TY - JOUR A1 - Kober, Christina A1 - Rohn, Susanne A1 - Weibel, Stephanie A1 - Geissinger, Ulrike A1 - Chen, Nanhai G. A1 - Szalay, Aladar A. T1 - Microglia and astrocytes attenuate the replication of the oncolytic vaccinia virus LIVP 1.1.1 in murine GL261 gliomas by acting as vaccinia virus traps JF - Journal of Translational Medicine N2 - Background Oncolytic virotherapy is a novel approach for the treatment of glioblastoma multiforme (GBM) which is still a fatal disease. Pathologic features of GBM are characterized by the infiltration with microglia/macrophages and a strong interaction between immune- and glioma cells. The aim of this study was to determine the role of microglia and astrocytes for oncolytic vaccinia virus (VACV) therapy of GBM. Methods VACV LIVP 1.1.1 replication in C57BL/6 and \(Foxn1^{nu/nu}\) mice with and without GL261 gliomas was analyzed. Furthermore, immunohistochemical analysis of microglia and astrocytes was investigated in non-, mock-, and LIVP 1.1.1-infected orthotopic GL261 gliomas in C57BL/6 mice. In cell culture studies virus replication and virus-mediated cell death of GL261 glioma cells was examined, as well as in BV-2 microglia and IMA2.1 astrocytes with M1 or M2 phenotypes. Co-culture experiments between BV-2 and GL261 cells and apoptosis/necrosis studies were performed. Organotypic slice cultures with implanted GL261 tumor spheres were used as additional cell culture system. Results We discovered that orthotopic GL261 gliomas upon intracranial virus delivery did not support replication of LIVP 1.1.1, similar to VACV-infected brains without gliomas. In addition, recruitment of \(Iba1^+\) microglia and \(GFAP^+\) astrocytes to orthotopically implanted GL261 glioma sites occurred already without virus injection. GL261 cells in culture showed high virus replication, while replication in BV-2 and IMA2.1 cells was barely detectable. The reduced viral replication in BV-2 cells might be due to rapid VACV-induced apoptotic cell death. In BV-2 and IMA 2.1 cells with M1 phenotype a further reduction of virus progeny and virus-mediated cell death was detected. Application of BV-2 microglial cells with M1 phenotype onto organotypic slice cultures with implanted GL261 gliomas resulted in reduced infection of BV-2 cells, whereas GL261 cells were well infected. Conclusion Our results indicate that microglia and astrocytes, dependent on their activation state, may preferentially clear viral particles by immediate uptake after delivery. By acting as VACV traps they further reduce efficient virus infection of the tumor cells. These findings demonstrate that glia cells need to be taken into account for successful GBM therapy development. KW - GBM KW - tumor microenvironment KW - microglia KW - polarization KW - VACV KW - OSC KW - IMA2.1 KW - BV-2 Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-126517 VL - 13 IS - 216 ER - TY - JOUR A1 - Tomei, Sara A1 - Adams, Sharon A1 - Uccellini, Lorenzo A1 - Bedognetti, Davide A1 - De Giorgi, Valeria A1 - Erdenebileg, Narnygerel A1 - Libera Ascierto, Maria A1 - Reinboth, Jennifer A1 - Liu, Qiuzhen A1 - Bevilacqua, Generoso A1 - Wang, Ena A1 - Mazzanti, Chiara A1 - Marincola, Francesco M. T1 - Association between HRAS rs12628 and rs112587690 polymorphisms with the risk of melanoma in the North American population JF - Medical Oncology N2 - HRAS belongs to the RAS genes superfamily. RAS genes are important players in several human tumors and the single-nucleotide polymorphism rs12628 has been shown to contribute to the risk of bladder, colon, gastrointestinal, oral, and thyroid carcinoma. We hypothesized that this SNP may affect the risk of cutaneous melanoma as well. HRAS gene contains a polymorphic region (rs112587690), a repeated hexanucleotide -GGGCCT- located in intron 1. Three alleles of this region, P1, P2, and P3, have been identified that contain two, three, and four repeats of the hexanucleotide, respectively. We investigated the clinical impact of these polymorphisms in a case–control study. A total of 141 melanoma patients and 118 healthy donors from the North America Caucasian population were screened for rs12628 and rs112587690 polymorphisms. Genotypes were assessed by capillary sequencing or fragment analysis, respectively, and rs12628 CC and rs112587690 P1P1 genotypes significantly associated with increased melanoma risk (OR = 3.83, p = 0.003; OR = 11.3, p = 0.033, respectively), while rs112587690 P1P3 frequency resulted significantly higher in the control group (OR = 0.5, p = 0.017). These results suggest that rs12628 C homozygosis may be considered a potential risk factor for melanoma development in the North American population possibly through the linkage to rs112587690. KW - HRAS KW - polymorphism KW - melanoma KW - rs12628 KW - rs112587690 Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-126834 VL - 29 IS - 5 ER - TY - JOUR A1 - Kirscher, Lorenz A1 - Deán-Ben, Xosé Luis A1 - Scadeng, Miriam A1 - Zaremba, Angelika A1 - Zhang, Qian A1 - Kober, Christina A1 - Fehm, Thomas Felix A1 - Razansky, Daniel A1 - Ntziachristos, Vasilis A1 - Stritzker, Jochen A1 - Szalay, Aladar A. T1 - Doxycycline Inducible Melanogenic Vaccinia Virus as Theranostic Anti-Cancer Agent JF - Theranostics N2 - We reported earlier the diagnostic potential of a melanogenic vaccinia virus based system in magnetic resonance (MRI) and optoacoustic deep tissue imaging (MSOT). Since melanin overproduction lead to attenuated virus replication, we constructed a novel recombinant vaccinia virus strain (rVACV), GLV-1h462, which expressed the key enzyme of melanogenesis (tyrosinase) under the control of an inducible promoter-system. In this study melanin production was detected after exogenous addition of doxycycline in two different tumor xenograft mouse models. Furthermore, it was confirmed that this novel vaccinia virus strain still facilitated signal enhancement as detected by MRI and optoacoustic tomography. At the same time we demonstrated an enhanced oncolytic potential compared to the constitutively melanin synthesizing rVACV system. KW - reporter gene KW - oncolysis KW - molecular imaging KW - virotherapy Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-124987 VL - 5 IS - 10 ER - TY - JOUR A1 - Adelfinger, Marion A1 - Bessler, Simon A1 - Cecil, Alexander A1 - Langbein-Laugwitz, Johanna A1 - Frentzen, Alexa A1 - Gentschev, Ivaylo A1 - Szalay, Aladar A. T1 - Preclinical Testing Oncolytic Vaccinia Virus Strain GLV-5b451 Expressing an Anti-VEGF Single-Chain Antibody for Canine Cancer Therapy JF - Viruses N2 - Virotherapy on the basis of oncolytic vaccinia virus (VACV) strains is a novel approach for canine cancer therapy. Here we describe, for the first time, the characterization and the use of VACV strain GLV-5b451 expressing the anti-vascular endothelial growth factor (VEGF) single-chain antibody (scAb) GLAF-2 as therapeutic agent against different canine cancers. Cell culture data demonstrated that GLV-5b451 efficiently infected and destroyed all four tested canine cancer cell lines including: mammary carcinoma (MTH52c), mammary adenoma (ZMTH3), prostate carcinoma (CT1258), and soft tissue sarcoma (STSA-1). The GLV-5b451 virus-mediated production of GLAF-2 antibody was observed in all four cancer cell lines. In addition, this antibody specifically recognized canine VEGF. Finally, in canine soft tissue sarcoma (CSTS) xenografted mice, a single systemic administration of GLV-5b451 was found to be safe and led to anti-tumor effects resulting in the significant reduction and substantial long-term inhibition of tumor growth. A CD31-based immuno-staining showed significantly decreased neo-angiogenesis in GLV-5b451-treated tumors compared to the controls. In summary, these findings indicate that GLV-5b451 has potential for use as a therapeutic agent in the treatment of CSTS. KW - canine cancer therapy KW - canine soft tissue sarcoma (CSTS) KW - oncolytic virus KW - cancer KW - canine cancer cell lines KW - antibody production KW - angiogenesis Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-125705 VL - 7 ER - TY - JOUR A1 - Tsoneva, Desislava A1 - Stritzker, Jochen A1 - Bedenk, Kristina A1 - Zhang, Qian A1 - Cappello, Joseph A1 - Fischer, Utz A1 - Szalay, Aladar A. T1 - Drug-encoded Biomarkers for Monitoring Biological Therapies JF - PLoS One N2 - Blood tests are necessary, easy-to-perform and low-cost alternatives for monitoring of oncolytic virotherapy and other biological therapies in translational research. Here we assessed three candidate proteins with the potential to be used as biomarkers in biological fluids: two glucuronidases from E. coli (GusA) and Staphylococcus sp. RLH1 (GusPlus), and the luciferase from Gaussia princeps (GLuc). The three genes encoding these proteins were inserted individually into vaccinia virus GLV-1h68 genome under the control of an identical promoter. The three resulting recombinant viruses were used to infect tumor cells in cultures and human tumor xenografts in nude mice. In contrast to the actively secreted GLuc, the cytoplasmic glucuronidases GusA and GusPlus were released into the supernatants only as a result of virus-mediated oncolysis. GusPlus resulted in the most sensitive detection of enzyme activity under controlled assay conditions in samples containing as little as 1 pg/ml of GusPlus, followed by GusA (25 pg/ml) and GLuc (≥375 pg/ml). Unexpectedly, even though GusA had a lower specific activity compared to GusPlus, the substrate conversion in the serum of tumor-bearing mice injected with the GusA-encoding virus strains was