TY - THES A1 - Fischer, Andreas T1 - Biochemische Charakterisierung der basischen Helix-Loop-Helix-Transkriptionsfaktoren Hey1 und Hey2 sowie Untersuchung ihrer Rolle während der Herz- und Gefäßentwicklung T1 - Biochemical characterisation of the basic helix-loop-helix transcription factors Hey1 and Hey2 and analysis of their role in cardiovascular development N2 - Die Entwicklung eines vielzelligen Organismus aus einer befruchteten Eizelle ist nur durch komplexe zelluläre Regulationsmechanismen möglich. Dabei spielt der Notch-Signaltransduktionsweg eine zentrale Rolle während der Determination von Zellschicksalen und der Zelldifferenzierung. Die primären Zielgene der Notch-Signalkaskaskade bei Vertebraten sind die Hes- sowie die kürzlich identifizierten Hey-Gene. Die Hey-(hairy and E(spl) related with YRPW motif)-Gene kodieren drei hairy/E(spl)/Hes-verwandte basische Helix-Loop-Helix-Transkriptionsfaktoren, die durch eine Orange-Domäne und einen charakteristischen Carboxyterminus gekennzeichnet sind. Während der Embryonalentwicklung werden die Hey-Gene dynamisch in zahlreichen Geweben exprimiert. Ziel dieser Arbeit war es, neue Hey-Interaktionsproteine aus embryonalen Genbanken zu isolieren, die Bindung an weitere bHLH-Transkriptionsfaktoren zu überprüfen und ihre DNA-Bindung zu analysieren. Um die physiologische Hey2-Funktion zu ergründen, wurden Hey2-Knockoutmäuse untersucht. In einem ersten Versuch wurde eine neue Screeningmethode erprobt, bei der Proteinexpressionsfilter mit markierten Hey1-Peptiden nach interagierenden Proteinen durchsucht wurden. Hierbei sind 53 Proteine isoliert worden, jedoch konnte nach eingehenderen Untersuchungen kein relevanter Bindungsspartner beschrieben werden. Für weitere Analysen unter mehr physiologischen Bedingungen wurde das Yeast Two-Hybrid Verfahren für Hey1 und Hey2 etabliert. Das Screening von murinen embryonalen cDNA-Genbanken mit verschiedenen Hey1-Fragmenten führte zur Isolation von mehreren hundert Klonen. Die interessantesten Kandidaten wurden weiteren biochemischen Tests unterzogen, wobei jedoch keine neuen Interaktionspartner verifiziert werden konnten. Mit gezielten direkten Yeast Two-Hybrid und GST-Pulldown Assays für vermutete Kandidaten konnte jedoch die Interaktion von Hey1 bzw. Hey2 mit den bHLH-Proteinen E2-2, E2-5, MyoD und c-hairy1 nachgewiesen werden. Außerdem wurde festgestellt, dass Hey1 und Hey2 Homodimere und Hey1/Hey2-Heterodimere bilden. Die stärkste Interaktion wurde mit dem in der Somitogenese rhythmisch exprimierten c-hairy1-Protein beobachtet. Da Hey2 und c-hairy1 im präsomitischen Mesoderm und in den Somiten coexprimiert werden und starke Heterodimere ausbilden, erscheint es wahrscheinlich, dass beide Proteine gemeinsam die Transkription nachgeschalteter Gene steuern. Diese Interaktionsstudien zeigten außerdem erstmals, dass die Orange-Domäne entscheidend an der Bildung der Dimere beteiligt ist, da durch sie die Dimerisierung in vivo deutlich verstärkt wurde. Schließlich konnte gezeigt werden, dass Hey1 und Hey2, im Gegensatz zu den übrigen hairy-Proteinen, nicht mit dem Corepressor Groucho/TLE1 interagieren. Electrophoretic Mobility Shift Assays ergaben, dass die Hey1- und Hey2-Proteine an eine E(spl)-spezifische E-Box DNA-Sequenz (CACGTG) binden. Auch die interagierenden bHLH-Proteine c-hairy1, E2-2 und E2-5 binden als Homodimere an diese DNA-Sequenz. Im zweiten Teil dieser Arbeit wurde die Hey2-Genfunktion an Hey2-Knockoutmäusen untersucht. Etwa 80 % der homozygoten Mäuse starben wenige Tage nach der Geburt. Sie zeigten eine massive Hypertrophie der Herzventrikel, die wahrscheinlich die Todesursache darstellt. Die lacZ-Expression der untersuchten Organe entsprach der Hey2-Expression im Wildtyp. Es fiel dabei auf, dass es postnatal zu einer Herunterregulation der Hey2-Transkription kommt. Mit Elektrokardiogrammen wurden keine Reizleitungsstörungen bei neugeborenen Hey2-Knockoutmäusen festgestellt. Interessanterweise konnte mit Arteriographien ausgeschlossen werden, dass die Ventrikelhypertophie Folge einer Aortenstenose wie bei der gridlock (zf-Hey2)-Mutante im Zebrafisch ist. Vielmehr führt eine homozygote Hey2-Deletion zu einer Kardiomyopathie in Kombination mit verschiedenene Herzfehlern. Untersuchungen der Hey1- und HeyL-Expression in Hey2-Knockoutembryonen mittels RNA in situ Hybridisierungen zeigten keine Veränderungen im Vergleich mit dem Wildtyp. Daraus kann gefolgert werden, dass Hey1 und HeyL zumindest dort, wo sie nicht mit Hey2 coexprimiert sind, die Hey2-Funktionen nicht kompensieren können. Weitere Erkenntnisse über die Funktionen der Hey-Gene werden sicherlich die Studien an den Doppelknockoutmäusen ergeben. Die bisherigen Ergebnisse zeigen eindeutig, dass die Hey-Gene essentiell für die murine Herzentwicklung sind. Weitere Untersuchungen müssen nun zeigen, welche Rolle diese Gene bei der Entstehung von kongenitalen Herzfehlern des Menschen spielen. N2 - The development from a single fertilized oocyte to a multicellular organism requires complex cellular regulatory mechanisms. During this process the Notch signalling pathway plays a crucial role in determining cell fate and differentiation. Primary target genes of the Notch signalling cascade in vertebrates are Hes and the recently identified Hey genes. Hey (hairy and E(spl) related with YRPW motif) genes encode three hairy/E(spl)/Hes related basic helix-loop-helix transcription factors characterised by an Orange domain and a conserved carboxyterminus. During embryonic development Hey genes are dynamically expressed in various tissues. The goal of this study was to isolate novel Hey-interacting proteins from embryonic cDNA libraries, to analyse the binding to other bHLH transcription factors and to examine their DNA-binding properties. To elucidate the physiological role of Hey2, Hey2 knockout mice were analysed. First, a new screening method was used to identify Hey1-binding proteins from protein expression filters hybridised with labelled Hey1 peptides. Out of 53 candidates isolated no relevant interaction partner could be verified after more detailed examination. For further analysis under more physiological conditions the yeast-two hybrid system was established for Hey1 and Hey2. Screening of murine embryonic cDNA libraries with different Hey1 fragments led to the identification of several hundred clones. The most interesting ones were further analysed with biochemical assays, but no novel interaction partner could be verified. With direct yeast-two hybrid and GST-pulldown assays of candidate proteins an interaction of Hey1 and Hey2 with the bHLH proteins E2-2, E2-5, MyoD and c-hairy1 was found. Furthermore, it could be shown that Hey1 and Hey2 can form homodimers as well as Hey1/Hey2 heterodimers. However, the strongest interaction was seen with c-hairy1, which is dynamically expressed during somitogenesis. Hey2 and c-haiy1 are coexpressed in the presomitic mesoderm and in somites and their strong interaction suggests that both proteins together regulate the transcription of target genes. These interaction studies showed for the first time that the Orange domain is important for dimer formation in vivo, because it strongly increased binding strength. Furthermore, it could be shown that Hey1 and Hey2 do not interact with the corepressor Groucho/TLE1, which is in contrast to all other hairy-related proteins. Electrophoretic mobility shift assays revealed that Hey1 and Hey2 proteins are able to bind an E(spl)-specific E-box DNA sequence (CACGTG). The interacting bHLH proteins c-hairy1, E2-2 and E2-5 could also bind to this sequence as homodimers. The aim of the second part of this study was to examine Hey2-lacZ knockout mice. About 80 % of the homozygous mice died within a few days after birth. They exhibited massive ventricular hypertrophy as the most likely cause of death. Expression of lacZ in the organs analysed was comparable to Hey2 in wildtype. It became clear that Hey2 transcription is downregulated postnatally. Electrocardiography showed no conduction failure or arrythmia in newborn knockouts. Interestingly, it could be ruled out by angiography that ventricular hypertrophy is caused by aortic coarctation as seen in the gridlock (zf-Hey2) zebrafish mutant. However, loss of Hey2 leads to cardiomyopathy combined with various cardiac structural defects. Hey1 and HeyL expression in Hey2 knockout embryos was not altered as shown by RNA in situ hybridisation. Therefore, it can be concluded that Hey1 and HeyL can not compensate Hey2 function, at least in organs where they are not coexpressed. A better understanding of the