary transcriptome of strain FZB42 grown under rhizospheremimicking conditions using differential RNA sequencing (dRNA-seq). Our analysis revealed 4,877 transcription start sites for protein-coding genes, identified genes differentially expressed under different growth conditions, and corrected many previously mis-annotated genes. We also identified a large number of riboswitches and cis-encoded antisense RNAs, as well as trans-encoded small noncoding RNAs that may play important roles in the gene regulation of Bacillus. Overall, our analyses provided a landscape of Bacillus primary transcriptome and improved the knowledge of rhizobacteria-host interactions. KW - gene expression KW - subtilis genome KW - enterica serovar thphimurium KW - small regulatory RNAs KW - binding protein HFQ KW - escherichia coli KW - messenger RNA KW - transcriptional landscape KW - mycobacterium tuberculosis KW - listeria monocytogenes Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-138369 VL - 10 IS - 11 ER - TY - THES A1 - Engelmann, Julia Cathérine T1 - DNA microarrays: applications and novel approaches for analysis and interpretation T1 - DNA Mikroarrays: Anwendungen und neue Ansätze für die Analyse und Interpretation N2 - In der vorliegenden Dissertation wird die Entwicklung eines phylogenetischen DNA Microarrays, die Analyse von mehreren Microarray-Genexpressionsdatensätzen und neue Ansätze für die Datenanalyse und Interpretation der Ergebnisse vorgestellt. Die Entwicklung und Analyse der Daten eines phylogenetischen DNA Microarrays wird in der ersten Publikation dargestellt. Ich konnte zeigen, dass die Spezies-Detektion mit phylogenetischen Microarrays durch die Datenanalyse mit einem linearen Regressionsansatz signifikant verbessert werden kann. Standard-Methoden haben bislang nur Signalintensitäten betrachtet und eine Spezies als an- oder abwesend bezeichnet, wenn die Signalintensität ihres Messpunktes oberhalb eines willkürlich gesetzten Schwellenwertes lag. Dieses Verfahren ist allerdings aufgrund von Kreuz-Hybridisierungen nicht auf sehr nah verwandte Spezies mit hoher Sequenzidentität anwendbar. Durch die Modellierung des Hybridisierungs und Kreuz-Hybridisierungsverhaltens mit einem linearen Regressionsmodell konnte ich zeigen, dass Spezies mit einer Sequenzähnlichkeit von 97% im Markergen immer noch unterschieden werden können. Ein weiterer Vorteil der Modellierung ist, dass auch Mischungen verschiedener Spezies zuverlässig vorhergesagt werden können. Theoretisch sind auch quantitative Vorhersagen mit diesem Modell möglich. Um die großen Datenmengen, die in öffentlichen Microarray-Datenbanken abgelegt sind besser nutzen zu können, bieten sich Meta-Analysen an. In der zweiten Publikation wird eine explorative Meta-Analyse auf Arabidopsis thaliana-Datensätzen vorgestellt. Mit der Analyse verschiedener Datensätze, die den Einfluss von Pflanzenhormonen, Pathogenen oder verschiedenen Mutationen auf die Genexpression untersucht haben, konnten die Datensätze anhand ihrer Genexpressionsprofile in drei große Gruppen eingeordnet werden: Experimente mit Indol-3-Essigsäure (IAA), mit Pathogenen und andere Experimente. Gene, die charakteristisch für die Gruppe der IAA-Datensätze beziehungsweise für die Gruppe der Pathogen-Datensätze sind, wurden näher betrachtet. Diese Gene hatten Funktionen, die bereits mit Pathogenbefall bzw. dem Einfluss von IAA in Verbindung gebracht wurden. Außerdem wurden Hypothesen über die Funktionen von bislang nicht annotierten Genen aufgestellt. In dieser Arbeit werden auch Primäranalysen von einzelnen Arabidopsis thaliana Genexpressions-Datensätzen vorgestellt. In der dritten Publikation wird ein Experiment beschrieben, das durchgeführt wurde um herauszufinden ob Mikrowellen-Strahlung einen Einfluss auf die Genexpression einer Zellkultur hat. Dazu wurden explorative Analysemethoden angewendet. Es wurden geringe aber signifikante Veränderungen in einer sehr kleinen Anzahl von Genen beobachtet, die experimentell bestätigt werden konnten. Die Funktionen der regulierten Gene und eine Meta-Analyse mit öffentlich zugänglichen Datensätzen einer Datenbank deuten darauf hin, dass die pflanzliche Zellkultur die Strahlung als eine Art Energiequelle ähnlich dem Licht wahrnimmt. Des weiteren wird in der vierten Publikation die funktionelle Analyse eines Arabidopsis thaliana Genexpressionsdatensatzes beschrieben. Die Analyse der Genexpressions eines pflanzlichen Tumores zeigte, dass er seinen Stoffwechsel von aerob und auxotroph auf anaerob und heterotroph umstellt. Gene der Photosynthese werden im Tumorgewebe reprimiert, Gene des Aminosäure- und Fettstoffwechsels, der Zellwand und Transportkanäle werden so reguliert, dass Wachstum und Entwicklung des Tumors gefördert werden. In der fünften Publikation in dieser Arbeit wird GEPAT (Genome Expression Pathway Analysis Tool) beschrieben. Es besteht aus einer Internet- Anwendung und einer Datenbank, die das einfache Hochladen von Datensätzen in die Datenbank und viele Möglichkeiten der Datenanalyse und die Integration anderer Datentypen erlaubt. In den folgenden zwei Publikationen (Publikation 6 und Publikation 7) wird GEPAT auf humane Microarray-Datensätze angewendet um Genexpressionsdaten mit weiteren Datentypen zu verknüpfen. Genexpressionsdaten und Daten aus vergleichender Genom-Hybridisierung (CGH) von primären Tumoren von 71 Mantel-Zell-Lymphom (MCL) Patienten ermöglichte die Ermittlung eines Prädiktors, der die Vorhersage der Überlebensdauer von Patienten gegenüber herkömmlichen Methoden verbessert. Die Analyse der CGH Daten zeigte, dass auch diese für die Vorhersage der Überlebensdauer geeignet sind. Für den Datensatz von Patienten mit großzellig diffusem B-Zell-Lymphom DLBCL konnte aus den Genexpressionsdaten ebenfalls ein neuer Prädiktor vorgeschlagen werden. Mit den zwischen lang und kurz überlebenden Patienten differentiell exprimierten Genen der MCL Patienten und mit den Genen, die zwischen den beiden Untergruppen von DLBCL reguliert sind, wurden Interaktionsnetzwerke gebildet. Diese zeigen, dass bei beiden Krebstypen Gene des Zellzyklus und der Proliferation zwischen Patienten mit kurzer und langer Überlebensdauer unterschiedlich reguliert sind. N2 - In this thesis, the development of a phylogenetic DNA microarray, the analysis of several gene expression microarray datasets and new approaches for improved data analysis and interpretation are described. In the first publication, the development and analysis of a phylogenetic microarray is presented. I could show that species detection with phylogenetic DNA microarrays can be significantly improved when the microarray data is analyzed with a linear regression modeling approach. Standard methods have so far relied on pure signal intensities of the array spots and a simple cutoff criterion was applied to call a species present or absent. This procedure is not applicable to very closely related species with high sequence similarity because cross-hybridization of non-target DNA renders species detection impossible based on signal intensities alone. By modeling hybridization and cross-hybridization with linear regression, as I have presented in this thesis, even species with a sequence similarity of 97% in the marker gene can be detected and distinguished from related species. Another advantage of the modeling approach over existing methods is that the model also performs well on mixtures of different species. In principle, also quantitative predictions can be made. To make better use of the large amounts of microarray data stored in public databases, meta-analysis approaches need to be developed. In the second publication, an explorative meta-analysis exemplified on Arabidopsis thaliana gene expression datasets is presented. Integrating datasets studying effects such as the influence of plant hormones, pathogens and different mutations on gene expression levels, clusters of similarly treated datasets could be found. From the clusters of pathogen-treated and indole-3-acetic acid (IAA) treated datasets, representative genes were selected which pointed to functions which had been associated with pathogen attack or IAA effects previously. Additionally, hypotheses about the functions of so far uncharacterized genes could be set up. Thus, this kind of meta-analysis could be used to propose gene functions and their regulation under different conditions. In this work, also primary data analysis of Arabidopsis thaliana datasets is presented. In the third publication, an experiment which was conducted to find out if microwave irradiation has an effect on the gene expression of a plant cell culture is described. During the first steps, the data analysis was