substantially higher than that of GusPlus. This was attributed to a 3.2 fold and 16.2 fold longer half-life of GusA in the blood stream compared to GusPlus and GLuc respectively, thus a more sensitive monitor of virus replication than the other two enzymes. Due to the good correlation between enzymatic activity of expressed marker gene and virus titer, we conclude that the amount of the biomarker protein in the body fluid semiquantitatively represents the amount of virus in the infected tumors which was confirmed by low light imaging. We found GusA to be the most reliable biomarker for monitoring oncolytic virotherapy among the three tested markers. KW - mouse models KW - vaccinia virus KW - luciferase KW - biomarkers KW - cytolysis KW - viral replication KW - cell cultures KW - blood Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-125265 VL - 10 IS - 9 ER - TY - JOUR A1 - Gentschev, Ivaylo A1 - Patil, Sadeep S. A1 - Petrov, Ivan A1 - Cappello, Joseph A1 - Adelfinger, Marion A1 - Szalay, Aladar A. T1 - Oncolytic Virotherapy of Canine and Feline Cancer JF - Viruses N2 - Cancer is the leading cause of disease-related death in companion animals such as dogs and cats. Despite recent progress in the diagnosis and treatment of advanced canine and feline cancer, overall patient treatment outcome has not been substantially improved. Virotherapy using oncolytic viruses is one promising new strategy for cancer therapy. Oncolytic viruses (OVs) preferentially infect and lyse cancer cells, without causing excessive damage to surrounding healthy tissue, and initiate tumor-specific immunity. The current review describes the use of different oncolytic viruses for cancer therapy and their application to canine and feline cancer. KW - oncolytic virus KW - oncolysis KW - cancer KW - canine and feline cancer therapy Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-119753 VL - 6 IS - 5 ER - TY - JOUR A1 - Donat, Ulrike A1 - Rother, Juliane A1 - Schäfer, Simon A1 - Hess, Michael A1 - Härtl, Barbara A1 - Kober, Christina A1 - Langbein-Laugwitz, Johanna A1 - Stritzker, Jochen A1 - Chen, Nanhai G. A1 - Aguilar, Richard J. A1 - Weibel, Stephanie A1 - Szalay, Alandar A. T1 - Characterization of Metastasis Formation and Virotherapy in the Human C33A Cervical Cancer Model JF - PLoS ONE N2 - More than 90% of cancer mortalities are due to cancer that has metastasized. Therefore, it is crucial to intensify research on metastasis formation and therapy. Here, we describe for the first time the metastasizing ability of the human cervical cancer cell line C33A in athymic nude mice after subcutaneous implantation of tumor cells. In this model, we demonstrated a steady progression of lumbar and renal lymph node metastases during tumor development. Besides predominantly occurring lymphatic metastases, we visualized the formation of hematogenous metastases utilizing red fluorescent protein (RFP) expressing C33A-RFP cells. RFP positive cancer cells were found migrating in blood vessels and forming micrometastases in lungs of tumor-bearing mice. Next, we set out to analyze the influence of oncolytic virotherapy in the C33A-RFP model and demonstrated an efficient virus-mediated reduction of tumor size and metastatic burden. These results suggest the C33A-RFP cervical cancer model as a new platform to analyze cancer metastases as well as to test novel treatment options to combat metastases. KW - metastasis KW - renal cancer KW - oncolytic viruses KW - lymph nodes KW - kidneys KW - lung and intrathoracic tumors KW - secondary lung tumors KW - cancer treatment Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-119674 SN - 1932-6203 VL - 9 IS - 6 ER - TY - THES A1 - Chari, Ashwin T1 - The Reaction Mechanism of Cellular U snRNP Assembly T1 - Der Reaktionsmechanismus zellulärer U snRNP Zusammenlagerung N2 - Macromolecular complexes, also termed molecular machines, facilitate a large spectrum of biological reactions and tasks crucial to the survival of cells. These complexes are composed of either protein only, or proteins bound to nucleic acids (DNA or RNA). Prominent examples for each class are the proteosome, the nucleosome and the ribosome. How such units are assembled within the context of a living cell is a central question in molecular biology. Earlier studies had indicated that even very large complexes such as ribosomes could be reconstituted from purified constituents in vitro. The structural information required for the formation of macromolecular complexes, hence, lies within the subunits itself and, thus, allow for self- assembly. However, increasing evidence suggests that in vivo many macromolecular complexes do not form spontaneously but require assisting factors (“assembly chaperones”) for their maturation. In this thesis the assembly