Hey genes will be achieved by studying double knockout mice. This work clearly shows that Hey genes are essential for murine heart development. Further analysis will reveal if these genes also play a role in congenital heart disease in humans. KW - Hey1 KW - Hey2 KW - Transkriptionsfaktoren KW - Herz KW - Gefäße KW - Hey1 KW - Hey2 KW - transcription factors KW - heart KW - vessels Y1 - 2002 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-6086 ER - TY - THES A1 - Schmidt, Arthur T1 - Die Interaktion der Transkriptionsfaktoren NF-ATc und GATA-3 in T-Helfer-Zellen T1 - The Interaction of the transcription factors NF-ATc and GATA-3 in T-helper cells N2 - Interleukin-5 ist ein Th2-Cytokin, das eosinophile Granulozyten aktiviert und B-Zellen zur Produktion von IgE stimuliert. Bei der Entstehung von allergischen (wie z.B. Asthma) und atopischen Reaktionen spielt die erhöhte Ausschüttung von IL-5 eine wichtige Rolle. Der Interleukin-5-Promoter weist unter anderem Bindestellen für NF-AT-Faktoren und GATA-3 auf. NF-ATc ist ein Mitglied der NF-AT („Nuclear Factor of Activated T-cells“)-Transkriptionsfaktoren, die an den verschiedensten immunologischen Funktionen beteiligt sind, vor allem aber an der Steuerung der Cytokingene. GATA-3 ist ein wichtiger Th2-spezifischer Zinkfinger-Transkriptionsfaktor aus der Familie der GATA-Faktoren, die an eine gemeinsame WGATAR-Sequenz der DNA binden. Molkentin et al. zeigten 1998, daß NF-AT3 und GATA-4 in Herzmuskelzellen physikalisch interagieren und daß ihre funktionelle Kooperation bei der Aktivierung verschiedener Promotoren letztendlich zur Entwicklung einer Herzhypertrophie beiträgt. In dieser Arbeit sollte untersucht werden, ob eine ähnliche physikalische Interaktion zwischen NF-ATc und GATA-3 in T-Zellen stattfindet. Zu diesem Zweck wurden im ersten Teil der Arbeit Coimmunopräzipitationen durchgeführt. Dabei konnte in mit NF-ATc und GATA-3 cotransfizierten 293T Zellen eine spezifische in vivo Interaktion der beiden Transkriptionsfaktoren nachgewiesen werden. Im zweiten Teil der Arbeit sollten mittels GST-„pulldown“-Experimenten die für die Interaktion wichtigen Proteindomänen von NF-ATc und GATA-3 bestimmt werden. Im ersten Schritt wurden die dafür benötigten Plasmide konstruiert. Im zweiten Schritt erfolgte die bakterielle Expression und nachfolgende Aufreinigung der GST-Fusionsproteine. Mit GST wurde jeweils eine N- und C-terminale Hälfte von NF-ATc und GATA-3 fusioniert. Mit diesen rekombinanten Proteinen wurden die „pulldown“-Experimente durchgeführt. Dabei konnte eine Interaktion des C-terminalen Anteils (enthält den zweiten Zinkfinger) von GATA-3 mit NF-ATc detektiert werden. Nachfolgende Ergebnisse deuteten auf eine Interaktion des C-terminalen Anteils (enthält die „Rel-Similarity-Domain“) von NF-ATc mit GATA-3 hin. Analog zeigten Molkentin et al., daß die RSD von NF-AT3 mit dem C-terminalen Zinkfinger von GATA-4 in Herzmuskelzellen interagiert. Die Interaktion von NF-ATc und GATA-3 scheint nicht nur physikalisch zu existieren, sondern auch funktionell von Bedeutung zu sein. In Luciferase-Reporteressays, die in unserem Labor durchgeführt wurden, zeigte sich bei Cotransfektion von NF-ATc und GATA-3 im Vergleich zu Einzeltranfektionen eine drastische Aktivitätssteigerung des IL-5 Promoters. Diese Ergebnisse weisen – wiederum analog zu den Vorgänge im Herzen - auf eine funktionelle Kooperation der beiden Transkriptionsfaktoren bei der Steuerung des IL-5 Promoters hin. N2 - This study investigates the interaction of the transcription factors NF-ATc and GATA-3. Both transcription factors are important in Th2-cells and both are required for optimal activation of the IL-5 promoter. The results of this study show a physical interacion of these 2 proteins and indicate that C-terminal domains of both factors are important for the interaction. KW - NF-AT KW - GATA-3 KW - T-Helfer Zellen KW - Transkriptionsfaktoren KW - NF-AT KW - GATA-3 KW - transcription factors KW - T helper cells Y1 - 2004 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-11664 ER - TY - THES A1 - König, Corinne T1 - Die transkriptionelle Regulation der Proteintyrosinkinase p 56 lck als Schlüsselenzym der Thymozytenreifung T1 - Transcriptional regulation of protein kinase p 56 lck a major enzyme in thymocyte developement N2 - In der vorliegenden Arbeit wurde die transkriptionelle Regulation des proximalen Promotors der lymphozytenspezifischen Proteintyrosinkinase lck untersucht. Das Hauptaugenmerk richtete sich auf die Beteiligung der Familie der NF-AT-Transkriptionsfaktoren an der Kontrolle der Promotoraktivität. Es konnte zunächst gezeigt werden, dass NF-ATs aus Zellkulturzellen sowie aus frisch isolierten Thymozyten spezifisch an Sequenzmotive in der regulatorischen Region des lck-Typ-I-Promotors binden. Die NF-AT-Bindungsstellen mit der höchsten Affinität wurden in Pos. –480/–476 (NF-AT-I lck) und in Pos. –216/–212 (NF-AT-II lck) identifiziert. Eine Mutation in den Bindungsmotiven verhinderte dementsprechend die Ausbildung von NF-AT-Komplexen mit der DNA. Darüber hinaus wurde nachgewiesen, dass NF-AT-Faktoren den proximalen lck-Promotor allein und zusammen mit Faktoren der Ets-Familie bzw. c-Myb aktivieren können. Die Untersuchung der Interaktion von NF-AT und c-Myb ergab, dass die beiden Transkriptionsfaktoren unmittelbar benachbart an die DNA binden. Unter Berücksichtigung dieses Bindungsverhaltens und der Kooperation in der Transaktivierung des Promotors konnten wir somit eine neue Form eines NF-AT-"composite elements" beschreiben. Bei der Untersuchung von NF-AT-"knock out"-Mäusen auf Anzeichen einer lck-Bildungsstörung zeigte sich eine deutliche Reduktion der lck-Typ-I-Transkripte in NF-AT1/NF-AT4 doppelt defizienten Tieren. Dies belegt die Relevanz der NF-AT-Faktoren für die Aktivität des proximalen lck-Promotors in vivo. N2 - The presented thesis covers the investigation of the transcriptional regulation of the proximal promotor of the lymphocyte specific protein tyrosine kinase lck. The main aspect is focused on the role of NF-AT family of transcription factors in the control of the promotor activity. It was shown that NF-ATs in cell culture cells as well as in freshly isolated murine thymocytes show specific binding to sequence motifs in the regulatory sequence of the lck type I promotor. The NF-AT binding sites with the strongest affinity were located in pos. -480/-476 (NF-ATI lck) and pos. -216/-212 (NF-AT II lck). Mutations in the binding motifs did therefore not allow any complex formation inbetween NF-AT an DNA. Moreover it was shown that NF-AT factors were able to activate the proximal lck-promotor by themselves and together with c-Myb and members of the Ets-family. The investigation of the interaction between NF-At and c-Myb revealed that the two factors bind the DNA in close proximity. Taking this into account and the fact that the two factors cooperate in the transactivation of the proximal lck promotor we were able to describe a new NF-AT "composite element". Examining NF-AT knock out mice for signs of lck-deprevation we saw a significant reduction of lck-type I transcripts in NF-AT1/NF-AT4-double negative animals. This stresses the relevance of NF-AT factors for the activity of the proximal lck-promotor in vivo. KW - Thymus KW - Transkriptionsfaktoren KW - NF-AT KW - lck KW - thymus KW - transcription factors KW - NF-AT KW - lck Y1 - 2004 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-8867 ER - TY - THES A1 - König, Thomas T1 - Die Rolle von NFAT-Transkriptionsfaktoren bei der Regulation der Apoptose peripherer T-Zellen T1 - The role of NFAT transcription factors in regulating apoptosis of peripheral T-cells N2 - In der vorliegenden Arbeit wurde die Rolle der NFAT-Transkriptionsfaktoren NFATc2 und NFATc3 beim AICD (Activation induced cell death) von peripheren T-Lymphozyten untersucht. Dazu wurde die Auslösbarkeit der Apoptose mittels Anti-CD3-Antikörper bei Wildtyp- bzw. Knock-out-Mäusen mit folgender NFAT-Ausstattung verglichen: NFAT c2+/+c3-/-, c2-/-c3+/+, c2-/-c3-/+, c2-/-c3-/-. Mittels FACS-Analyse von T-Helfer-Zellen aus den Lymphknoten dieser Mäuse zeigte sich, dass die CD3-vermittelte Apoptose - im Gegensatz zur Fas-vermittelten - mit dem Gesamtgehalt der Zellen an NFATc2 und NFAT c3 korreliert und diesbezüglich eine direkte Proportionalität angenommen werden kann. N2 - This thesis is abot the role of NFAT transkription faktors (NFATc2 and NFATc3) in the activation induced cell death of peripheral T-cells. Therfore we looked at the inducability of apoptosis by anti-CD3-antibodies in wildtype- or knock-out-mice with