carried out blinded and exploratory analysis methods were applied to find out if the irradiation had an effect on gene expression of plant cells. Small but statistically significant changes in a few genes were found and could be experimentally confirmed. From the functions of the regulated genes and a meta-analysis with publicly available microarray data, it could be suspected that the plant cell culture somehow perceived the irradiation as energy, similar to perceiving light rays. The fourth publication describes the functional analysis of another Arabidopsis thaliana gene expression dataset. The gene expression data of the plant tumor dataset pointed to a switch from a mainly aerobic, auxotrophic to an anaerobic and heterotrophic metabolism in the plant tumor. Genes involved in photosynthesis were found to be repressed in tumors; genes of amino acid and lipid metabolism, cell wall and solute transporters were regulated in a way that sustains tumor growth and development. Furthermore, in the fifth publication, GEPAT (Genome Expression Pathway Analysis Tool), a tool for the analysis and integration of microarray data with other data types, is described. It consists of a web application and database which allows comfortable data upload and data analysis. In later chapters of this thesis (publication 6 and publication 7), GEPAT is used to analyze human microarray datasets and to integrate results from gene expression analysis with other datatypes. Gene expression and comparative genomic hybridization data from 71 Mantle Cell Lymphoma (MCL) patients was analyzed and allowed proposing a seven gene predictor which facilitates survival predictions for patients compared to existing predictors. In this study, it was shown that CGH data can be used for survival predictions. For the dataset of Diffuse Large B-cell lymphoma (DLBCL) patients, an improved survival predictor could be found based on the gene expression data. From the genes differentially expressed between long and short surviving MCL patients as well as for regulated genes of DLBCL patients, interaction networks could be set up. They point to differences in regulation for cell cycle and proliferation genes between patients with good and bad prognosis. KW - Microarray KW - Differentielle Genexpression KW - Genexpression KW - Statistische Analyse KW - Cluster-Analyse KW - Datenanalyse KW - Explorative Datenanalyse KW - Non-Hodgkin-Lymphom KW - B-Zell-Lymphom KW - Metabolom KW - Tumorklassifikation KW - Tumor KW - Krebs KW - Schmalwa KW - phylogenetische Arrays KW - Interaktionsnetzwerke KW - lineare Regression KW - DNA microarray KW - gene expression KW - statistical analysis KW - clustering KW - classification KW - interaction networks Y1 - 2008 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-29747 ER - TY - JOUR A1 - Deeken, Rosalia A1 - Gohlke, Jochen A1 - Scholz, Claus-Juergen A1 - Kneitz, Susanne A1 - Weber, Dana A1 - Fuchs, Joerg A1 - Hedrich, Rainer T1 - DNA Methylation Mediated Control of Gene Expression Is Critical for Development of Crown Gall Tumors JF - PLoS Genetics N2 - Crown gall tumors develop after integration of the T-DNA of virulent Agrobacterium tumefaciens strains into the plant genome. Expression of the T-DNA–encoded oncogenes triggers proliferation and differentiation of transformed plant cells. Crown gall development is known to be accompanied by global changes in transcription, metabolite levels, and physiological processes. High levels of abscisic acid (ABA) in crown galls regulate expression of drought stress responsive genes and mediate drought stress acclimation, which is essential for wild-type-like tumor growth. An impact of epigenetic processes such as DNA methylation on crown gall development has been suggested; however, it has not yet been investigated comprehensively. In this study, the methylation pattern of Arabidopsis thaliana crown galls was analyzed on a genome-wide scale as well as at the single gene level. Bisulfite sequencing analysis revealed that the oncogenes Ipt, IaaH, and IaaM were unmethylated in crown galls. Nevertheless, the oncogenes were susceptible to siRNA–mediated methylation, which inhibited their expression and subsequently crown gall growth. Genome arrays, hybridized with methylated DNA obtained by immunoprecipitation, revealed a globally hypermethylated crown gall genome, while promoters were rather hypomethylated. Mutants with reduced non-CG methylation developed larger tumors than the wild-type controls, indicating that hypermethylation inhibits plant tumor growth. The differential methylation pattern of crown galls and the stem tissue from which they originate correlated with transcriptional changes. Genes known to be transcriptionally inhibited by ABA and methylated in crown galls became promoter methylated upon treatment of A. thaliana with ABA. This suggests that the high ABA levels in crown galls may mediate DNA methylation and regulate expression of genes involved in drought stress protection. In summary, our studies provide evidence that epigenetic processes regulate gene expression, physiological processes, and the development of crown gall tumors. KW - DNA methylation KW - DNA transcription KW - gene expression KW - oncogenes KW - plant genomics KW - sequence motif analysis KW - arabidopsis thaliana KW - agrobacterium tumefaciens Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96318 ER - TY - JOUR A1 - Schubert, Maria A1 - Spahn, Martin A1 - Kneitz, Susanne A1 - Scholz, Claus Jürgen A1 - Joniau, Steven A1 - Stroebel, Philipp A1 - Riedmiller, Hubertus A1 - Kneitz, Burkhard T1 - Distinct microRNA Expression Profile in Prostate Cancer Patients with Early Clinical Failure and the Impact of let-7 as Prognostic Marker in High-Risk Prostate Cancer JF - PLoS ONE N2 - Background The identification of additional prognostic markers to improve risk stratification and to avoid overtreatment is one of the most urgent clinical needs in prostate cancer (PCa). MicroRNAs, being important regulators of gene expression, are promising biomarkers in various cancer entities, though the impact as prognostic predictors in PCa is poorly understood. The aim of this study was to identify specific miRNAs as potential prognostic markers in high-risk PCa and to validate their clinical impact. Methodology and Principal Findings We performed miRNA-microarray analysis in a high-risk PCa study group selected by their clinical outcome (clinical progression free survival (CPFS) vs. clinical failure (CF)). We identified seven candidate miRNAs (let-7a/b/c, miR-515-3p/5p, -181b, -146b, and -361) that showed differential expression between both groups. Further qRT-PCR analysis revealed down-regulation of members of the let-7 family in the majority of a large, well-characterized high-risk PCa cohort (n = 98). Expression of let-7a/b/and -c was correlated to clinical outcome parameters of this group. While let-7a showed no association or correlation with clinical relevant data, let-7b and let-7c were associated with CF in PCa patients and functioned partially as independent prognostic marker. Validation of the data using an independent high-risk study cohort revealed that let-7b, but not let-7c, has impact as an independent prognostic marker for BCR and CF. Furthermore, we identified HMGA1, a non-histone protein, as a new target of let-7b and found correlation of let-7b down-regulation with HMGA1 over-expression in primary PCa samples. Conclusion Our findings define a distinct miRNA expression profile in PCa cases with early CF and identified let-7b as prognostic biomarker in high-risk PCa. This study highlights the importance of let-7b as tumor suppressor miRNA in high-risk PCa and presents a basis to improve individual therapy for high-risk PCa patients. KW - biomarkers KW - gene expression KW - gene targeting KW - luciferase KW - MircoRNA KW - microarrays KW - oncogenes KW - prostate cancer Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96825 ER - TY - JOUR A1 - Kreß, Luisa A1 - Egenolf, Nadine A1 - Sommer, Claudia A1 - Üçeyler, Nurcan T1 - Cytokine expression profiles in white blood cells of patients with small fiber neuropathy JF - BMC Neuroscience N2 - Background The role of cytokines in the pathophysiology, diagnosis, and prognosis of small fiber neuropathy (SFN) is incompletely understood. We studied expression profiles of selected pro- and anti-inflammatory cytokines in RNA from white blood cells (WBC) of patients with a medical history and a clinical phenotype suggestive for SFN and compared data with healthy controls. Methods We prospectively recruited 52 patients and 21 age- and sex-matched healthy controls. Study participants were characterized