of RNA-protein (RNP) complexes has been studied by a combination of biochemical and structural approaches. A resourceful model system to study this process is the biogenesis pathway of the uridine-rich small nuclear ribonucleoproteins (U snRNPs) of the spliceosome. This molecular machine catalyzes pre-mRNA splicing, i.e. the removal of non-coding introns and the joining of coding exons to functional mRNA. The composition and architecture of U snRNPs is well defined, also, the nucleo-cytoplasmic transport events enabling the formation of these particles in vivo have been analyzed in some detail. Furthermore, recent studies suggest that the formation of U snRNPs in vivo is mediated by an elaborate assembly machinery consisting of protein arginine methyltransferase (PRMT5)- and survival motor neuron (SMN)-complexes. The elucidation of the reaction mechanism of cellular U snRNP assembly would serve as a paradigm for our understanding of how RNA-protein complexes are formed in the cellular environment. The following key findings were obtained as part of this study: 1) Efforts were made to establish a full inventory of the subunits of the SMN-complex. This was achieved by the biochemical definition and characterization of an atypical component of this complex, the unrip protein. This protein is associated with the SMN-complex exclusively in the cytoplasm and influences its subcellular localization. 2) With a full inventory of the components in hand, the architecture of the SMN-complex was defined on the basis of an interaction map of all subunits. This study elucidated that the proteins SMN, Gemin7 and Gemin8 form a backbone, onto which the remaining subunits adhere in a modular manner. 3) The two studies mentioned above formed the basis to elucidate the reaction mechanism of cellular U snRNP assembly. Initially, an early phase in the SMN-assisted formation of U snRNPs was analyzed. Two subunits of the U7 snRNP (LSm10 and 11) were found to interact with the PRMT5-complex, without being methylated. This report suggests that the stimulatory role of the PRMT5-complex is independent of its methylation activity. 4) Key reaction intermediates in U snRNP assembly were found and characterized by a combination of biochemistry and structural studies. Initially, a precursor to U snRNPs with a sedimentation coefficient of 6S is formed by the pICln subunit of the PRMT5-complex and Sm proteins. This intermediate was shown to constitute a kinetic trap in the U snRNP assembly reaction. Progression towards the assembled U snRNP depends on the activity of the SMN-complex, which acts as a catalyst. The formation of U snRNPs is shown to be structurally similar to the way clamps are deposited onto DNA to tether poorly processive polymerases. 5) The human SMN-complex is composed of several subunits. However, it is unknown whether all subunits of this entity are essential for U snRNP assembly. A combination of bioinformatics and biochemistry was applied to tackle this question. By mining databases containing whole-genome assemblies, the SMN-Gemin2 heterodimer is recognized as the most ancestral form of the SMN-complex. Biochemical purification of the Drosophila melanogaster SMN-complex reveals that this complex is composed of the same two subunits. Furthermore, evidence is provided that the SMN-Gemin2 heterodimer is necessary and sufficient to promote faithful U snRNP assembly. Future studies will adress further details in the reaction mechanism of cellular U snRNP assembly. The results obtained in this thesis suggest that the SMN and Gemin2 subunits are sufficient to promote U snRNP formation. What then is the function of the remaining subunits of the SMN-complex? The reconstitution schemes established in this thesis will be instrumental to address this question. Furthermore, additional mechanistic insights into the U snRNP assembly reaction will require the elucidation of structures of the assembly machinery trapped at various states. The prerequisite for these structural studies, the capability to generate homogenous complexes in sufficient amounts, has been accomplished in this thesis. N2 - Makromolekulare Komplexe, auch molekulare Maschinen genannt, ermöglichen eine grosse Vielfalt biologischer Reaktionen und Aufgaben, die für das Überleben von Organismen kritisch sind. Diese Komplexe bestehen entweder nur aus Protein, oder setzen sich aus Protein und Nukleinsäure (DNA oder RNA) zusammen. Prominente Beispiele für diese Klassen molekularer Maschinen sind das Proteosom, das Nukleosom oder das Ribosom. Wie sich solche Einheiten innerhalb einer Zelle zusammenlagern ist eine grundlegende Frage der Molekularbiologie. Frühere Studien hatten angeduetet, dass es möglich ist sogar sehr grosse Komplexe wie das Ribosom in vitro aus gereinigten