respect to specific NFAT-genes: NFAT c2+/+c3-/-, c2-/-c3+/+, c2-/-c3-/+, c2-/-c3-/-. With FACS-analysis of CD4-positive T-cells taken from lymphnodes of these mice we found, that CD3-mediated apoptosis - contraty to Fas-mediated - correlates with the amount of NFATc2 and NFAT c3 in the cell in a direct proportional manner. KW - NFAT KW - Knock-out-Mäuse KW - T-Zellen KW - AICD KW - Lymphozyten KW - NFAT KW - knock out mice KW - AICD KW - apoptosis KW - transcription factors Y1 - 2006 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-23594 ER - TY - THES A1 - Queisser, Nina T1 - Oxidative and nitrosative stress induced by the mineralocorticoid aldosterone - Mechanism of induction and role of signal transduction pathways and transcription factors T1 - Oxidativer und nitrosativer Stress induziert durch das Mineralocorticoid Aldosteron - Mechanismen der Induktion und Rolle von Signalwegen und Transkriptionsfaktoren N2 - Several epidemiological studies found that hypertensive patients have an increased risk to develop kidney cancer. Hyperaldosteronism frequently results in arterial hypertension and contributes to the development and progression of kidney injury, with reactive oxygen species (ROS) playing an important role. ROS are thought to be associated with many pathological conditions such as cancer and other disorders, like cardiovascular complications , which often go along with hypertension. The aim of the present work was to investigate whether the effects of elevated aldosterone concentrations might be involved in the increased cancer incidence of hypertensive individuals. First, the potential capacity of aldosterone to induce oxidative stress and DNA damage was investigated in vitro and in vivo. In LLC-PK1 porcine kidney cells and MDCK canine kidney cells the significant formation of ROS, and especially of superoxide (O2˙ˉ) was assessed. With two genotoxicity tests, the comet assay and the micronucleus frequency test, the DNA damaging potential of aldosterone was quantified. In both genotoxicity tests a dose-dependent increase in aldosterone-induced structural DNA damage was observed. Oxidative stress and DNA damage were prevented by antioxidants, suggesting ROS as a major cause of DNA damage. Furthermore, the oxidatively modified DNA lesion 8-oxo-7,8-dihydro-2´-deoxyguanosine (8-oxodG), was found to be significantly elevated. In kidneys of rats with desoxycorticosterone acetate (DOCA)/salt-induced hypertension, which is a model of severe mineralocorticoid-dependent hypertension, elevated levels of ROS and superoxide were found, compared to kidneys of sham rats. Also DNA strand breaks, measured with the comet assay and double strand breaks, visualized with antibodies against the double strand break-marker gamma-H2AX were significantly elevated in kidneys of DOCA/salt-treated rats. In addition, significantly increased amounts of 8-oxodG were detected. Proliferation of kidney cells was found to be increased, which theoretically enables the DNA damage to manifest itself as mutations, since the cells divide. Second, the effects of aldosterone on the activation of transcription factors and signaling pathways were investigated. A significant activation of the potentially protective transcription factor Nrf2 was observed in LLC-PK1 cells. This activation was triggered by an increase of ROS or reactive nitrogen species (RNS). In response to oxidative stress, glutathione synthesis and detoxifying enzymes, such as the subunits of the glutathione-cysteine-ligase or heme oxygenase 1 were rapidly induced after 4 h. Nevertheless, after 24 h a decrease of glutathione levels was observed. Since ROS levels were still high after 24 h, but Nrf2 activation decreased, this adaptive survival response seems to be transient and quickly saturated and overwhelmed by ROS/RNS. Furthermore, Nrf2 activation was not sufficient to protect cells against oxidative DNA damage, because the amounts of double strand breaks and 8-oxodG lesions steadily rose up to 48 h of aldosterone treatment. The second transcription factor that was time- and dose-dependently activated by aldosterone in LLC-PK1 and MDCK cells was NF-kappaB. Furthermore, a significant cytosolic and nuclear activation of ERK was detected. Aldosterone induced the phosphorylation of the transcription factors CREB, STAT1 and STAT3 through ERK. Third, the underlying mechanisms of oxidant production, DNA damage and activation of transcription factors and signaling pathways were studied. Aldosterone exclusively acted via the MR, which was proven by the MR antagonists eplerenone, spironolactone and BR-4628, whereas the glucocorticoid receptor (GR) antagonist mifepristone did not show any effect. Furthermore, aldosterone needed cytosolic calcium to exert its negative effects. Calcium from intracellular stores and the influx of calcium across the plasma membrane was involved in aldosterone signaling. The calcium signal activated on the one hand, the prooxidant enzyme complex NAD(P)H oxidase through PKC, which subsequently caused the generation of O2˙ˉ. On the other hand, nitric oxide synthase (NOS) was activated, which in turn produced NO. NO and O2˙ˉ can react to the highly reactive species ONOO- that can damage the DNA more severely than the less reactive O2˙ˉ. In the short term, the activation of transcription factors and signaling pathways could be a protective response against aldosterone-induced oxidative stress and DNA damage. However, a long-term NF-B and ERK/CREB/STAT activation by persistently high aldosterone levels could unfold the prosurvival activity of NF-kappaB and ERK/CREB/STAT in aldosterone-exposed cells. DNA damage caused by increased ROS might become persistent and could be inherited to daughter cells, probably initiating carcinogenesis. If these events also occur in patients with hyperaldosteronism, these results suggest that aldosterone could be involved in the increased cancer incidence of hypertensive individuals. N2 - Mehrere epidemiologische Studien haben ein erhöhtes Nierenkrebsrisko bei Patienten mit Bluthochdruck aufgedeckt. Hyperaldosteronismus führt oft zu arteriellem Bluthochdruck und trägt zur Entwicklung und zum Fortschreiten von Nierenschäden bei, wobei reaktive Sauerstoffspezies (ROS) eine wichtige Rolle spielen. Immer häufiger werden ROS mit Krankheitsbildern wie Krebs und kardiovaskulären Erkrankungen, die mit Bluthochdruck einhergehen, in Verbindung gebracht. Das Ziel dieser Arbeit war es, zu untersuchen, ob erhöhte Aldosteronkonzentrationen an dem gesteigerten Krebsrisiko von hypertensiven Patienten beteiligt sein könnten. Zunächst wurde die potentielle Kapazität von Aldosteron, oxidativen Stress und DNA-Schaden in vitro und in vivo induzieren zu können, untersucht. In der Schweine-Nierenzelllinie LLC-PK1 und der Hunde-Nierenzelllinie MDCK wurde die Entstehung von ROS und speziell die Bildung von Superoxid (O2˙ˉ) nachgewiesen. Das gentoxische Potential von Aldosteron wurde mit zwei Genotoxizitätstests, dem Comet Assay und dem Mikrokernfrequenztest bestimmt. In beiden Genotoxizitätstests konnte ein dosis-abhängiger Anstieg des strukturellen DNA-Schadens beobachtet werden. Antioxidantien konnten den oxidativen Stress und die DNA-Schäden verringern, was annehmen lässt, dass ROS die Hauptursache für die Entstehung der DNA-Schäden sind. Darüberhinaus wurden signifikant erhöhte Mengen der oxidativ modifizierten DNA Läsion 8-Oxo-7,8-dihydro-2´-deoxyguanosin (8-oxodG) gefunden. In Nieren von Ratten mit Desoxycorticosteron-Acetat (DOCA) und Salz-induziertem Bluthochdruck, ein Modell für massiven Mineralocorticoid-induzierten Bluthochdruck, wurde ebenfalls eine erhöhte Bildung von ROS und O2˙ˉ in Nieren von DOCA/Salz-Ratten im Vergleich zu Sham-Ratten beobachtet. Auch im Comet Assay erfasste DNA-Strangbrüche und Doppelstrangbrüche, die mit Hilfe von Antikörpern gegen den Doppelstrangbruchmarker gamma-H2AX sichtbar gemacht wurden, waren in den Nieren der DOCA/Salz-behandelten Ratten signifikant erhöht. Weiterhin wurden erhöhte 8-oxodG-Spiegel in DOCA/Salz-Ratten beobachtet. Auch eine erhöhte Proliferationsrate in DOCA/Salz-behandelten Ratten konnte festgestellt werden, was theoretisch dazu führen könnte, dass sich die DNA-Schäden als Mutationen manifestieren, da sich die Zellen teilen. Im zweiten Teil der Arbeit wurde der Einfluss von Aldosteron auf die Aktivierung von Transkriptionsfaktoren und Signalwegen untersucht. Zunächst konnte die Aktivierung des potentiell schützenden Transkriptionsfaktors Nrf2 in LLC-PK1 Zellen mittels electrophoretic mobility shift assay (EMSA) beobachtet werden. Diese