in detail and underwent complete neurological examination. Venous blood was drawn for routine and extended laboratory tests, and for WBC isolation. Systemic RNA expression profiles of the pro-inflammatory cytokines interleukin (IL)-1ß, IL-2, IL-8, tumor necrosis factor-alpha (TNF) and the anti-inflammatory cytokines IL-4, IL-10, transforming growth factor beta-1 (TGF) were analyzed. Protein levels of IL-2, IL-8, and TNF were measured in serum of patients and controls. Receiver operating characteristic (ROC)-curve analysis was used to determine the accuracy of IL-2, IL-8, and TNF in differentiating patients and controls. To compare the potential discriminatory efficacy of single versus combined cytokines, equality of different AUCs was tested. Results WBC gene expression of IL-2, IL-8, and TNF was higher in patients compared to healthy controls (IL-2: p = 0.02; IL-8: p = 0.009; TNF: p = 0.03) and discriminated between the groups (area under the curve (AUC) ≥ 0.68 for each cytokine) with highest diagnostic accuracy reached by combining the three cytokines (AUC = 0.81, sensitivity = 70%, specificity = 86%). Subgroup analysis revealed the following differences: IL-8 and TNF gene expression levels were higher in female patients compared to female controls (IL-8: p = 0.01; TNF: p = 0.03). The combination of TNF with IL-2 and TNF with IL-2 and IL-8 discriminated best between the study groups. IL-2 was higher expressed in patients with moderate pain compared to those with severe pain (p = 0.02). Patients with acral pain showed higher IL-10 gene expression compared to patients with generalized pain (p = 0.004). We further found a negative correlation between the relative gene expression of IL-2 and current pain intensity (p = 0.02). Serum protein levels of IL-2, IL-8, and TNF did not differ between patients and controls. Conclusions We identified higher systemic gene expression of IL-2, IL-8, and TNF in SFN patients than in controls, which may be of potential relevance for diagnostics and patient stratification. KW - gene expression KW - small fiber neuropathy KW - cytokines KW - white blood cells Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-300619 VL - 24 IS - 1 ER - TY - JOUR A1 - Pascoalino, Bruno A1 - Dindar, Gülcin A1 - Vieira-da-Rocha, João P. A1 - Machado, Carlos Renato A1 - Janzen, Christian J. A1 - Schenkman, Sergio T1 - Characterization of two different Asf1 histone chaperones with distinct cellular localizations and functions in Trypanosoma brucei JF - Nucleic Acids Research N2 - The anti-silencing function protein 1 (Asf1) is a chaperone that forms a complex with histones H3 and H4 facilitating dimer deposition and removal from chromatin. Most eukaryotes possess two different Asf1 chaperones but their specific functions are still unknown. Trypanosomes, a group of early-diverged eukaryotes, also have two, but more divergent Asf1 paralogs than Asf1 of higher eukaryotes. To unravel possible different functions, we characterized the two Asf1 proteins in Trypanosoma brucei. Asf1A is mainly localized in the cytosol but translocates to the nucleus in S phase. In contrast, Asf1B is predominantly localized in the nucleus, as described for other organisms. Cytosolic Asf1 knockdown results in accumulation of cells in early S phase of the cell cycle, whereas nuclear Asf1 knockdown arrests cells in S/G2 phase. Overexpression of cytosolic Asf1 increases the levels of histone H3 and H4 acetylation. In contrast to cytosolic Asf1, overexpression of nuclear Asf1 causes less pronounced growth defects in parasites exposed to genotoxic agents, prompting a function in chromatin remodeling in response to DNA damage. Only the cytosolic Asf1 interacts with recombinant H3/H4 dimers in vitro. These findings denote the early appearance in evolution of distinguishable functions for the two Asf1 chaperons in trypanosomes. KW - chromatin assembly factors KW - DNA-damage checkpoint KW - tousled-like kinases KW - saccharomyes cerevisiae KW - gene expression KW - acetyltransferase RTT109 KW - african trypanosomes KW - antigenetic variation KW - cycle regulation KW - nuclear import Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-117220 SN - 1362-4962 VL - 42 IS - 5 ER - TY - JOUR A1 - Schlereth, Katharina A1 - Heyl, Charlotte A1 - Krampitz, Anna-Maria A1 - Mernberger, Marco A1 - Finkernagel, Florian A1 - Scharfe, Maren A1 - Jarek, Michael A1 - Leich, Ellen A1 - Rosenwald, Andreas A1 - Stiewe, Thorsten T1 - Characterization of the p53 Cistrome - DNA Binding Cooperativity Dissects p53's Tumor Suppressor Functions JF - PLOS Genetics N2 - p53 protects us from cancer by transcriptionally regulating tumor suppressive programs designed to either prevent the development or clonal expansion of malignant cells. How p53 selects target genes in the genome in a context-and tissue-specific manner remains largely obscure. There is growing evidence that the ability of p53 to bind DNA in a cooperative manner prominently influences target gene selection with activation of the apoptosis program being completely dependent on DNA binding cooperativity. Here, we used ChIP-seq to comprehensively profile the cistrome of p53 mutants with reduced or increased cooperativity. The analysis highlighted a particular relevance of cooperativity for extending the p53 cistrome to non-canonical binding sequences characterized by deletions, spacer insertions and base mismatches. Furthermore, it revealed a striking functional separation of the cistrome on the basis of cooperativity; with low cooperativity genes being significantly enriched for cell cycle and high cooperativity genes for apoptotic functions. Importantly, expression of high but not low cooperativity genes was correlated with superior survival in breast cancer patients. Interestingly, in contrast to most p53-activated genes, p53-repressed genes did not commonly contain p53 binding elements. Nevertheless, both the degree of gene activation and repression were cooperativity-dependent, suggesting that p53-mediated gene repression is largely indirect and mediated by cooperativity-dependently transactivated gene products such as CDKN1A, E2F7 and non-coding RNAs. Since both activation of apoptosis genes with non-canonical response elements and repression of pro-survival genes are crucial for p53's apoptotic activity, the cistrome analysis comprehensively explains why p53-induced apoptosis, but not cell cycle arrest, strongly depends on the intermolecular cooperation of p53 molecules as a possible safeguard mechanism protecting from accidental cell killing. KW - cell-cycle arrest KW - gene expression KW - breast cancer KW - human genome KW - transcriptional repression KW - consensus DNA KW - in-vivo KW - apoptosis KW - network KW - damage Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-127579 SN - 1553-7404 VL - 9 IS - 8 ER - TY - JOUR A1 - Schul, Daniela A1 - Schmitt, Alexandra A1 - Regneri, Janine A1 - Schartl, Manfred A1 - Wagner, Toni Ulrich T1 - Bursted BMP Triggered Receptor Kinase Activity Drives Smad1 Mediated Long-Term Target Gene Oscillation in c2c12 Cells JF - PLoS ONE N2 - Bone Morphogenetic Proteins (BMPs) are important growth factors that regulate many cellular processes. During embryogenesis they act as morphogens and play a critical role during organ development. They influence cell fates via concentration-gradients in the embryos where cells transduce this extracellular information into gene expression profiles and cell fate decisions. How receiving cells decode and quantify BMP2/4 signals is hardly understood. There is little data on the quantitative relationships between signal input, transducing molecules, their states and location, and ultimately their ability to integrate graded systemic inputs and generate qualitative responses. Understanding this signaling network on a quantitative level should be considered a prerequisite for efficient pathway modulation, as the BMP pathway is a prime target for therapeutic invention. Hence, we quantified the spatial distribution of the main signal transducer of the BMP2/4 pathway in response to different types and levels of stimuli in c2c12 cells. We found that the subcellular localization of Smad1 is independent of ligand concentration. In contrast, Smad1 phosphorylation levels relate proportionally to BMP2 ligand concentrations and they are entirely located in the nucleus. Interestingly, we found that BMP2 stimulates target gene expression in non-linear, wave-like forms. Amplitudes showed a clear concentration-dependency, for sustained and transient stimulation. We found that even burst-stimulation triggers gene-expression wave-like modulations that are detectable for at