Bestandteilen zu einem aktiven Partikel zu rekonstruieren. Die Strukturinformation, die für die Bildung von makromolekularen Komplexen erforderlich ist, liegt also in den Untereinheiten selbst. Im Gegensatz dazu mehren sich heute die Hinweise dafür, dass sich viele makromolekulare Komplexe nicht spontan zusammenlagern, sondern die Aktivität assistierender Faktoren („Assembly Chaperone“) für ihre Reifung benötigen. In dieser Arbeit wurde der Zusammenbau von RNA-Protein (RNP) Partikeln durch eine Kombination aus Biochemie und Strukturbiologie untersucht. Ein ergiebiges System, um diesen Prozess zu studieren, ist die Biogenese der RNPs (U snRNPs) des Spleissosoms. Aufgabe dieser molekularen Maschine ist das Herausschneiden nicht-kodierender Introns und das Zusammenfügen kodiereneder Exons um so funktionelle mRNA zu bilden. Die Zusammensetzung und Architektur von U snRNPs sind gut definiert. Auch ist der Kern- Zytoplasma Transport, der für die Reifung dieser Partikel notwendig sind, detailliert beschrieben worden. Außerdem weisen neueste Studien darauf hin, dass die Bildung von U snRNPs in vivo durch eine komplexe Maschinerie, die aus den Protein-Arginin- Methyltransferase 5 (PRMT5)- und Survival-Motor-Neuron (SMN)- Komplexen besteht, vermittelt wird. Die Entschlüsselung des Reaktionsmechanismus des zellulärem U snRNP Zusammenbaus würde als Musterbeispiel für unser Verständnis dienen, wie RNPs in einer Zelle gebildet werden. Folgende Erkenntnisse wurden in dieser Arbeit gewonnen: 1) Es wurde zunächst versucht eine komplette Bestandsliste der Untereinheiten des SMN-Komplexes zu erstellen. Dies wurde durch die biochemische Definition und Charakterisierung einer atypischen Komponente dieses Komplexes, des Unrip Proteins, erreicht. Dieses Protein bindet ausschliesslich im Zytoplasma an den SMN-Komplex und beeinflusst dessen subzelluläre Lokalisation. 2) Die komplette Inventarisierung des SMN-Komplexes ermöglichte die Untersuchung der Wechselwirkung aller Untereinheiten und somit die Untersuchung seiner Architektur. Diese Studie zeigte, dass die Proteine SMN, Gemin7 und Gemin8 das Rückgrat des SMN-Komplexes bilden auf dem die restlichen Untereinheiten modular angeordnet werden. 3) Die zwei oben erwähnten Studien bildeten die Grundlage, den Reaktionsmechanismus zellulärer U snRNP Zusammenlagerung zu entschlüsseln. Zunächst wurde eine frühe Phase im SMN-vermittelten U snRNP Zusammenbau analysiert. Es konnte gezeigt werden, dass zwei Untereinheiten des U7 snRNP (LSm10 und 11) mit dem PRMT5-Komplex wechselwirken, ohne methyliert zu werden. Dies deutet darauf hin, dass die unterstützende Rolle des PRMT5-Komplexes von seiner Methylierungsaktivität unabhängig ist. 4) Schlüsselintermediate im Zusammenschluss von U snRNPs wurden identifiziert und durch eine Kombination von Biochemie und Strukturbiologie charakterisiert. In einer ersten Stufe bildet sich ein Vorgänger von U snRNPs mit einem Sedimentationskoeffizienten von 6S aus. Dieses Intermediat, bestehend aus pICln (einer Untereinheit des PRMT5-Komplexes) und Sm Proteinen, stellt eine kinetische Falle in der U snRNP Zusammenlagerung dar. Das Voranschreiten zum maturen U snRNP hängt von der Aktivität des SMN-Komplexes ab, der als Katalysator wirkt. Weiterhin konnte gezeigt werden, dass die Ausbildung von U snRNPs strukturell ähnlich zu der Reaktion verläuft, die Polymerasen mit geringer Prozessivität an der DNA verankert und die als „clamp-loading“ bezeichnet wird. 5) Der menschliche SMN-Komplex setzt sich aus mehreren Untereinheiten zusammen. Es ist jedoch unbekannt, ob alle Teile des Komplexes für die Zusammenlagerung von U snRNPs notwendig sind. Diese Frage wurde durch eine Kombination aus Bioinformatik und Biochemie adressiert. Durch Datenbanksuchen in komplett sequenzierten Genomen wurde festgestellt, dass die evolutionär ursprüngliche Form des SMN-Komplexes aus den zwei Proteinen SMN und Gemin2 besteht. Die biochemische Reinigung des Komplexes der Taufliege Drosophila melanogaster offenbarte, dass er auch in diesem Organismus aus denselben zwei Untereinheiten zusammengebaut ist. Außerdem wurde der Beweis erbracht, dass das SMN-Gemin2 heterodimer notwendig und hinreichend ist, um U snRNPs akkurat zusammenzulagern. Zukünftige Studien werden weitere detaillierte Ansichten des Reaktionsmechanismus in der zellulären Zusammenlagerung von U snRNPs liefern. Die Ergebnisse, die in der vorliegenden Arbeit erhalten wurden, deuten darauf hin, dass die Untereinheiten SMN und Gemin2 des SMN-Komplexes für den Zusammenbau von U snRNPs hinreichend sind. Was also ist die Funktion der weiteren Untereinheiten des SMN-Komplexes? Die Rekonstitutionsschemata, die in dieser Arbeit etabliert wurden, werden essentiell für die Beantwortung dieser Frage sein. Darüberhinaus werden weitere mechanistische