Aktivierung wurde durch den Anstieg an ROS und reaktiven Stickstoffspezies (RNS) ausgelöst. Als Antwort auf den oxidativen Stress, wurde die Glutathion-Synthese und detoxifizierende Enzyme, wie die Untereinheiten der Glutathion-Cystein-Ligase oder Hämoxygenase 1, nach 4 Stunden rasch hochreguliert. Nichtsdestotrotz konnte nach 24 Stunden eine Abnahme des Glutathionspiegels festgestellt werden. Da die Konzentration an ROS nach 24 Stunden immer noch signifikant erhöht war, die Aktivierung von Nrf2 allerdings stark zurückgegangen ist, scheint diese adaptive Überlebensstrategie nur kurzfristig, und somit schnell durch ROS/RNS gesättigt zu sein. Weiterhin war die Aktivierung von Nrf2 nicht ausreichend, um die Zellen vor dem durch Aldosteron-induzierten DNA-Schaden zu schützen, da Doppelstrangbrüche, sowie 8-oxodG-Läsionen bei bis zu 48-stündiger Inkubation mit Aldosteron stetig anstiegen. Der zweite Transkriptionsfaktor, der zeit- und dosisabhängig durch Aldosteron aktiviert wurde, war NF-kappaB. Ausserdem wurde die cytosolische und nukleäre Aktivierung von ERK nachgewiesen. Aldosteron induzierte weiterhin die Phosphorylierung der Transkriptionsfaktoren CREB, STAT1 und STAT3 durch ERK. Im dritten Teil dieser Arbeit wurden die zugrundeliegenden Mechanismen der Entstehung von ROS/RNS, des DNA-Schadens und der Aktivierung von Transkriptionsfaktoren untersucht. Aldosteron wirkte ausschließlich über den MR, bewiesen durch Einsatz der MR-Antagonisten Eplerenon, Spironolakton und BR-4628. Der Glucocorticoid-Rezeptor-Antagonist Mifepriston zeigte dagegen keinen Effekt. Weiterhin benötigte Aldosteron cytosolisches Calcium, um seine negativen Effekte auszuüben. Es waren intrazelluäres Calcium, sowie ein Calciuminflux über die Plasmamembran am Aldosteronsignal beteiligt. Einerseits wurde der prooxidative Enzymkomplex NAD(P)H-Oxidase von Calcium durch die Proteinkinase C (PKC) aktiviert, was wiederum zur Bildung von O2˙ˉ führte. Andererseits kam es durch erhöhtes cytosolisches Calcium zur Aktivierung der NO-Synthase (NOS), welche daraufhin Stickoxid (NO) produzierte. NO und O2˙ˉ können zu dem hochreaktiven Peroxynitrit (ONOO-) reagieren, welches die DNA mehr schädigen kann als das etwas weniger reaktive O2˙ˉ. Kurzfristig könnte die Aktivierung der Transkriptionsfaktoren und Signalwege eine schützende Wirkung gegen den durch Aldosteron-induzierten oxidativen Stress und DNA-Schaden in den Zellen haben. Allerdings kann eine länger anhaltende Aktivierung von NF-kappaB und ERK/CREB/STAT durch permanent hohe Aldosteronspiegel zur Induktion einer Überlebensstrategie durch NF-kappaB und ERK/CREB/STAT in Aldosteron-exponierten Zellen führen. Der DNA-Schaden, der durch erhöhte ROS-Spiegel entsteht, könnte persistent und somit an Tochterzellen weitervererbt werden, was eventuell zur Entstehung von Krebs beitragen könnte. Falls diese Effekte auch in Patienten mit Hyperaldosteronismus gefunden werden können, dann könnte Aldosteron an der erhöhten Krebsinzidenz bei Bluthochdruck beteiligt sein. KW - Aldosteron KW - Oxidativer Stress KW - DNS-Schädigung KW - NADPH-Oxidase KW - Stickstoffoxidsynthase KW - Aldosteron KW - Oxidativer Stress KW - Nitrosativer Stress KW - DNA-Schaden KW - Transkriptionsfaktoren KW - aldosterone KW - oxidative stress KW - nitrosative stress KW - DNA damage KW - transcription factors Y1 - 2010 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-53566 ER - TY - THES A1 - Thoma, Eva Christina T1 - Directed differentiation of pluripotent stem cells induced by single genes T1 - Gerichtete Differenzierung pluripotenter Stammzellen induziert durch einzelne Gene N2 - Pluripotency describes the ability of stem cells to form every cell type of the body.. Pluripotent stem cells are e.g. embryonic stem cells (ESCs), but also the so called induced pluripotent stem cells (IPS cells), that are generated by reprogramming differentiated somatic cells into a pluripotent state. Furthermore, it has been shown that spermatogonia (SG) derived from adult testes of mouse or human are pluripotent. Because of their ability to differentiate into every somatic cell type, pluripotent stem cells have a unique status in research and regenerative medicine. For the latter, they offer a valuable opportunity to replace destroyed tissues or organs. For basic research, stem cells represent a useful system to study differentiation or developmental processes that are difficult to access in the physiological situation e.g. during embryogenesis. Both applications, however, require methods that allow efficient and directed differentiation of stem cells into defined specialized cell types. This study first aims to investigate the differentiation potential of SG derived from the teleost fish medaka (Oryzias latipes). My results demonstrate that medaka SG are able to form different somatic cell types, namely adipocytes, melanocytes, osteoblasts, and neurons. This indicates that medake SG have retained a broad differentiation potential suggesting that pluripotency is not restricted to mouse and human SG but might be conserved among vertebrates. Next, I wanted to establish a differentiation method that is solely based on ectopic expression of genes known to be essential for the formation of certain somatic cell types – so called master regulators (MRs). My findings show that ectopic expression of the melanocyte-specific transcription factor mitf-m that has previously been shown to induce differentiation of medaka ESCs into pigment cells resulted in the formation of the same cell type in medaka SG. This approach could be used to generate other somatic cell types. Thus, ectopic expression of the MRs cbfa1 and mash1 in MF-SG was sufficient to induce differentiation into osteoblasts and neurons, respectively. Interestingly, these differentiation processes included the activation of genes that are expressed earlier during embryogenesis than the differentiation-inducing MR. Furthermore, my findings show that the approach of MR-induced differentiation can be transferred to mammalian stem cell systems. Ectopic expression of the neural transcription factor ngn2 was sufficient to induce efficient and rapid differentiation of neurons in mouse ESCs. This differentiation process also included the induction of genes that in vivo are activated at earlier stages that ngn2. By generating a transgenic cell line allowing induction of ectopic ngn2 expression, it was possible to obtain a relatively pure culture of functional neurons. Ngn2-induced differentiation did not require any additional signals and occurred even under pluripotency promoting conditions. Moreover, ectopic expression of ngn2 did also induce the formation of cells with neuronal morphology in IPS cells indicating that MR-induced differentiation is operative in different stem cell types. Furthermore, protein transduction of Ngn2 into mouse ESCs also resulted in a neuronal differentiation process up to the appearance of neural precursor cells. Last, my results show that MR-induced differentiation can also be used to generate other cell types than neurons from mouse ESCs. Myoblasts and macrophage-like cells were generated by ectopic expression of the MRs myoD and cebpa, respectively. Using transgenic cell lines enabling induction of MR expression it was possible to obtain mixed cultures with two different differentiation processes occurring in parallel. Altogether this study shows that ectopic expression of single genes is sufficient to induce directed differentiation of stem cells into defined cell types. The feasibility of this approach was demonstrated for different MRs and consequently different somatic cell types. Furthermore, MR induced differentiation was operative in different stem cell types from fish and mouse. Thus, one can conclude that certain genes are able to define cell fates in in vitro stem cell systems and that this cell fate defining potential appears to be a conserved feature in vertebrates. These findings therefore provide new insights in the role of MRs in cell commitment and differentiation processes. Furthermore, this study presents a new method to induce directed differentiation of stem cells that offers several advantages regarding efficiency, rapidness, and reproducibility. MR-induced differentiation therefore represents a promising tool for both stem cell research and regenerative medicine. N2 - Pluripotenz bezeichnet die Fähigkeit einer Stammzelle, jede Zelle des Körpers zu bilden. Zu den pluripotenten Stammzellen gehören embryonale Stammzellen (ESZ), aber auch so genannte induzierte pluripotente Stammzellen (IPS Zellen), die durch