least 30 h. Finally, we show here that target gene expression oscillations depend on receptor kinase activity, as the kinase drives further expression pulses without receptor reactivation and the target gene expression breaks off after inhibitor treatment in c2c12 cells. KW - gene expression KW - BMP signaling KW - SMAD signaling KW - genetic oscillators KW - cell fusion KW - DNA-binding proteins KW - luciferase KW - kinase inhibitors Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-130131 VL - 8 IS - 4 ER - TY - JOUR A1 - Tilstam, Pathricia V. A1 - Gijbels, Marion J. A1 - Habbeddine, Mohamed A1 - Cudejko, Celine A1 - Asare, Yaw A1 - Theelen, Wendy A1 - Zhou, Baixue A1 - Döring, Yvonne A1 - Drechsler, Maik A1 - Pawig, Lukas A1 - Simsekyilmaz, Sakine A1 - Koenen, Rory R. A1 - de Winther, Menno P. J. A1 - Lawrence, Toby A1 - Bernhagen, Jürgen A1 - Zernecke, Alma A1 - Weber, Christian A1 - Noels, Heidi T1 - Bone Marrow-Specific Knock-In of a Non-Activatable Ikkα Kinase Mutant Influences Haematopoiesis but Not Atherosclerosis in Apoe-Deficient Mice JF - PLOS ONE N2 - Background: The Ikkα kinase, a subunit of the NF-kappa B-activating IKK complex, has emerged as an important regulator of inflammatory gene expression. However, the role of Ikkα-mediated phosphorylation in haematopoiesis and atherogenesis remains unexplored. In this study, we investigated the effect of a bone marrow (BM)-specific activation-resistant Ikk alpha mutant knock-in on haematopoiesis and atherosclerosis in mice. Methods and Results: Apolipoprotein E (Apoe)-deficient mice were transplanted with BM carrying an activation-resistant Ikkα gene (Ikkα(AA/AA) Apoe(-/-)) or with Ikkα(+/+) Apoe(-/-) BM as control and were fed a high-cholesterol diet for 8 or 13 weeks. Interestingly, haematopoietic profiling by flow cytometry revealed a significant decrease in B-cells, regulatory T-cells and effector memory T-cells in Ikkα(AA/AA) Apoe(-/-) BM-chimeras, whereas the naive T-cell population was increased. Surprisingly, no differences were observed in the size, stage or cellular composition of atherosclerotic lesions in the aorta and aortic root of Ikkα(AA/AA) Apoe(-/-) vs Ikkα(+/+) Apoe(-/-) BM-transplanted mice, as shown by histological and immunofluorescent stainings. Necrotic core sizes, apoptosis, and intracellular lipid deposits in aortic root lesions were unaltered. In vitro, BM-derived macrophages from Ikkα(AA/AA) Apoe(-/-) vs Ikkα(+/+) Apoe(-/-) mice did not show significant differences in the uptake of oxidized low-density lipoproteins (oxLDL), and, with the exception of Il-12, the secretion of inflammatory proteins in conditions of Tnf-α or oxLDL stimulation was not significantly altered. Furthermore, serum levels of inflammatory proteins as measured with a cytokine bead array were comparable. Conclusion: Our data reveal an important and previously unrecognized role of haematopoietic Ikkα kinase activation in the homeostasis of B-cells and regulatory T-cells. However, transplantation of Ikkα AA mutant BM did not affect atherosclerosis in Apoe(-/-) mice. This suggests that the diverse functions of Ikkα in haematopoietic cells may counterbalance each other or may not be strong enough to influence atherogenesis, and reveals that targeting haematopoietic Ikkα kinase activity alone does not represent a therapeutic approach. KW - NF-KAPPA-B KW - regulatory T cells KW - indoleamine 2,3-dioxygenase KW - dendritic cells KW - gene expression KW - increases atherosclersosis KW - receptor KW - inhibition KW - pathway KW - beta Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-117450 VL - 9 IS - 2 ER - TY - JOUR A1 - Aukema, Sietse M. A1 - Kreuz, Markus A1 - Kohler, Christian W. A1 - Rosolowski, Maciej A1 - Hasenclever, Dirk A1 - Hummel, Michael A1 - Küppers, Ralf A1 - Lenze, Diddo A1 - Ott, German A1 - Pott, Christiane A1 - Richter, Julia A1 - Rosenwald, Andreas A1 - Szczepanowski, Monika A1 - Schwaenen, Carsten A1 - Stein, Harald A1 - Trautmann, Heiko A1 - Wessendorf, Swen A1 - Trümper, Lorenz A1 - Loeffler, Markus A1 - Spang, Rainer A1 - Kluin, Philip M. A1 - Klapper, Wolfram A1 - Siebert, Reiner T1 - Biological characterization of adult MYC-translocation-positive mature B-cell lymphomas other than molecular Burkitt lymphoma JF - Haematologica N2 - Chromosomal translocations affecting the MYC oncogene are the biological hallmark of Burkitt lymphomas but also occur in a subset of other mature B-cell lymphomas. If accompanied by a chromosomal break targeting the BCL2 and/or BCL6 oncogene these MYC translocation-positive (MYC+) lymphomas are called double-hit lymphomas, otherwise the term single-hit lymphomas is applied. In order to characterize the biological features of these MYC+ lymphomas other than Burkitt lymphoma we explored, after exclusion of molecular Burkitt lymphoma as defined by gene expression profiling, the molecular, pathological and clinical aspects of 80 MYC-translocation-positive lymphomas (31 single-hit, 46 double-hit and 3 MYC+-lymphomas with unknown BCL6 status). Comparison of single-hit and double-hit lymphomas revealed no difference in MYC partner (IG/non-IG), genomic complexity, MYC expression or gene expression profile. Double-hit lymphomas more frequently showed a germinal center B-cell-like gene expression profile and had higher IGH and MYC mutation frequencies. Gene expression profiling revealed 130 differentially expressed genes between BCL6(+)/MYC+ and BCL2(+)/MYC+ double-hit lymphomas. BCL2(+)/MYC+ double-hit lymphomas more frequently showed a germinal center B-like gene expression profile. Analysis of all lymphomas according to MYC partner (IG/non-IG) revealed no substantial differences. In this series of lymphomas, in which immunochemotherapy was administered in only a minority of cases, single-hit and double-hit lymphomas had a similar poor outcome in contrast to the outcome of molecular Burkitt lymphoma and lymphomas without the MYC break. Our data suggest that, after excluding molecular Burkitt lymphoma and pediatric cases, MYC+ lymphomas are biologically quite homogeneous with single-hit and double-hit lymphomas as well as IG-MYC and non-IG-MYC+ lymphomas sharing various molecular characteristics. KW - Rituximab plus KW - cyclophsophamide KW - c-myc KW - gene expression KW - genomic aberrations KW - follicular lymphoma KW - prognostic factor KW - poor prognosis KW - grade 3B KW - distinct Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-116882 SN - 1592-8721 VL - 99 IS - 4 ER - TY - THES A1 - Blenk, Steffen T1 - Bioinformatical analysis of B-cell lymphomas T1 - Bioinformatische Analyse von B-Zell Lymphomen N2 - Background: The frequency of the most observed cancer, Non Hodgkin Lymphoma (NHL), is further rising. Diffuse large B-cell lymphoma (DLBCL) is the most common of the NHLs. There are two subgroups of DLBCL with different gene expression patterns: ABC (“Activated B-like DLBCL”) and GCB (“Germinal Center B-like DLBCL”). Without therapy the patients often die within a few months, the ABC type exhibits the more aggressive behaviour. A further B-cell lymphoma is the Mantle cell lymphoma (MCL). It is rare and shows very poor prognosis. There is no cure yet. Methods: In this project these B-cell lymphomas were examined with methods from bioinformatics, to find new characteristics or undiscovered events on the molecular level. This would improve understanding and therapy of lymphomas. For this purpose we used survival, gene expression and comparative genomic hybridization (CGH) data. In some clinical studies, you get large data sets, from which one can reveal yet unknown trends. Results (MCL): The published proliferation signature correlates directly with survival. Exploratory analyses of gene expression and CGH data of MCL samples (n=71) revealed a valid grouping according to the median of the proliferation signature values. The second axis of correspondence analysis distinguishes between good and bad prognosis. Statistical testing (moderate t-test, Wilcoxon rank-sum test) showed differences in the cell cycle and delivered a network of kinases, which are responsible for the difference between good and bad prognosis. A set of seven genes (CENPE, CDC20, HPRT1, CDC2, BIRC5, ASPM, IGF2BP3) predicted, similarly well, survival patterns as proliferation signature with 20 genes. Furthermore, some bands could be associated with prognosis in the explorative analysis (chromosome 9: 9p24, 9p23, 9p22, 9p21, 9q33 and 9q34). Results (DLBCL): New normalization of gene expression data of DLBCL patients revealed better separation of risk groups by the 2002 published signature based predictor. We could achieve, similarly well, a separation with six genes. Exploratory