Einsichten in die Zusammenlagerung von U snRNPs von der Ermittlung von Strukturen der Assembly-Maschinerie in verschiedenen Zuständen abhängen. Die Voraussetzung für diese strukturbiologische Untersuchungen, die Möglichkeit ausreichende Mengen homogener Komplexe herzustellen, ist ebenfalls in dieser Arbeit geschaffen worden. KW - Small nuclear RNP KW - Katalysator KW - Enzym KW - Maschine KW - Biopolymere KW - Makromolekül KW - Biogenese KW - Reaktionsmechanismus KW - Small nuclear RNP KW - Catalyst KW - Enzyme KW - Molecular Machine KW - Chaperone KW - Macromolecular Complex Y1 - 2009 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-40804 ER - TY - THES A1 - Markert, Andreas T1 - LARP7 – ein La ähnliches Protein reguliert die Elongation der PolII Transkription durch das 7SK RNP T1 - LARP7 - a La related protein regulates the elongation of polII transcription by the 7SK RNP N2 - Genexpression in Eukaryoten beschreibt einen mehrstufigen Prozess, welcher auf Ebene der Transkription durch den positiven Transkriptionselongationsfaktor P-TEFb entscheidend reguliert wird. PTEFb bildet einen heterodimeren Komplex aus der Cyclin abhängigen Kinase 9 und deren Kofaktor Cyclin T1/2. Dieser Komplex aktiviert die Elongation der Transkription durch Phosphorylierung der negativen Elongationsfaktoren DSIF und NELF. Darüber hinaus phosphoryliert PTEFb Serin2 Reste in der C-terminalen Domäne von RNA PolII und stimuliert so die kotranskriptionelle Prozessierung der synthetisierten prä-mRNA. In Anpassung an unterschiedliche Wachstumsbedingungen wird die Aktivität dieses Faktors durch reversible Interaktion mit 7SK RNA und HEXIM Proteinen innerhalb eines katalytisch inaktiven Ribonukleoproteinpartikels (7SK RNP) streng kontrolliert. Dieses sensible Gleichgewicht zwischen P-TEFb auf der einen und dem 7SK RNP auf der anderen Seite bildet die Grundlage der Regulation der Transkriptionselongation. Trotz der hohen Abundanz von 7SK RNA in der Zelle, assoziiert in vivo jedoch nur ein relativ kleiner Teil hiervon mit P-TEFb, sodass die effektiv zur Verfügung stehende RNA-Menge für die Bildung des 7SK RNP vermutlich limitierend wirkt. Ziel der vorliegenden Arbeit war es daher neue 7SK RNA interagierende Faktoren zu identifizieren, welche die Interaktion von PTEFb mit dem 7SK RNP steuern und so die PolII abhängige Transkription regulieren. Anhand verschiedener chromatographischer Reinigungen konnte zunächst ein bislang uncharakterisiertes La ähnliches Protein (LARP7) mit einer spezifischen Affinität für Pyrimidinreiche RNAs isoliert werden. LARP7 bindet, wie durch immunbiochemische Analysen und RNA- Bindungsstudien gezeigt werden konnte, quantitativ an das hoch konservierte uridylreiche 3´- Ende von 7SK RNA. Diese Assoziation erfordert dessen La- und RRMDomänen und erhöht wesentlich die Stabilität der RNA. Darüber hinaus kofraktioniert LARP7 mit weiteren Faktoren des 7SK RNP, bindet direkt an HEXIM1 und P-TEFb und stellt somit ebenfalls eine integrale Komponente des 7SK RNP dar. Die gewonnenen Daten weisen außerdem erstmals darauf hin, dass P-TEFb durch einen vorgeformten trimeren Komplexes, bestehend aus HEXIM1, 7SK RNA und LARP7 inhibiert wird. Reportergenanalysen in TZMbl-Zellen, welche Luziferase unter der Kontrolle des streng P-TEFb abhängigen HIV-1-LTRPromotors exprimieren zeigten, dass diese Inhibition im Wesentlichen durch LARP7 vermittelt wird. So ließ sich nach Reduktion der LARP7 Expression mittels RNAi eine signifikante Steigerung der Transkription vom HIV-1-LTR-Promotor beobachten. Eine ähnliche Stimulation der Transkription von PolII konnte in LARP7 defizienten HeLa-Zellen durch quantitative Real-Time-PCR auch für eine Reihe zellulärer Gene nachgewiesen werden. Die Beobachtung, dass LARP7 die generelle PolII Transkription reprimiert, korreliert zudem mit einer bereits beschriebenen Tumorsupressorfunktion des LARP7 homologen mxc Proteins aus D. melanogaster. Somit beeinflusst LARP7 das zelluläre Gleichgewicht zwischen freiem und 7SK RNP-gebundenem P-TEFb und fungiert somit als negativer Regulator der PolII Transkription in vivo. N2 - Eucaryotic gene expression is a multistep process, which is critically regulated on the level of RNA polII transcription by the positive transcription elongation factor P-TEFb. P-TEFb forms a heterodimeric complex, consisting of the cyclin-dependent kinase 9 and its cofactor cyclin T1/2. This complex stimulates transcriptional elongation as well as the cotranscriptional processing of the synthesized pre-mRNA by phosphorylation of negative elongation factors and the RNA polII Cterminal domain. To accommodate different growth conditions, P-TEFb activity is kept under tight control through its reversible interaction with 7SK RNA and HEXIM proteins in a catalytically inactive ribonucleoprotein particle (RNP). This sensitive balance between PTEFb on the one hand and the 7SK RNP on the other represents the basis of transcriptional regulation of elongation. Despite the high abundance of 7SK RNA in the cell, only a small part is associated with P-TEFb in vivo, suggesting that the actual amount of RNA available limits the formation of the 7SK RNP. Hence, the objective of the present study was to identify novel 7SK RNA interacting factors, which direct the interaction of P-TEFb with the 7SK RNP, thereby regulating polII dependent transcription. At first, using different chromatographic purification strategies, an as yet uncharacterized La related protein (LARP7) with an affinity to pyrimidine- rich RNAs was isolated. Immunobiochemical analysis and RNA binding studies revealed, that LARP7 quantitatively associates with the highly conserved 3´-UUU-OH terminus of 7SK RNA. This binding requires its La- and RRM-domain and dramatically increases RNA stability. Moreover, LARP7 co-fractionates with additional factors of the 7SK RNP, binds directly to HEXIM1 and P-TEFb and therefore likewise constitutes an integral component of the 7SK RNP. Data presented here indicate that P-TEFb is inhibited upon association with a trimeric complex consisting of HEXIM1, 7SK RNA and LARP7. Furthermore, reporter gene analysis in TZMbl cells - cells expressing luciferase under the control of the strictly P-TEFb dependent HIV-1-LTR promoter - demonstrated this inhibition to be mainly mediated by LARP7. Thus, reduction of LARP7 expression by RNA-interference led to a significant stimulation of transcription in TZMbl cells. In addition, quantitative real time pcr revealed a similar effect on transcription for a series of cellular genes in LARP7 deficient HeLa cells. Moreover, the observation, that LARP7 represses polII transcription in general correlates well with a known function of the d. melanogaster LARP7 homologue mxc as a tumor suppressor. Thus, LARP7 affects the cellular P-TEFb/7SK RNP equilibrium und serves as a negative regulator of polII transcription in vivo. KW - LARP7 KW - P-TEFb KW - 7SK RNA KW - Transkription KW - Elongation KW - LARP7 KW - P-TEFb KW - 7SK RNA KW - transcription KW - elongation Y1 - 2009 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-41773 ER - TY - THES A1 - Bedenk, Kristina T1 - Biochemische und strukturelle Charakterisierung der Genexpressionsmaschinerie des Vaccinia Virus T1 - The biochemical and structural characterization of the gene expression machinery of the Vaccinia virus N2 - Die Familie der Pockenviren zeichnet sich durch ein komplexes DNA Genom aus und hat großes medizinisches Potential. Am eindrucksvollsten ist dies für das Vaccinia-Virus (VACV) belegt, welches nicht nur als Pocken-Impfstoff eingesetzt wird, sondern auch als onkolytisches Virus in der Tumorbiologie. VACV hat einen außergewöhnlichen Replikationszyklus, welcher ausschließlich im Zytoplasma der Wirtszelle stattfindet. Somit ist die gesamte virale Genexpressionsmaschinerie völlig unabhängig von kernvermittelten Reaktionen des Wirts und somit auch aus Sicht der Grundlagenforschung von größtem Interesse. Die Schlüsselkomponente der viralen Genexpression ist die makromolekulare DNA-abhängige RNA Polymerase (vvRPO), deren Untereinheiten allesamt Virus-kodiert sind. Zwar wurden in den letzten Jahren Protokolle zur biochemischen und funktionellen Charakterisierung der vvRPO etabliert, ein detailliertes Wissen über deren Zusammenlagerung in vivo und die räumlichen und zeitlichen Interaktionen mit den Transkriptions- bzw. Prozessierungsfaktoren sind aber weitgehend unbekannt. Diese Arbeit umfasst Untersuchungen zur strukturellen und funktionellen Charakterisierung der vvRPO und seiner assoziierten Faktoren. Grundlage hierfür war die Etablierung eines Reinigungsprotokolls mithilfe eines neu konstruierten rekombinanten VACV (GLV-1h439). Diese Strategie erlaubte es hoch-molekulare native vvRPO Komplexe zu isolieren. Ein transkriptions-inaktiver Komplex (Komplex I) mit einer kalkulierten Masse von 575 kDa bestand aus den acht Untereinheiten des vvRPO Holoenzyms und den Polymerase-assoziierten Faktoren RAP94 und D6. Ein zweiter, transkriptionell aktiver Komplex (Komplex II) mit einer Masse von 803 kDa enthielt, neben dem Holoenzym der vvRPO, noch weitere Faktoren, die primär die Erkennung der DNA-Matrize und die Prozessierung der naszierenden RNA vermitteln. Hierbei handelt es sich um RAP94, das virale Capping Enzym bestehend aus den zwei Untereinheiten D1 und D12, A7 und dem Terminationsfaktor NPH I. Interessanterweise enthielt dieser Komplex zusätzlich mit E11 eine bislang unbekannte weitere Protein-Komponente, sowie tRNAGln und tRNAArg. Der isolierte Kompelx II ist daher ein Ribonukleoprotein (RNP). Die Verfügbarkeit von hoch-reinen vvRPO