Rückprogrammierung ausdifferenzierter Körperzellen in einen pluripotenten Status gewonnen werden. Außerdem wurde gezeigt, dass adulte Spermatogonien (SG) in Maus und Mensch pluripotent sind. Pluripotente Stammzellen sind von großer Wichtigkeit für Forschung und regenerative Medizin. Für letztere bieten diese Zellen aufgrund ihrer Fähigkeit, jede Körperzellen zu bilden, eine vielversprechende Möglichkeit, zerstörte Gewebe oder Organe zu ersetzen. In der Forschung stellen sie ein nützliches System dar, um Entwicklungs- und Differenzierungsprozesse zu untersuchen, die in der physiologischen Situation z.B. der Embryonalentwicklung – schwer zugänglich sind. Eine wichtige Grundlage für diese Anwendungen sind jedoch Methoden, die die effiziente und gerichtete Differenzierung von Stammzellen in einen bestimmten Zelltyp erlauben. In dieser Arbeit wird zunächst das Differenzierungspotential von SG der Fischspezies Medaka (Oryzias latipes) untersucht, um festzustellen, ob Pluripotenz von SG, die bisher nur in Maus und Mensch gezeigt wurde, auch in anderen Wirbeltieren außerhalb der Säuger erhalten ist. Meine Ergebnisse zeigen, dass Medaka-SG fähig sind verschiedene somatische Zelltypen zu bilden. Das zweite Ziel dieser Studie ist die Entwicklung einer Differenzierungsmethode, die nur auf der Expression einzelner so genannter Masterregulatoren (MR) beruht – Gene, die als essentiell für die Entwicklung bestimmter Zelltypen bekannt sind. Meine Ergebnisse zeigen, dass der Pigmentzell-spezifische Transkriptionsfaktor Mitf-M, von dem gezeigt wurde, dass er die Differenzierung von Medaka-ESZ in Pigmentzellen induzieren kann, die Bildung desselben Zelltyps in Medaka-SG induziert. Dieser Ansatz ermöglichte auch die Bildung anderer somatischer Zelltypen. So führte Überexpression der MR cbfa1 und mash1 in Medaka SG zur Differenzierung in Osteoblasten bzw. Neuronen. Interessanterweise wurde bei diesen Differenzierungsprozessen die Aktivierung von Genen beobachtet, die während der Embryonalentwicklung vor dem Differenzierung-auslösenden MR aktiviert werden. Weiterhin zeigen meine Ergebnisse, dass der Ansatz einer gerichteten Differenzierung, ausgelöst durch einzelne MR, auch auf Säuger-Stammzellen übertragen werden kann. So wurde durch Überexpression des neuronalen Genes ngn2 in murinen ESZ die effiziente und schnelle Bildung von Nervenzellen induziert, wobei auch hier die Aktivierung von Genen beobachtet wurde, deren Expression in der Embryogenese der von ngn2 vorangeht. Die Herstellung einer transgenen Zelllinie, in der die Überexpression von ngn2 aktiviert werden kann, erlaubte die Entstehung einer fast reinen Kultur funktionaler Neuronen. Der durch ngn2 ausgelöste Differenzierungsprozess war unabhängig von zusätzlichen Faktoren und lief sogar unter Bedingungen ab, die normalerweise den pluripotenten Zustand unterstützen. Außerdem führte Überexpression von ngn2 auch in IPS Zellen zur Bildung von Zellen mit neuronalem Phenotyp. Weiterhin konnte auch durch Transduktion des Ngn2-Proteins in murine ESZ neuronale Differenzierung ausgelöst werden, und zwar die Bildung neuronaler Vorläuferzellen. Zuletzt wird bewiesen, dass gerichtete Differenzierung von murinen ESZ durch einzelne MR Gene neben neuronalen Zelltypen auch die Bildung anderer somatischer Zellen erlaubt: Überexpression der Gene myoD oder cebpa induzierte die Differenzierung in Muskelzellen bzw. Macrophagen-ähnliche Zellen. Unter Verwendung transgener Zelllinien, die die Aktivierung jeweils eines MRs erlauben, war es möglich, gemischte Kulturen zu erhalten, in denen zwei verschiedene Differenzierungsprozesse parallel abliefen. Diese Studie zeigt, dass die Überexpression einzelner Gene ausreichend ist, um gerichtete Differenzierungsprozesse in einen bestimmten Zelltyp auszulösen. Die erfolgreiche Durchführung dieses Ansatzes wird nicht nur mit verschiedenen Genen und somit verschiedenen resultierenden Zelltypen nachgewiesen, sondern auch in verschiedenen Stammzelltypen aus Fisch und Maus. Dies erlaubt die Schlussfolgerung, dass bestimmte Gene in vitro das Schicksal von Stammzellen festlegen können und dass diese Fähigkeit eine konservierte Eigenschaft in Wirbeltieren zu sein scheint. Somit präsentiert diese Arbeit neuen Erkenntnisse über die Rolle von MR bei der Festlegung von Zellidentitäten und in Differenzierungsprozessen. Weiterhin wird eine neue Methode zur Induktion gerichteter Differenzierung in Stammzellen aufgezeigt, die mehrere Vorteile in Bezug auf Effizienz, Geschwindigkeit und Reproduzierbarkeit hat. Auslösung von Differenzierung durch MR Gene bietet somit einen neuen vielversprechenden Ansatz mit potentieller Anwendung sowohl in Stammzellforschung, als auch in regenerativer Medizin. KW - Stammzelle KW - Zelldifferenzierung KW - Transkriptionsfaktor KW - Pluripotenz KW - Pluripotent stem cells KW - differentiation KW - transcription factors Y1 - 2011 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-54706 ER - TY - JOUR A1 - Klotz, Barbara A1 - Mentrup, Birgit A1 - Regensburger, Martina A1 - Zeck, Sabine A1 - Schneidereit, Jutta A1 - Schupp, Nicole A1 - Linden, Christian A1 - Merz, Cornelia A1 - Ebert, Regina A1 - Jakob, Franz T1 - 1,25-Dihydroxyvitamin D3 Treatment Delays Cellular Aging in Human Mesenchymal Stem Cells while Maintaining Their Multipotent Capacity JF - PLoS ONE N2 - 1,25-dihydroxyvitamin D3 (1,25D3) was reported to induce premature organismal aging in fibroblast growth factor-23 (Fgf23) and klotho deficient mice, which is of main interest as 1,25D3 supplementation of its precursor cholecalciferol is used in basic osteoporosis treatment. We wanted to know if 1,25D3 is able to modulate aging processes on a cellular level in human mesenchymal stem cells (hMSC). Effects of 100 nM 1,25D3 on hMSC were analyzed by cell proliferation and apoptosis assay, beta-galactosidase staining, VDR and surface marker immunocytochemistry, RT-PCR of 1,25D3-responsive, quiescence-and replicative senescence-associated genes. 1,25D3 treatment significantly inhibited hMSC proliferation and apoptosis after 72 h and delayed the development of replicative senescence in long-term cultures according to beta-galactosidase staining and P16 expression. Cell morphology changed from a fibroblast like appearance to broad and rounded shapes. Long term treatment did not induce lineage commitment in terms of osteogenic pathways but maintained their clonogenic capacity, their surface marker characteristics (expression of CD73, CD90, CD105) and their multipotency to develop towards the chondrogenic, adipogenic and osteogenic pathways. In conclusion, 1,25D3 delays replicative senescence in primary hMSC while the pro-aging effects seen in mouse models might mainly be due to elevated systemic phosphate levels, which propagate organismal aging. KW - perspectives KW - bone marrow KW - mutant mice KW - oxidative stress KW - transcription factors KW - vitamin-D-receptor KW - differentiation KW - tissue KW - 2',7'-dichlorofluorescin KW - homeostasis Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-133392 VL - 7 IS - 1 ER - TY - JOUR A1 - Amich, Jorge A1 - Schafferer, Lukas A1 - Haas, Hubertus A1 - Krappmann, Sven T1 - Regulation of Sulphur Assimilation Is Essential for Virulence and Affects Iron Homeostasis of the Human-Pathogenic Mould Aspergillus fumigatus JF - PLoS Pathogens N2 - Abstract Sulphur is an essential element that all pathogens have to absorb from their surroundings in order to grow inside their infected host. Despite its importance, the relevance of sulphur assimilation in fungal virulence is largely unexplored. Here we report a role of the bZIP transcription factor MetR in sulphur assimilation and virulence of the human pathogen Aspergillus fumigatus. The MetR regulator is essential for growth on a variety of sulphur sources; remarkably, it is fundamental for assimilation of inorganic S-sources but dispensable for utilization of methionine. Accordingly, it strongly supports expression of genes directly related to inorganic sulphur assimilation but not of genes connected to methionine metabolism. On a broader scale, MetR orchestrates the comprehensive transcriptional adaptation to sulphur-starving conditions as demonstrated by digital gene expression analysis. Surprisingly, A. fumigatus is able to utilize volatile sulphur compounds produced by its methionine catabolism, a process that has not been described before and that is MetR-dependent. The A. fumigatus MetR transcriptional activator is important for virulence in both leukopenic mice and an alternative mini-host model of aspergillosis, as it was essential for the development