analysis of gene expression data could confirm the subgroups ABC and GCB. We recognized a clear difference in early and late cell cycle stages of cell cycle genes, which can separate ABC and GCB. Classical lymphoma and best separating genes form a network, which can classify and explain the ABC and GCB groups. Together with gene sets which identify ABC and GCB we get a network, which can classify and explain the ABC and GCB groups (ASB13, BCL2, BCL6, BCL7A, CCND2, COL3A1, CTGF, FN1, FOXP1, IGHM, IRF4, LMO2, LRMP, MAPK10, MME, MYBL1, NEIL1 and SH3BP5; Altogether these findings are useful for diagnosis, prognosis and therapy (cytostatic drugs). N2 - Hintergrund: Die Häufigkeit von Non-Hodgkin-Lymphomen (NHL), den am meisten beobachteten Krebserkrankungen, steigt weiter an. Von den aggressiven Non-Hodgkin-Lymphomen (NHL) macht das “großzellige, diffuse B-Zell-Lymphom” (DLBCL) den größten Anteil aus. Durch Genexpressionsmuster wurden zwei Subtypen definiert: ACB (“Activated B-like DLBCL”) und GCB (“Germinal Center B-like DLBCL”). Die Patienten der Gruppe ABC sterben ohne Therapie oft innerhalb weniger Monate, weil der ABC Typ einen aggressiveren Krankheitsverlauf aufweist. Ein weiteres, von einer malignen Entartung der B-Lymphozyten ausgehendes Lymphom, ist das “Mantelzell Lymphom” (MCL). Es tritt selten auf und ist ebenfalls mit einer schlechten Prognose verbunden. Eine vollständige Heilung nach der Therapie ist sehr selten. Methoden: In diesem Projekt wurden diese B-zell Lymphome mit bioinformatischen Methoden untersucht, um auf molekularer Ebene neue Eigenschaften oder bisher unentdeckte Zusammenhänge zu finden. Das würde das Verständnis und damit auch die Therapie voranbringen. Dafür standen uns Überlebens-, Genexpressions- und chromosomale Aberrationsdaten zur Verfügung. Sie sind die bevorzugte Wahl der Mittel, um genetische Veränderungen in Tumorzellen zu bestimmen. Hierbei fallen oft große Datenmengen an, aus welchen man mit bioinformatischen Methoden vorher unerkannte Trends und Hinweise identifizieren kann. Ergebnisse (MCL): Explorative Analysen sowohl der Genexpressions- (zweite Hauptachse der Korrespondenz Analyse) als auch der chromosomalen Aberrationsdaten des Mantelzell-Lymphom zeigten uns hierbei, daß es trotz der linearen Korrelation zwischen der veröffentlichten Proliferationssignatur und der Überlebenszeit sinnvoll ist, in den Patienten (n=71) zwei Ausprägungen zu betrachten: Patienten mit schlechter und mit guter Prognose. Statistische Tests (moderate t-test, Wilcoxon rank-sum test) dieser beiden Typen zeigten Unterschiede im Zellzyklus und ein Netzwerk von Kinasen auf, welche für den Unterschied zwischen guter und schlechter Prognose verantwortlich sind. Sieben Gene (CENPE, CDC20, HPRT1, CDC2, BIRC5, ASPM, IGF2BP3) konnten gefunden werden, die eine ähnliche gute Prognose für Überlebenszeiten ermöglichen, wie eine früher veröffentlichte Proliferationssignatur mit 20 Genen. Außerdem konnten chromosomale Banden durch eine explorative Analyse mit der Prognose assoziiert werden (Chromosom 9: 9p24, 9p23, 9p22, 9p21, 9q33 and 9q34). Ergebnisse (DLBCL): Durch geeignete Normalisierung der Genexpressionsdaten von 248 DLBCL-Patienten trennte der Signatur basierte Predictor die Risikogruppen nun besser auf. Eine ähnlich gute Auftrennung konnte von uns sogar mit sechs Genen erreicht werden. Die explorative Analyse der Genexpressionsdaten konnte die Subtypen ABC und GCB als valide Gruppen bestätigen. In den Genen, die ABC und GCB unterscheiden, ergab sich eine Häufung in späten und frühen Zellzyklusstadien. Klassische Lymphommarker, neu aufgefundene spezielle Gene und Zellzyklusgene bilden ein Netzwerk, das die ABC und GCB Gruppen klassifizieren und Unterschiede in deren Regulation erklären kann (ASB13, BCL2, BCL6, BCL7A, CCND2, COL3A1, CTGF, FN1, FOXP1, IGHM, IRF4, LMO2, LRMP, MAPK10, MME, MYBL1, NEIL1 and SH3BP5. Dies ist auch für die Diagnose, Prognose und Therapie (Zytostatika) interessant. KW - Bioinformatik KW - Genexpression KW - Auswertung KW - B-Zell-Lymphom KW - Diffuses großzelliges B-Zell-Lymphom KW - Mantelzell-Lymphom KW - Bioinformatics KW - gene expression KW - B-cell lymphoma KW - Diffuse large B-cell lymphoma (DLBCL) KW - Mantle cell lymphoma (MCL) Y1 - 2007 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-27421 ER - TY - THES A1 - Schwarz, Ulrike T1 - Biochemische und Molekularbiologische Charakterisierung der Wechselwirkungen zwischen Humanen Thrombozyten und Endothelzellen T1 - Biochemical and Molecular Characterization of Interactions Between Human Platelets and Endothelial Cells N2 - Der Blutkreislauf ist als wichtigstes Transportsystem im menschlichen Körper essentiell für die Versorgung der Gewebe und Organe mit Sauerstoff, Nährstoffen, Hormonen etc. Zwei Zelltypen, die eine wichtige Rolle bei der Aufrechterhaltung eines funktionell intakten Blutgefäßsystems spielen, sind Thrombozyten, die zentralen Mediatoren der Blutgerinnung, und Endothelzellen, welche die luminale Seite der Gefäßwände auskleiden. Diese beiden Zellen sind aber auch wesentlich an der Pathologie der Atherosklerose und kardiovaskulärer Erkrankungen beteiligt. Durch direkte und indirekte Interaktionen beeinflussen sich diese beiden Zelltypen gegenseitig und regulieren ihre Aktivität. Im Rahmen dieser Arbeit wurde eine Analysenmethode entwickelt, welche den Funktionszustand der Thrombozyten quantitativ erfaßt. Sowohl die Aktivierung als auch die Hemmung humaner Thrombozyten wird durch die Phosphorylierung spezifischer Signalproteine reguliert. Basierend auf der Verwendung phosphorylierungsspezifischer Antikörper und der Durchflußzytometrie wurde eine Methode etabliert, welche die Proteinphosphorylierung auf Einzelzellebene erfaßt, schnell quantifizierbare Ergebnisse liefert und für die Analyse im Vollblut geeignet ist. Da die Sekretion von Endothelfaktoren den Phosphorylierungszustand dieser Proteine in den Thrombozyten beeinflußt, kann die Methode auch dazu verwendet werden, indirekt Rückschlüsse auf den Funktionszustand der Endothelzellen zu gewinnen. In einer ersten klinischen Anwendung wurde die Methode eingesetzt, um den Therapieverlauf der antithrombotischen Medikamente Ticlopidin und Clopidogrel, welche gezielt die ADP-induzierte Thrombozytenaktivierung hemmen, zu verfolgen und das Antwortverhalten von Patienten auf diese Medikamente zu messen. Mehrere Personen, bei denen Ticlopidin und Clopidogrel keine Wirkung zeigten, wurden gefunden, ein Hinweis darauf, daß eine Resistenz gegen Thienopyridine vorkommt. Es ist bekannt, daß Endothelfaktoren bestimmte Aspekte der Thrombozytenaktivierung hemmen. In dieser Arbeit wurde gezeigt, daß die Phosphorylierung der p38 und p42 Mitogen-aktivierten Proteinkinasen, die im Verlauf der Thrombozytenaktivierung von zahlreichen Agonisten induziert wird, ebenfalls durch die endothelialen Vasodilatatoren NO (Stickstoffmonoxid) und Prostaglandin gehemmt wurde. Außerdem hemmten diese Substanzen die Translokation der inflammatorischen Moleküle P-Selektin und CD40 Ligand (CD40L) aus intrazellulären Speicherorganellen auf die Thrombozytenoberfläche. P-Selektin und CD40L werden auf aktivierten Thrombozyten exprimiert und sind direkt an der Interaktion von Thrombozyten mit Leukozyten und Endothelzellen beteiligt. Um die Auswirkung von CD40L, P-Selektin und weiteren Faktoren aktivierter Thrombozyten auf humane Endothelzellen zu untersuchen, wurde mit Hilfe von cDNA-Arrays die differentielle Genexpression in Endothelzellen nach Koinkubation mit aktivierten Thrombozyten analysiert. Neben einer bereits bekannten Hochregulierung von Faktoren, die an inflammatorischen Prozessen beteiligt sind, wurde eine verstärkte Expression von Transkriptionsfaktoren (c-Jun, Egr1, CREB2), Wachstumsfaktoren (PDGF) sowie von Adhäsionsrezeptoren für extrazelluläre Matrixproteine (Integrin av, Integrin b1) gefunden. Diese Faktoren weisen darauf hin, daß aktivierte Thrombozyten die Migration und Proliferation der Endothelzellen anregen und damit die Wundheilung, aber auch pathophysiologische Prozesse wie die Ausbildung atherosklerotischer Plaques induzieren könnten. N2 - The blood circulation is the human body's main transport system and is essential for supplying tissues and organs with oxygen, nutrients, hormones, etc. Blood platelets, the central mediators of coagulation, and endothelial cells which line the inner wall of blood vessels, play important roles in the maintenance of functionally intact blood vessels. On the other hand, these cells also participate in the pathogenesis of atherosclerosis and cardiovascular diseases. These two cell types mutually influence each other and regulate their activity via direct and indirect interactions. In