Komplexen erlaubte es erstmals deren strukturelle Architektur zu untersuchen. Hierfür wurden drei experimentelle Ansätze, die klassische Röntgenstrukturanalyse, die Kryo-Elektronenmikroskopie (Kryo-EM) und Quervernetzungssstudien miteinander kombiniert. Die Strukturen der Komplexe I und II haben eine Auflösung von 11-12 Å, wobei auffällig war, dass beide eine markante strukturelle Ähnlichkeit zur eukaryotischen RNA Polymerase II aufwiesen. Darüber hinaus gelang es zusätzliche Bereiche im Komplex II zu definieren, welche die Polymerase-assoziierten Prozessierungsfaktoren beherbergen. Zudem konnte die atomare Struktur von E11, mittels Röntgenstrukturanalyse bei einer Auflösung von 1,9 Å, gelöst werden. Das E11 Protein besitzt ein neuartiges Faltungsmuster und weist einen intensiven Dimerisierungskontakt auf, welcher sich über vier ß-Faltblätter ausbildet. Die im Rahmen dieser Arbeit erhaltenen Daten legen die Grundlage für ein detailliertes Verständnis der räumlichen Organisation der viralen Transkriptonsmaschinerie. Darüber hinaus werden sie funktionelle Studien ermöglichen, welche die Rolle der einzelnen Proteine, sowie der tRNAs bei der mRNA Synthese klären helfen. N2 - Poxviruses comprise a diverse family of complex DNA-genome viruses with great medical potenial. This is exemplified by vaccinia virus, which not only served as a vaccine against smallpox but is also used as a promising tool in viral anti-cancer therapies. A key feature that distinguishes the poxvirus family from other DNA viruses is their replication cycle, which is confined to the cytoplasm. This results in a high level of independence from the host cell, which supports transcription and replication events only in the nucleus. Accordingly, virus specific, rather than host cell enzymes mediate most processes including DNA replication and mRNA synthesis. The key component of viral gene expression is the DNA-dependent RNA polymerase (vvRPO), which constitutes the virus-encoded macromolecular machine ensuring viral mRNA synthesis. Although this enzyme has been studied in some details in the past years, neither its mode of assembly in vivo nor its spatio-temporal association with transcription and processing factors has been understood in detail. In this thesis I present work that focuses on the structural and functional characterization of vvRPO and its associated factors. To gain insights into the structure and the assembly of the VACV transcription system we established an efficient purification protocol by generating recombinant virus strains expressing tagged subunits of vvRPO (GLV-1h439). These recombinant virus strains enabled the isolation of high molecular weight vvRPO complexes. Complex I, which was transcriptionally inactive in vitro displayed a calculated mass of about 575 kDa, consisted of eight subunits of the vvRPO holoenzym and two additional polymerase-associated factors termed RAP94 and D6. A second, transcriptionally active complex (complex II) with a mass of 803 kDa, was related to the first one. It consisted apart from the factors of the holoenzyme already found in complex I additional factors that mediate primarily binding of the polymerase to its DNA template and the processing of nascent RNA. These factors comprise the viral capping enzyme (D1, D12), A7 and the termination factor NPH I. Interestingly, complex II contained in addition the viral protein E11, thus far not connected to viral transcription als well as tRNAGln, tRNAArg). Complex II is hence a ribonucleoprotein (RNP). The availability of highly pure vvRPO complexes allowed for the first time to investigate their structure. To this end, three experimental approaches, the classic X-ray crystallography, cryo-electron microscopy (cryo-EM) and chemical crosslinking were combined. Structures of both polymerase complexes were obtained at a resolution of 11-12 Å and revealed a striking structural similarity to eukaryotic RNA polymerase II. Moreover, it was possible to allocate positions in the structure of complex II that are likely to harbour the polymerase-associated processing factors. In addition we were able to solve atomic structure of E11 by X-ray crystallography at a resolution of 1.9 Å. Interestingly, the structure of E11 showed a novel folding pattern that forms a dimer, which is mostly composed of four ß-sheets. These studies provide the basis for a detailed investigation of the architecture of the viral transcriptional machinery. Furthermore, the pave the way for functional studies aimed at elucidating the function of individual proteins and tRNA in the generation of viral mRNA. KW - Vaccinia-Virus KW - Vaccinia-Virus KW - Genexpressionsmaschinerie KW - RNA-Polymerase KW - Struktur KW - Genexpression Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-135538 ER -