of pulmonary aspergillosis and supported the systemic dissemination of the fungus. MetR action under sulphur-starving conditions is further required for proper iron regulation, which links regulation of sulphur metabolism to iron homeostasis and demonstrates an unprecedented regulatory crosstalk. Taken together, this study provides evidence that regulation of sulphur assimilation is not only crucial for A. fumigatus virulence but also affects the balance of iron in this prime opportunistic pathogen. Author Summary Invasive pulmonary aspergillosis (IPA) is a life-threatening disease that affects primarily immunosuppressed patients. During the last decades the incidence of this disease that is accompanied by high mortality rates has increased. Since opportunistic pathogenic fungi, unlike other pathogens, do not express specific virulence factors, it is becoming more and more clear that the elucidation of fungal metabolism is an essential task to understand fungal pathogenicity and to identify novel antifungal targets. In this work we report genetic inactivation of the sulphur transcription regulator MetR in Aspergillus fumigatus and subsequent study of the resulting phenotypes and transcriptional deregulation of the mutant. Here we show that regulation of sulphur assimilation is an essential process for the manifestation of IPA. Moreover, a regulatory connection between sulphur metabolism and iron homeostasis, a further essential virulence determinant of A. fumigatus, is demonstrated in this study for the first time. A deeper knowledge of sulphur metabolism holds the promise of increasing our understanding of fungal virulence and might lead to improved antifungal therapy. KW - gene regulation KW - transcription factors KW - DNA transcription KW - aspergillus fumigatus KW - methionine KW - sulfur KW - fungal pathogens KW - sulfates Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-130372 VL - 9 IS - 8 ER - TY - JOUR A1 - Morschhäuser, Joachim A1 - Ramírez-Zavala, Bernardo A1 - Weyler, Michael A1 - Gildor, Tsvia A1 - Schmauch, Christian A1 - Kornitzer, Daniel A1 - Arkowitz, Robert T1 - Activation of the Cph1-Dependent MAP Kinase Signaling Pathway Induces White-Opaque Switching in Candida albicans JF - PLoS Pathogens N2 - Depending on the environmental conditions, the pathogenic yeast Candida albicans can undergo different developmental programs, which are controlled by dedicated transcription factors and upstream signaling pathways. C. albicans strains that are homozygous at the mating type locus can switch from the normal yeast form (white) to an elongated cell type (opaque), which is the mating-competent form of this fungus. Both white and opaque cells use the Ste11-Hst7-Cek1/Cek2 MAP kinase signaling pathway to react to the presence of mating pheromone. However, while opaque cells employ the transcription factor Cph1 to induce the mating response, white cells recruit a different downstream transcription factor, Tec1, to promote the formation of a biofilm that facilitates mating of opaque cells in the population. The switch from the white to the opaque cell form is itself induced by environmental signals that result in the upregulation of the transcription factor Wor1, the master regulator of white-opaque switching. To get insight into the upstream signaling pathways controlling the switch, we expressed all C. albicans protein kinases from a tetracycline-inducible promoter in a switching-competent strain. Screening of this library of strains showed that a hyperactive form of Ste11 lacking its N-terminal domain (Ste11ΔN467) efficiently stimulated white cells to switch to the opaque phase, a behavior that did not occur in response to pheromone. Ste11ΔN467-induced switching specifically required the downstream MAP kinase Cek1 and its target transcription factor Cph1, but not Cek2 and Tec1, and forced expression of Cph1 also promoted white-opaque switching in a Wor1-dependent manner. Therefore, depending on the activation mechanism, components of the pheromone-responsive MAP kinase pathway can be reconnected to stimulate an alternative developmental program, switching of white cells to the mating-competent opaque phase. KW - biofilms KW - candida albicans KW - library screening KW - pheromones KW - protein expressions KW - protein kinase signaling cascade KW - regulator genes KW - transcription factors Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-97281 ER - TY - JOUR A1 - Brand, Susanne A1 - Amann, Kerstin A1 - Mandel, Philipp A1 - Zimnol, Anna A1 - Schupp, Nicole T1 - Oxidative DNA Damage in Kidneys and Heart of Hypertensive Mice Is Prevented by Blocking Angiotensin II and Aldosterone Receptors JF - PLOS ONE N2 - INTRODUCTION: Recently, we could show that angiotensin II, the reactive peptide of the blood pressure-regulating renin-angiotensin-aldosterone-system, causes the formation of reactive oxygen species and DNA damage in kidneys and hearts of hypertensive mice. To further investigate on the one hand the mechanism of DNA damage caused by angiotensin II, and on the other hand possible intervention strategies against end-organ damage, the effects of substances interfering with the renin-angiotensin-aldosterone-system on angiotensin II-induced genomic damage were studied. METHODS: In C57BL/6-mice, hypertension was induced by infusion of 600 ng/kg • min angiotensin II. The animals were additionally treated with the angiotensin II type 1 receptor blocker candesartan, the mineralocorticoid receptor blocker eplerenone and the antioxidant tempol. DNA damage and the activation of transcription factors were studied by immunohistochemistry and protein expression analysis. RESULTS: Administration of angiotensin II led to a significant increase of blood pressure, decreased only by candesartan. In kidneys and hearts of angiotensin II-treated animals, significant oxidative stress could be detected (1.5-fold over control). The redox-sensitive transcription factors Nrf2 and NF-κB were activated in the kidney by angiotensin II-treatment (4- and 3-fold over control, respectively) and reduced by all interventions. In kidneys and hearts an increase of DNA damage (3- and 2-fold over control, respectively) and of DNA repair (3-fold over control) was found. These effects were ameliorated by all interventions in both organs. Consistently, candesartan and tempol were more effective than eplerenone. CONCLUSION: Angiotensin II-induced DNA damage is caused by angiotensin II type 1 receptor-mediated formation of oxidative stress in vivo. The angiotensin II-mediated physiological increase of aldosterone adds to the DNA-damaging effects. Blocking angiotensin II and mineralocorticoid receptors therefore has beneficial effects on end-organ damage independent of blood pressure normalization. KW - aldosterone KW - oxidative stress KW - transcription factors KW - kidneys KW - heart KW - hypertension KW - DNA damage KW - blood pressure Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-118011 SN - 1932-6203 VL - 9 IS - 12 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 - THES A1 - Hartmann, Laura T1 - Die funktionelle Rolle der Transkriptionsfaktoren bZIP1 und bZIP53 in der Arabidopsis thaliana- Wurzel nach Salstress T1 - The functional role of bZIP1 and bZIP53 transcription factors in salt treated roots of Arabisopsis thaliana N2 - Die zunehmende Versalzung des Bodens führt weltweit zu starken Ernteeinbußen. Ob- wohl die Wurzeln der Pflanzen als erstes mit dem Salzstress in Berührung kommen, ist noch nicht viel über Signaltransduktionswege in Wurzeln zur Anpassung der Pflanze an Salzstress bekannt. Die bZIP-Transkriptionsfaktoren der Gruppe S1, bZIP1 und bZIP53, werden gewebespezifisch in der Wurzel nach Salzstress aktiviert. In dieser Arbeit werden diese bZIPs in ein Netzwerk eingeordnet, von der Aktivierung der Tran- skriptionsfaktoren bis zur Funktion in der Regulation des Stoffwechsels in der salzgest- ressten Pflanze. Die Aktivierung von bZIP1 kann über verschiedene sowohl ionische als auch osmotische Stimuli erfolgen und ist abhängig von Calcium, der HEXOKINASE 1 und SnRK1- Kinasen (Snf1 RELATED PROTEIN KINASE 1). Die dunkelinduzierte Expression von bZIP1 wird HXK1-abhängig durch Glucose inhibiert, bei Energiemangelbedingungen ist die Aktivierung von bZIP1 SnRK1-abhängig. Beide Enzyme spielen auch in der salzinduzierten Expression von bZIP1 eine Rolle. Über Transkriptom- und Me- tabolomanalysen kann gezeigt werden, dass bZIP1 und bZIP53 an der Umprogram- mierung des Kohlenhydrat- und Aminosäuremetabolismus teilhaben. Besonders Gene der Glukoneogenese (PYRUVAT ORTHOPHOSPHAT