this work, a method which allows quantitative analysis of platelet function was developed. Platelet activation and inhibition is regulated by phosphorylation of specific signaling proteins. Based on the use of phosphorylation-specific antibodies and flow cytometry, a method was established which measures protein phosphorylation in single cells, gives fast and quantitative results, and is also suitable for analysis of whole blood samples. Since secretion of endothelial cell factors influences the phosphorylation state of these proteins, the method may also be used to get indirect information about the functional integrity of endothelial cells. In a first clinical application, this method was used to monitor the progression of a therapy with the anti-thrombotic drugs ticlopidine and clopidogrel which selectively inhibit ADP-induced platelet activation, and to determine the patients' responsiveness to these drugs. Several non-responders were identified, indicating the existence of a thienopyridine resistance. Endothelial cell factors are known to inhibit different aspects of platelet activation. In this work, phosphorylation of platelet p38 and p42 mitogen-activated protein kinases, which is induced by various platelet activators, was found to be inhibited by the endothelium-derived vasodilators nitric oxide (NO) and prostacyclin. Furthermore, these endothelial cell factors inhibited translocation of the inflammatory molecules P-selectin and CD40 ligand (CD40L) from intracellular granules to the platelet surface membrane. P-selectin and CD40L are expressed on activated platelets and are directly involved in the interaction of platelets with leukocytes and endothelial cells. To study effects of P-selectin, CD40L, and other parameters of activated platelets on human endothelial cells, cDNA Arrays were used to analyze differential gene expression in endothelial cells after coincubation with activated platelets. Besides the already known up-regulation of certain inflammatory factors, a number of additional genes which belong mainly to the group of transcription factors (c-Jun, Egr1, CREB2) and growth factors (PDGF) and of adhesion receptors for extracellular matrix proteins (integrin av, integrin b1) was found to be up-regulated by activated platelets. Expression of these genes indicates that activated platelets may induce migration and proliferation of endothelial cells and thereby initiate wound healing, but may also have pathophysiological effects like the development of atherosclerotic plaques. KW - Thrombozyt KW - Endothelzelle KW - Genexpression KW - Phosphorylierung KW - Signaltransduktion KW - Thrombozyten KW - Endothelzellen KW - Durchflußzytometrie KW - Proteinphosphorylierung KW - Signaltransduktion KW - Genexpression KW - cDNA-Arrays KW - Atherosklerose KW - platelets KW - endothelial cells KW - flow cytometry KW - protein phosphorylation KW - signal transduction KW - gene expression KW - cDNA arrays KW - atherosclerosis Y1 - 2001 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-2030 ER - TY - JOUR A1 - Gross, Henrik A1 - Hennard, Christine A1 - Masouris, Ilias A1 - Cassel, Christian A1 - Barth, Stephanie A1 - Stober-Grässer, Ute A1 - Mamiani, Alfredo A1 - Moritz, Bodo A1 - Ostareck, Dirk A1 - Ostareck-Lederer, Antje A1 - Neuenkirchen, Nils A1 - Fischer, Utz A1 - Deng, Wen A1 - Leonhardt, Heinrich A1 - Noessner, Elfriede A1 - Kremmer, Elisabeth A1 - Grässer, Friedrich A. T1 - Binding of the Heterogeneous Ribonucleoprotein K (hnRNP K) to the Epstein-Barr Virus Nuclear Antigen 2 (EBNA2) Enhances Viral LMP2A Expression JF - PLoS One N2 - The Epstein-Barr Virus (EBV) -encoded EBNA2 protein, which is essential for the in vitro transformation of B-lymphocytes, interferes with cellular processes by binding to proteins via conserved sequence motifs. Its Arginine-Glycine (RG) repeat element contains either symmetrically or asymmetrically di-methylated arginine residues (SDMA and ADMA, respectively). EBNA2 binds via its SDMA-modified RG-repeat to the survival motor neurons protein (SMN) and via the ADMA-RG-repeat to the NP9 protein of the human endogenous retrovirus K (HERV-K (HML-2) Type 1). The hypothesis of this work was that the methylated RG-repeat mimics an epitope shared with cellular proteins that is used for interaction with target structures. With monoclonal antibodies against the modified RG-repeat, we indeed identified cellular homologues that apparently have the same surface structure as methylated EBNA2. With the SDMA-specific antibodies, we precipitated the Sm protein D3 (SmD3) which, like EBNA2, binds via its SDMA-modified RG-repeat to SMN. With the ADMA-specific antibodies, we precipitated the heterogeneous ribonucleoprotein K (hnRNP K). Specific binding of the ADMA-antibody to hnRNP K was demonstrated using E. coli expressed/ADMA-methylated hnRNP K. In addition, we show that EBNA2 and hnRNP K form a complex in EBV-infected B-cells. Finally, hnRNP K, when co-expressed with EBNA2, strongly enhances viral latent membrane protein 2A (LMP2A) expression by an unknown mechanism as we did not detect a direct association of hnRNP K with DNA-bound EBNA2 in gel shift experiments. Our data support the notion that the methylated surface of EBNA2 mimics the surface structure of cellular proteins to interfere with or co-opt their functional properties. KW - SM proteins KW - protein argentine methyltranserase KW - motor-neuron protein KW - RNA-polymerase-II KW - messenger RNA KW - C-MYC KW - gene expression KW - splicing factor KW - down regulation KW - living cells Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-133707 VL - 7 IS - 8 ER - TY - JOUR A1 - Jazbutyte, Virginija A1 - Stumpner, Jan A1 - Redel, Andreas A1 - Lorenzen, Johan M. A1 - Roewer, Norbert A1 - Thum, Thomas A1 - Kehl, Franz T1 - Aromatase Inhibition Attenuates Desflurane-Induced Preconditioning against Acute Myocardial Infarction in Male Mouse Heart In Vivo JF - PLoS One N2 - The volatile anesthetic desflurane (DES) effectively reduces cardiac infarct size following experimental ischemia/reperfusion injury in the mouse heart. We hypothesized that endogenous estrogens play a role as mediators of desflurane-induced preconditioning against myocardial infarction. In this study, we tested the hypothesis that desflurane effects local estrogen synthesis by modulating enzyme aromatase expression and activity in the mouse heart. Aromatase metabolizes testosterone to 17b- estradiol (E2) and thereby significantly contributes to local estrogen synthesis. We tested aromatase effects in acute myocardial infarction model in male mice. The animals were randomized and subjected to four groups which were pre-treated with the selective aromatase inhibitor anastrozole (A group) and DES alone (DES group) or in combination (A+DES group) for 15 minutes prior to surgical intervention whereas the control group received 0.9% NaCl (CON group). All animals were subjected to 45 minutes ischemia following 180 minutes reperfusion. Anastrozole blocked DES induced preconditioning and increased infarct size compared to DES alone (37.94615.5% vs. 17.163.62%) without affecting area at risk and systemic hemodynamic parameters following ischemia/reperfusion. Protein localization studies revealed that aromatase was abundant in the murine cardiovascular system with the highest expression levels in endothelial and smooth muscle cells. Desflurane application at pharmacological concentrations efficiently upregulated aromatase expression in vivo and in vitro. We conclude that desflurane efficiently regulates aromatase expression and activity which might lead to increased local estrogen synthesis and thus preserve cellular integrity and reduce cardiac damage in an acute myocardial infarction model. KW - smooth muscle cells KW - estrogens KW - heart KW - anesthetics KW - immunostaining KW - endothelial cells KW - gene expression KW - myocardial infarction Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-151258 VL - 7 IS - 8 ER - TY - JOUR A1 - Huang, Bei A1 - Belharazem, Djeda A1 - Li, Li A1 - Kneitz, Susanne A1 - Schnabel, Philipp A. A1 - Rieker, Ralf J. A1 - Körner, Daniel A1 - Nix, Wilfried A1 - Schalke, Berthold A1 - Müller-Hermelink, Hans Konrad A1 - Ott, German A1 - Rosenwald, Andreas A1 - Ströbel, Philipp A1 - Marx, Alexander T1 - Anti-apoptotic signature in thymic squamous cell carcinomas – functional relevance of anti-apoptotic BIRC3 expression in the thymic carcinoma cell line 1889c JF - Frontiers in Oncology N2 - The molecular pathogenesis of thymomas and thymic arcinomas (TCs) is poorly understood and results of adjuvant therapy are unsatisfactory in case of metastatic disease and tumor recurrence. For