DIKINASE und FRUCTOSE- 1,6-BISPHOS- PHATASE) bzw. des Aminosäurekatabolismus (BRANCHED- CHAIN AMINO ACID TRANSAMINASE 2, METHYLCROTONYL- COA-CARBOXYLASE A und HOMOGENTISATE 1,2-DIOXYGENASE ) werden von den Transkriptionsfaktoren reguliert. Das spricht für eine Umprogrammierung des Metabolismus und der Mobilisierung von Energie aus Aminosäuren zur Anpassung an die Stressbedingungen. Die Transkriptionsfaktoren der Gruppe S1 bilden vorzugsweise Heterodimere mit der Gruppe C. Mit Mutantenanalysen, die zum einen die Transkriptionsfaktoren des C/S1-Netzwerks und zum anderen Komponenten der Abscisinsäure (ABA) abhängigen Signaltransduktion beinhalten, konnte ein Signaltransduktionsnetzwerk aufgestellt werden, das die Antwort auf abiotischen Stress mittels des Signalwegs über ABA, SnRK2 und AREB (ABA RESPONSIVE ELEMENTS-BINDING PROTEIN) mit der SnRK1-vermittelten Antwort auf Energiemangelbedingungen in der Pflanze verknüpft. Die gefundenen stress- bzw. energieresponsiven Gene konnten nach den Mutantenana- lysen auf Grund ihrer unterschiedlichen Regulation in vier Klassen eingeteilt werden, wovon nur eine, die Klasse 4, von dem C/S1 Netzwerk reguliert wird. Die Klassen 1- 3 sind unabhängig von den bZIP-Transkriptionsfaktoren der Gruppe C. Die Klasse 1 bilden typische ABA-responsive Gene, die von den Gruppe A-bZIPs reguliert werden. Faktoren der Gruppe A sind auch an der Expression der Gene der Klasse 2 beteiligt, diese werden aber auch durch bZIP1 und bZIP53 induziert. Dieser Klasse konnten Gene zugeordnet werden, die im Abbau verzweigtkettiger Aminosäuren eine Rolle spielen. Am Aminosäureabbau sind außerdem die Gene der Klasse 2 beteiligt. Für diese Gene konnte eine Expressionsregulation durch bZIP1 und bZIP53 gezeigt werden. Für die Bestimmung möglicher Heterodimerisierungspartner bedarf es noch weiterer Analysen. Dieses Model, das den abitoschen Stress abhängigen ABA-Signalweg mit dem ener- gieabhängigen SnRK1-Signaltransduktionsweg verknüpft, zeigt die präzise Regulation von mindestens 4 Gen-Klassen, deren Expression durch die Kombination verschiedener bZIP-Transkriptionsfaktoren aktiviert wird. N2 - Increasing salinization of soil has led to significant crop loss worldwide. Notwith- standing the fact that plant roots are the first to be affected by salt stress, signal transduction pathways in roots for salt stress adaptation are still mostly unknown In this work the group S1 bZIP transcription factors bZIP1 and bZIP53 that are spe- cifically induced by salt stress in roots, were functionally characterized with respect to their role in salt stress response in plants. Transcriptional activation of bZIP1 can be mediated by both ionic and osmotic stimuli and is dependent on Ca2+, HEXO- KINASE 1 (HXK1) and the SnRK1 kinases (Snf1 RELATED PROTEIN KINASE 1). Dark induced expression of bZIP1 is inhibited by glucose depending on HXK1 acti- vity. In starvation conditions the transcription of bZIP1 is mediated by SnRK1. Here both signaling enzymes are shown to be involved in salt induced bZIP1 transcripti- on. Transcriptome and metabolome analyses reveal an important function of bZIP1 and bZIP53 concerning the reprogramming of primary carbohydrate and amino acid metabolism during salt stress in the Arabidopsis root. Particularly genes involved in gluconeogenesis (PYRUVAT ORTHOPHOSPHAT DIKINASE and FRUCTOSE-1,6- BISPHOSPHATASE )or amino acid catabolism (BRANCHED- CHAIN AMINO ACID TRANSAMINASE 2, METHYLCROTONYL- COA-CARBOXYLASE A and HOMO- GENTISATE 1,2-DIOXYGENASE) are regulated by these transcription factors. This points to reprogramming of metabolism and remobilization of energy by amino acid degradation under stress. Group S1 bZIPs preferably form heterodimers with group C bZIP transcription factors. Mutant analyses of C/S1 bZIPs and ABA signaling com- ponents, respectively, revealed a complex network connecting abiotic stress responses via ABA-SnRK2-AREB (ABA RESPONSIVE ELEMENTS-BINDING PROTEIN) to SnRK1 mediated starvation responses. The detected genes were grouped in four classes according to their different regulation, of which only class 4 is regulated by the C/S1 network. Classes 1-3 are controlled independently of group C transcription factors. Class 1 contains typical ABA responsive genes, regulated by group A bZIPs. These are also involved in gene expression of class 2 genes, which are as well induced by bZIP1 and bZIP53. Genes of branched chain amino acid catabolism belong to this class. Al- so involved in amino acid catabolism are genes of class 2, these genes were shown to be transcriptionally regulated by bZIP1 and bZIP53. Further analyses are required to reveal possible heterodimerization partners. This model, that links the abiotic stress responding ABA pathway to the energy dependent SnRK1 signaling pathway, reveals at least four gene classes that are very precisely regulated by combining different bZIP transcription factors. KW - Salzstress KW - salt KW - Transkriptionsfaktor KW - Ackerschmalwand KW - transcription factors KW - root KW - Wurzel Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-99423 ER - TY - JOUR A1 - Salat, Daniela A1 - Winkler, Anja A1 - Urlaub, Henning A1 - Gessler, Manfred T1 - Hey bHLH Proteins Interact with a FBXO45 Containing SCF Ubiquitin Ligase Complex and Induce Its Translocation into the Nucleus JF - PLoS One N2 - The Hey protein family, comprising Hey1, Hey2 and HeyL in mammals, conveys Notch signals in many cell types. The helix-loop-helix (HLH) domain as well as the Orange domain, mediate homo- and heterodimerization of these transcription factors. Although distinct interaction partners have been identified so far, their physiological relevance for Hey functions is still largely unclear. Using a tandem affinity purification approach and mass spectrometry analysis we identified members of an ubiquitin E3-ligase complex consisting of FBXO45, PAM and SKP1 as novel Hey1 associated proteins. There is a direct interaction between Hey1 and FBXO45, whereas FBXO45 is needed to mediate indirect Hey1 binding to SKP1. Expression of Hey1 induces translocation of FBXO45 and PAM into the nucleus. Hey1 is a short-lived protein that is degraded by the proteasome, but there is no evidence for FBXO45-dependent ubiquitination of Hey1. On the contrary, Hey1 mediated nuclear translocation of FBXO45 and its associated ubiquitin ligase complex may extend its spectrum to additional nuclear targets triggering their ubiquitination. This suggests a novel mechanism of action for Hey bHLH factors. KW - ubiquitination KW - glycerol KW - transcription factors KW - DNA-binding proteins KW - immunoprecipitation KW - protein interactions KW - protein domains Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-125769 VL - 10 IS - 6 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 - Klein-Hessling, Stefan A1 - Rudolf, Ronald A1 - Muhammad, Khalid A1 - Knobeloch, Klaus-Peter A1 - Maqbool, Muhammad Ahmad A1 - Cauchy, Pierre A1 - Andrau, Jean-Christophe A1 - Avots, Andris A1 - Talora, Claudio A1 - Ellenrieder, Volker A1 - Screpanti, Isabella A1 - Serfling, Edgar A1 - Patra, Amiya Kumar T1 - A threshold level of NFATc1 activity facilitates thymocyte differentiation and opposes notch-driven leukaemia development JF - Nature Communications N2 - NFATc1 plays a critical role in double-negative thymocyte survival and differentiation. However, the signals that regulate Nfatc1 expression are incompletely characterized. Here we show a developmental stage-specific differential expression pattern of Nfatc1 driven by the distal (P1) or proximal (P2) promoters in thymocytes. Whereas, preTCR-negative thymocytes exhibit only P2 promoter-derived Nfatc1β expression, preTCR-positive thymocytes express both Nfatc1β and P1 promoter-derived Nfatc1α transcripts. Inducing NFATc1α activity from P1 promoter in preTCR-negative thymocytes, in addition to the NFATc1β from P2 promoter impairs thymocyte development resulting in severe T-cell lymphopenia. In addition, we show that NFATc1 activity suppresses the B-lineage potential of immature thymocytes, and consolidates their differentiation to T cells. Further, in the pTCR-positive DN3 cells, a threshold level of NFATc1 activity is vital in facilitating T-cell differentiation and to prevent Notch3-induced T-acute lymphoblastic leukaemia. Altogether, our results show NFATc1 activity is crucial in determining the T-cell fate of thymocytes. KW - acute lymphocytic leukaemia KW - transcription factors KW - lymphocyte differentiation Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-172974 VL - 7 ER - TY - JOUR A1 - Telorac, Jonas A1 - Prykhozhij, Sergey V. A1 - Schöne, Stefanie A1 - Meierhofer, David A1 - Sauer, Sascha A1 - Thomas-Chollier, Morgane A1 - Meijsing, Sebastiaan H. T1 - Identification and characterization of DNA sequences that prevent glucocorticoid receptor binding to nearby response elements JF - Nucleic Acids Research N2 - Out of the myriad of potential DNA binding sites of the glucocorticoid receptor (GR) found in the human genome, only a cell-type specific minority is actually bound, indicating that the presence of a recognition sequence alone is insufficient to specify where GR binds. Cooperative interactions with other transcription factors (TFs) are known to contribute to binding specificity. Here, we reasoned that sequence signals preventing GR recruitment to certain loci provide an alternative means to confer specificity. Motif analyses uncovered candidate Negative Regulatory Sequences (NRSs) that interfere with genomic GR binding. Subsequent functional analyses demonstrated that NRSs indeed prevent GR binding to nearby response elements. We show that NRS activity is conserved across species, found in most tissues and that they also interfere with the genomic binding of other TFs. Interestingly, the effects of NRSs appear not to be a simple consequence of changes in chromatin accessibility. Instead, we find that NRSs interact with proteins found at sub-nuclear structures called paraspeckles and that these proteins might mediate the repressive effects of NRSs. Together, our studies suggest that the joint influence of positive and negative sequence signals partition the genome into regions where GR can bind and those where it cannot. KW - DNA sequencing KW - glucocorticoid receptor KW - DNA binding KW - transcription factors Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-166330 VL - 44 IS - 13 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 - Hampe, Irene A. I. A1 - Friedman, Justin A1 - Edgerton, Mira A1 - Morschhäuser, Joachim T1 - An acquired mechanism of antifungal drug resistance simultaneously enables Candida albicans to escape from intrinsic host defenses JF - PLoS Pathogens N2 - The opportunistic fungal pathogen Candida albicans frequently produces genetically altered variants to adapt to environmental changes and new host niches in the course of its life-long association with the human host. Gain-of-function mutations in zinc cluster transcription factors, which result in the constitutive upregulation of their target genes, are a common cause of acquired resistance to the widely used antifungal drug fluconazole, especially during long-term therapy of oropharyngeal candidiasis. In this study, we investigated if C. albicans also can develop resistance to the antimicrobial peptide histatin 5, which is secreted in the saliva of humans to protect the oral mucosa from pathogenic microbes. As histatin 5 has been shown to be transported out of C. albicans cells by the Flu1 efflux pump, we screened a library of C. albicans strains that contain artificially activated forms of all zinc cluster transcription factors of this fungus for increased FLU1 expression. We found that a hyperactive Mrr1, which confers fluconazole resistance by upregulating the multidrug efflux pump MDR1 and other genes, also causes FLU1 overexpression. Similarly to the artificially activated Mrr1, naturally occurring gain-of-function mutations in this transcription factor also caused FLU1 upregulation and increased histatin 5 resistance. Surprisingly, however, Mrr1-mediated histatin 5 resistance was mainly caused by the upregulation of MDR1 instead of FLU1, revealing a previously unrecognized function of the Mdr1 efflux pump. Fluconazole-resistant clinical C. albicans isolates with different Mrr1 gain-of-function mutations were less efficiently killed by histatin 5, and this phenotype was reverted when MRR1 was deleted. Therefore, antimycotic therapy can promote the evolution of strains that, as a consequence of drug resistance mutations, simultaneously have acquired increased resistance against an innate host defense mechanism and are thereby better adapted to certain host niches. KW - antimicrobial resistance KW - transcriptional control KW - Candida albicans KW - transcription factors KW - mutation KW - hyperexpression techniques KW - antifungals KW - point mutation Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-158883 VL - 13 IS - 9 ER - TY - JOUR A1 - Sturm, Laura A1 - Geißel, Bernadette A1 - Martin, Ronny A1 - Wagener, Johannes T1 - Differentially Regulated Transcription Factors and ABC Transporters in a Mitochondrial Dynamics Mutant Can Alter Azole Susceptibility of Aspergillus fumigatus JF - Frontiers in Microbiology N2 - Azole resistance of the fungal pathogen Aspergillus fumigatus is an emerging problem. To identify novel mechanisms that could mediate azole resistance in A. fumigatus, we analyzed the transcriptome of a mitochondrial fission/fusion mutant that exhibits increased azole tolerance. Approximately 12% of the annotated genes are differentially regulated in this strain. This comprises upregulation of Cyp51A, the azole target structure, upregulation of ATP-binding cassette (ABC) superfamily and major facilitator superfamily (MFS) transporters and differential regulation of transcription factors. To study their impact on azole tolerance, conditional mutants were constructed of seven ABC transporters and 17 transcription factors. Under repressed conditions, growth rates and azole susceptibility of the mutants were similar to wild type. Under induced conditions, several transcription factor mutants showed growth phenotypes. In addition, four ABC transporter mutants and seven transcription factor mutants exhibited altered azole susceptibility. However, deletion of individual identified ABC transporters and transcription factors did not affect the increased azole tolerance of the fission/fusion mutant. Our results revealed the ability of multiple ABC transporters and transcription factors to modulate the azole susceptibility of A. fumigatus and support a model where mitochondrial dysfunctions trigger a drug resistance network that mediates azole tolerance of this mold. KW - mitochondrial dynamics KW - azole resistance KW - efflux pumps KW - transcription factors Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-204874 SN - 1664-302X VL - 11 ER - TY - JOUR A1 - Fusi, Lorenza A1 - Paudel, Rupesh A1 - Meder, Katharina A1 - Schlosser, Andreas A1 - Schrama, David A1 - Goebeler, Matthias A1 - Schmidt, Marc T1 - Interaction of transcription factor FoxO3 with histone acetyltransferase complex subunit TRRAP modulates gene expression and apoptosis JF - Journal of Biological Chemistry N2 - Forkhead box O (FoxO) transcription factors are conserved proteins involved in the regulation of life span and age-related diseases, such as diabetes and cancer. Stress stimuli or growth factor deprivation promotes nuclear localization and activation of FoxO proteins, which—depending on the cellular context—can lead to cell cycle arrest or apoptosis. In endothelial cells (ECs), they further regulate angiogenesis and may promote inflammation and vessel destabilization implicating a role of FoxOs in vascular diseases. In several cancers, FoxOs exert a tumor-suppressive function by regulating proliferation and survival. We and others have previously shown that FoxOs can regulate these processes via two different mechanisms: by direct binding to forkhead-responsive elements at the promoter of target genes or by a poorly understood alternative process that does not require direct DNA binding and regulates key targets in primary human ECs. Here, we performed an interaction study in ECs to identify new nuclear FoxO3 interaction partners that might contribute to FoxO-dependent gene regulation. Mass spectrometry analysis of FoxO3-interacting proteins revealed transformation/transcription domain–associated protein (TRRAP), a member of multiple histone acetyltransferase complexes, as a novel binding partner of FoxO family proteins. We demonstrate that TRRAP is required to support FoxO3 transactivation and FoxO3-dependent G1 arrest and apoptosis in ECs via transcriptional activation of the cyclin-dependent kinase inhibitor p27\(^{kip1}\) and the proapoptotic B-cell lymphoma 2 family member, BIM. Moreover, FoxO–TRRAP interaction could explain FoxO-induced alternative gene regulation via TRRAP-dependent recruitment to target promoters lacking forkhead-responsive element sequences. KW - FoxO3 KW - TRRAP KW - transcription factors Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-299820 VL - 298 IS - 3 ER -