these clinical settings, novel therapeutic strategies are urgently needed. Recently, limited sequencing efforts revealed that a broad spectrum of genes that play key roles in various common cancers are rarely affected in thymomas and TCs, suggesting that other oncogenic principles might be important.This made us re-analyze historic expression data obtained in a spectrumof thymomas and thymic squamous cell carcinomas (TSCCs) with a custom-made cDNA microarray. By cluster analysis, different anti-apoptotic signatures were detected in type B3 thymoma and TSCC, including overexpression of BIRC3 in TSCCs. This was confirmed by qRT-PCR in the original and an independent validation set of tumors. In contrast to several other cancer cell lines, the BIRC3-positive TSCC cell line, 1889c showed spontaneous apoptosis after BIRC3 knock-down. Targeting apoptosis genes is worth testing as therapeutic principle in TSCC. KW - gene expression KW - MTCH2 KW - targeted KW - myasthenia gravis KW - apoptosis KW - thymus KW - thymoma KW - thymic carcinoma Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-132214 VL - 3 IS - 316 ER - TY - JOUR A1 - Curtaz, Carolin J. A1 - Reifschläger, Leonie A1 - Strähle, Linus A1 - Feldheim, Jonas A1 - Feldheim, Julia J. A1 - Schmitt, Constanze A1 - Kiesel, Matthias A1 - Herbert, Saskia-Laureen A1 - Wöckel, Achim A1 - Meybohm, Patrick A1 - Burek, Malgorzata T1 - Analysis of microRNAs in exosomes of breast cancer patients in search of molecular prognostic factors in brain metastases JF - International Journal of Molecular Sciences N2 - Brain metastases are the most severe tumorous spread during breast cancer disease. They are associated with a limited quality of life and a very poor overall survival. A subtype of extracellular vesicles, exosomes, are sequestered by all kinds of cells, including tumor cells, and play a role in cell-cell communication. Exosomes contain, among others, microRNAs (miRs). Exosomes can be taken up by other cells in the body, and their active molecules can affect the cellular process in target cells. Tumor-secreted exosomes can affect the integrity of the blood-brain barrier (BBB) and have an impact on brain metastases forming. Serum samples from healthy donors, breast cancer patients with primary tumors, or with brain, bone, or visceral metastases were used to isolate exosomes and exosomal miRs. Exosomes expressed exosomal markers CD63 and CD9, and their amount did not vary significantly between groups, as shown by Western blot and ELISA. The selected 48 miRs were detected using real-time PCR. Area under the receiver-operating characteristic curve (AUC) was used to evaluate the diagnostic accuracy. We identified two miRs with the potential to serve as prognostic markers for brain metastases. Hsa-miR-576-3p was significantly upregulated, and hsa-miR-130a-3p was significantly downregulated in exosomes from breast cancer patients with cerebral metastases with AUC: 0.705 and 0.699, respectively. Furthermore, correlation of miR levels with tumor markers revealed that hsa-miR-340-5p levels were significantly correlated with the percentage of Ki67-positive tumor cells, while hsa-miR-342-3p levels were inversely correlated with tumor staging. Analysis of the expression levels of miRs in serum exosomes from breast cancer patients has the potential to identify new, non-invasive, blood-borne prognostic molecular markers to predict the potential for brain metastasis in breast cancer. Additional functional analyzes and careful validation of the identified markers are required before their potential future diagnostic use. KW - breast cancer KW - breast cancer metastases KW - blood-brain barrier KW - patient serum KW - exosomes KW - microRNA KW - gene expression KW - prognostic marker Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-284476 SN - 1422-0067 VL - 23 IS - 7 ER - TY - THES A1 - Hock, Matthias T1 - Analyse der NFATc1-Genexpression durch eGFP-BAC-Reportermäuse T1 - Analysis of NFATc1 gene expression using eGFP-BAC reporter mice N2 - In Lymphozyten wird nach Antigenaktivierung die Expression des Nfatc1-Gens durch Aktivierung des P1-Promoters stark induziert. Dagegen ist die, durch den Promoter P2 vermittelte Expression ebenso wie die der anderen NFAT Faktoren c2 und c3 konstitutiv. Die Akkumulation der dabei gebildeten Isoform NFATc1/αA ist sowohl für Effektorfunktionen wie die Zytokinproduktion sowie die Proliferation und das Überleben der aktivierten Zellen wichtig (Chuvpilo et al., 2002). Um die Expression des Nfatc1-Gens auf Einzelzellebene messen zu können, wurden BAC (bacterial artificial chromosom) transgene Mauslinien generiert, die einen 210kb großen Bereich des Nfatc1-Gens der Maus enthalten. In diesen Lokus wurde ein eGFP-Reportergen innerhalb des allen Isoformen gemeinsamen, dritten Exons integriert. In dieser Arbeit wird durch semiquantitative RT-PCR-Experimente von Gesamt-Milzzellen und TLymphozyten gezeigt, dass in den B6/NFATc1-eGFP-BAC-Reportermäusen die Expression der eGFP-cDNA analog zum endogenen Nfatc1-Lokus der Kontrolle der beiden Promotoren P1 und P2 unterliegt. In Western Blot Experimenten wird in diesen Zellen mittels eines NFATc1α-spezifischen Antikörpers eine induzierbare und CsA-sensitive α-GFP-Isoform - vergleichbar mit der endogenen NFATc1α-Isoform - nachgewiesen. Gleichzeitig zeigen NFATc1-Antikörper das konstitutiv exprimierte GFPβ-Protein. Die Korrelation der Expression von NFATc1 und GFP auf mRNA- und Proteinebene machen in B6/NFATc1-eGFP-BAC-Reportermäusen das GFP-Protein somit zu einem sensitiven und spezifischen Marker der NFATc1-Aktivität. In FACS-Analysen gibt der Anstieg der GFP-Fluoreszenzintensität bei Stimulation von Gesamt- Milzzellen bzw. T-Lymphozyten um bis auf das Dreifache die Induktion von NFATc1 wider. Unter dem Einfluss von CsA verbleibt die GFPFluoreszenzintensität auf dem Niveau unstimulierter Zellen. Die GFPFluoreszenz korreliert darüber hinaus bei Primärstimulation mit der Expression des IL-2-Gens, dessen Promotor mit 5 NFAT-Bindestellen den Prototyp eines NFATc1-Targets darstellt (Serfling et al., 1989). Die Analyse der Koexpression von NFATc1 und GFP mittels Fluoreszenzmikroskopie zeigt in allen stimulierten, GFP-positiven CD4+-Lymphozyten die nukleäre Lokalisation von 75 NFATc1, vor allem von NFATc1α. Die Analyse des GFP-Phänotyps in alloreaktiven T-Zellen zeigt bei Abstoßungsreaktionen in vitro („Mixed Lymphocyte Reactions“) eine selektive Zunahme der Fluoreszenz dieser Zellen um bis auf das Vierfache, was die Rolle von NFATc1 für die Effektorfunktion aktivierter T-Lymphozyten verdeutlicht. GFP und das endogene NFATc1 werden bei Stimulation konventioneller T-Zellen (Tcons, CD4+CD25-FoxP3-) stark exprimiert, während natürliche regulatorische T-Zellen (nTregs, CD4+CD25+FoxP3+) konstant geringe NFATc1- und GFP-Konzentrationen zeigen. In induzierten regulatorischen T-Lymphozyten (iTregs) supprimiert TGF- β konzentrationsabhängig die GFP-Fluoreszenz bis auf das Niveau unstimulierter Lymphozyten. Während in nTregs die Suppression des Nfatc1- Gens im wesentlichen durch FoxP3 erfolgt (Torgerson et al., 2009), scheint dies in iTregs vor allem über den TGF-β Signalweg vermittelt zu werden. Die Analyse der GFP-Expression in den verschiedenen Stadien der TZellentwicklung zeigt weiterhin deutliche Unterschiede in der Aktivität des Nfatc1-Gens. Dies wird durch die starke Aktivität des BAC-Genlokus in CD4- CD8- DN Thymozyten, welche eine sechsfach höhere GFP-Expression aufweisen als CD4+CD8+ DP Zellen, deutlich. N2 - Activation of lymphocytes causes a high level of Nfatc1 due to P1-promoter induction, whereas the P2-promoter leads to an constitutive expression of NFATc2/c3. NFATc1/αA is essential for effector-function, proliferation and survival of activated cells (Chuvpilo et al., 2002). Here we show that the eGFP-cDNA integrated in a NFATc1-eGFP-BAC-construct is under control of both promoters (P1, P2) and correlates with the NFATc1-Expression on mRNA and protein-levels. In FACS-analysis there is an increase in eGFP-fluorescence intensity, which is highly CsA-sensitive. In natural and induced Tregs we observed a low level of eGFP-expression correlating with concentration of TGF-β. CD4-CD8- DN cells show the highest eGFP-Expression in thymocytes. KW - NFATc1 KW - Genexpression KW - eGFP KW - BAC-Konstrukt KW - NFATc1 KW - Genexpression KW - eGFP KW - BAC-Konstrukt KW - NFATc1 KW - gene expression KW - eGFP KW - BAC-construct Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-80596 ER - TY - JOUR A1 - Schulte, Leon N. A1 - Schweinlin, Matthias A1 - Westermann, Alexander J. A1 - Janga, Harshavardhan A1 - Santos, Sara C. A1 - Appenzeller, Silke A1 - Walles, Heike A1 - Vogel, Jörg A1 - Metzger, Marco T1 - An Advanced Human Intestinal Coculture Model Reveals Compartmentalized Host and Pathogen Strategies during Salmonella Infection JF - mBio N2 - A major obstacle in infection biology is the limited ability to recapitulate human disease trajectories in traditional cell culture and animal models, which impedes the translation of basic research into clinics. Here, we introduce a three-dimensional (3D) intestinal tissue model to study human enteric infections at a level of detail that is not achieved by conventional two-dimensional monocultures. Our model comprises epithelial and endothelial layers, a primary intestinal collagen scaffold, and immune cells. Upon Salmonella infection, the model mimics human gastroenteritis, in that it restricts the pathogen to the epithelial compartment, an advantage over existing mouse models. Application of dual transcriptome sequencing to the Salmonella-infected model revealed the communication of epithelial, endothelial, monocytic, and natural killer cells among each other and with the pathogen. Our results suggest that Salmonella uses its type III secretion systems to manipulate STAT3-dependent inflammatory responses locally in the epithelium without accompanying alterations in the endothelial compartment. Our approach promises to reveal further human-specific infection strategies employed by Salmonella and other pathogens. IMPORTANCE Infection research routinely employs in vitro cell cultures or in vivo mouse models as surrogates of human hosts. Differences between murine and human immunity and the low level of complexity of traditional cell cultures, however, highlight the demand for alternative models that combine the in vivo-like properties of the human system with straightforward experimental perturbation. Here, we introduce a 3D tissue model comprising multiple cell types of the human intestinal barrier, a primary site of pathogen attack. During infection with the foodborne pathogen Salmonella enterica serovar Typhimurium, our model recapitulates human disease aspects, including pathogen restriction to the epithelial compartment, thereby deviating from the systemic infection in mice. Combination of our model with state-of-the-art genetics revealed Salmonella-mediated local manipulations of human immune responses, likely contributing to the establishment of the pathogen's infection niche. We propose the adoption of similar 3D tissue models to infection biology, to advance our understanding of molecular infection strategies employed by bacterial pathogens in their human host. KW - Salmonella KW - gene expression KW - infectious disease Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-229428 VL - 11, 2020 IS - 1 ER - TY - JOUR A1 - Rosenbaum, Corinna A1 - Schick, Martin Alexander A1 - Wollborn, Jakob A1 - Heider, Andreas A1 - Scholz, Claus-Jürgen A1 - Cecil, Alexander A1 - Niesler, Beate A1 - Hirrlinger, Johannes A1 - Walles, Heike A1 - Metzger, Marco T1 - Activation of Myenteric Glia during Acute Inflammation In Vitro and In Vivo JF - PLoS One N2 - Background Enteric glial cells (EGCs) are the main constituent of the enteric nervous system and share similarities with astrocytes from the central nervous system including their reactivity to an inflammatory microenvironment. Previous studies on EGC pathophysiology have specifically focused on mucosal glia activation and its contribution to mucosal inflammatory processes observed in the gut of inflammatory bowel disease (IBD) patients. In contrast knowledge is scarce on intestinal inflammation not locally restricted to the mucosa but systemically affecting the intestine and its effect on the overall EGC network. Methods and Results In this study, we analyzed the biological effects of a systemic LPS-induced hyperinflammatory insult on overall EGCs in a rat model in vivo, mimicking the clinical situation of systemic inflammation response syndrome (SIRS). Tissues from small and large intestine were removed 4 hours after systemic LPS-injection and analyzed on transcript and protein level. Laser capture microdissection was performed to study plexus-specific gene expression alterations. Upon systemic LPS-injection in vivo we observed a rapid and dramatic activation of Glial Fibrillary Acidic Protein (GFAP)-expressing glia on mRNA level, locally restricted to the myenteric plexus. To study the specific role of the GFAP subpopulation, we established flow cytometry-purified primary glial cell cultures from GFAP promotor-driven EGFP reporter mice. After LPS stimulation, we analyzed cytokine secretion and global gene expression profiles, which were finally implemented in a bioinformatic comparative transcriptome analysis. Enriched GFAP+ glial cells cultured as gliospheres secreted increased levels of prominent inflammatory cytokines upon LPS stimulation. Additionally, a shift in myenteric glial gene expression profile was induced that predominantly affected genes associated with immune response. Conclusion and Significance Our findings identify the myenteric GFAP-expressing glial subpopulation as particularly susceptible and responsive to acute systemic inflammation of the gut wall and complement knowledge on glial involvement in mucosal inflammation of the intestine. KW - gene expression KW - gastrointestinal tract KW - inflammatory bowel disease KW - central nervous system KW - systemic inflammatory response syndrome KW - inflammation KW - astrocytes KW - cytokines Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-146544 VL - 11 IS - 3 ER - TY - JOUR A1 - Molochnikov, Leonid A1 - Rabey, Jose M. A1 - Dobronevsky, Evgenya A1 - Bonuccelli, Ubaldo A1 - Ceravolo, Roberto A1 - Frosini, Daniela A1 - Grünblatt, Edna A1 - Riederer, Peter A1 - Jacob, Christian A1 - Aharon-Peretz, Judith A1 - Bashenko, Yulia A1 - Youdim, Moussa B. H. A1 - Mandel, Silvia A. T1 - A molecular signature in blood identifies early Parkinson's disease JF - Molecular Neurodegeneration N2 - Background: The search for biomarkers in Parkinson's disease (PD) is crucial to identify the disease early and monitor the effectiveness of neuroprotective therapies. We aim to assess whether a gene signature could be detected in blood from early/mild PD patients that could support the diagnosis of early PD, focusing on genes found particularly altered in the substantia nigra of sporadic PD. Results: The transcriptional expression of seven selected genes was examined in blood samples from 62 early stage PD patients and 64 healthy age-matched controls. Stepwise multivariate logistic regression analysis identified five genes as optimal predictors of PD: p19 S-phase kinase-associated protein 1A (odds ratio [OR] 0.73; 95% confidence interval [CI] 0.60-0.90), huntingtin interacting protein-2 (OR 1.32; CI 1.08-1.61), aldehyde dehydrogenase family 1 subfamily A1 (OR 0.86; 95% CI 0.75-0.99), 19 S proteasomal protein PSMC4 (OR 0.73; 95% CI 0.60-0.89) and heat shock 70-kDa protein 8 (OR 1.39; 95% CI 1.14-1.70). At a 0.5 cut-off the gene panel yielded a sensitivity and specificity in detecting PD of 90.3 and 89.1 respectively and the area under the receiving operating curve (ROC AUC) was 0.96. The performance of the five-gene classifier on the de novo PD individuals alone composing the early PD cohort (n = 38), resulted in a similar ROC with an AUC of 0.95, indicating the stability of the model and also, that patient medication had no significant effect on the predictive probability (PP) of the classifier for PD risk. The predictive ability of the model was validated in an independent cohort of 30 patients at advanced stage of PD, classifying correctly all cases as PD (100% sensitivity). Notably, the nominal average value of the PP for PD (0.95 (SD = 0.09)) in this cohort was higher than that of the early PD group (0.83 (SD = 0.22)), suggesting a potential for the model to assess disease severity. Lastly, the gene panel fully discriminated between PD and Alzheimer's disease (n = 29). Conclusions: The findings provide evidence on the ability of a five-gene panel to diagnose early/mild PD, with a possible diagnostic value for detection of asymptomatic PD before overt expression of the disorder. KW - cerebrospina KW - magnetic-resonance-spectroscopy KW - protein KW - biomarkers KW - E3 ubiquitin ligase KW - SCF KW - SKP1 KW - heat shock protein Hsc-70 KW - early diagnosis KW - fluid KW - alpha-synuclein KW - dehydrogenases KW - Alzheimer's disease KW - sporadic Parkinson's disease KW - blood biomarker KW - CSF KW - multiple system atrophy KW - clinical diagnosis KW - substantia nigra KW - gene expression Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-134508 VL - 7 IS - 26 ER -