Rinderpest Virus Transcription : Functional Dissection Of Viral RNA Polymerase And Role Of Host Factor Ebp1 In Virus Multiplication

Gopinath, M

01 1900

Rinderpest virus (RPV) belongs to the order Mononegavirale which comprises non segmented negative sense RNA viruses including human pathogens such as Measles, Ebola and Marburg virus. RPV is the causative agent of Rinderpest disease in large ruminants, both domesticated and wild. The viral genome contains a non segmented negative sense RNA encapsidated by nucleocapsid protein (N-RNA). Viral transcription/replication is carried out by the virus encoded RNA dependent RNA polymerase represented by the large protein L and phosphoprotein P as (L-P) complex. Viral transcription begins at the 3’ end of the genome 3’le-N-P-M-F-H-N-tr-5’ with the synthesis of 55nt leader RNA followed by the synthesis of other viral mRNAs. A remarkable feature common to all members of Paramyxoviridae family is the gradient of transcription from 3’ end to the 5’ end of the genome due to attenuation of polymerase transcription at each gene junction. The present study aims at functional characterization of Rinderpest virus transcription and the associated activities required for viral mRNA capping. In addition, an attempt has been made to understand the novel role of a host factor, Ebp1, playing a key role in virus multiplication in infected cells. The specific aims of the study are presented in detail below. 1. Development of in vitro transcription system for RPV mRNA synthesis and role of phosphorylation of P protein in transcription. The transition of viral polymerase from transcription to replication in infected cells has been a long standing puzzle in all paramyxoviruses. Earlier work carried out using RPV minigenome with a CAT reporter gene and studies with phosphorylation null mutant P, has revealed the importance of P phosphorylation for viral transcription in vivo. However, the contribution of other cellular factors in the viral transcription/replication switch could not be ruled out in these assays. In order to understand the specific role of P protein in transcription/replication, it was necessary to develop a cell free transcription system for viral mRNA synthesis. Hence, viral genomic RNA (N-RNA) was purified from RPV infected cells using CsCl density gradient centrifugation. The viral RNA polymerase consisting of L-P complex was separately expressed in insect cells and partially purified by glycerol gradient centrifugation. Glycerol gradient fraction containing the L-P complex was found to be active in viral transcription. Notably, the gradient of transcription of viral mRNA was observed in vitro with the partially purified recombinant L-P complex similar to in vivo. However, the recombinant polymerase complex failed to synthesis the 55nt leader RNA, in agreement with the recent finding in VSV that the transcriptase complex was unable to synthesize leader RNA and viral transcription is initiated at the N gene start site unlike the conventional 3’ entry mode. The newly developed in vitro reconstituted transcription system was used to analyze the effect of P phosphorylation on viral transcription. The results presented in chapter 2, indicate that phosphorylated P supports transcription whereas unphosphorylated P transdominantly inhibits the transcription in vitro suggesting the possible role of the status of P protein phosphorylation in determining transcription/replication switch. 2. Enzymatic activities associated with RPV L protein- role in viral mRNA capping. Post transcriptional modification of mRNA such as capping and methylation determines the translatability of viral mRNA by cellular ribosome. In negative sense RNA viruses, synthesis of viral mRNA is carried out by the viral encoded RNA polymerase in the host cell cytoplasm. Since the host capping and methylation machinery is localized to the nucleus, viruses should either encode their own mRNA modification enzymes or adopt alternative methods as has been reported for orthomyxoviruses (cap snatching) and picornaviruses (presence of IRES element). In order to test, if RPV RNA polymerase possesses any of the capping and methylation activities, both virus as well as the RNP complex containing the viral N-RNA and RNA polymerase (L-P) were purified from infected cells. Using the purified virus and RNP complex, the first two activities required for mRNA capping vis-à-vis, RNA triphosphatase and guanylyltransferase were tested and the results are described in chapter 3 and 4. Purified virus as well as the RNP complex showed both RNA triphosphatase (RTPase) and Nucleotide triphosphatase activities. Neither purified N-RNA or recombinant P proteins show these activities suggesting that it is indeed mediated by viral L protein. By the metal dependency of the reaction and by the motif conservation with other reported RTPases, RPV L protein was assigned to the metal dependent RTPase tunnel family. Capping activity was also seen with the L protein present in RNP complex by its ability to form a covalent complex with GMP moiety of GTP. The specificity of the reaction with GTP, inhibition of Enzyme-GMP complex formation by the inorganic pyrophosphate and the susceptibility of Enzyme-GMP complex under acidic conditions clearly indicated that RPV L represents the viral guanylyl transferase. Further confirmation was obtained by the indirect capping assay in which Enzyme-GMP complex was formed when recombinant L protein was incubated with the cap labeled RNA due to the reversible nature of capping reaction. Owing to the large size of L protein (240 KDa), it is conceivable that the L protein functions in a modular fashion for different activities pertaining to RNA synthesis and modification. Sequence comparison of L proteins from different morbilliviruses revealed the presence of three conserved domains namely domain I (aa 1-606), domain II (aa 650-1694) and domain III (aa 1717-2183). Since domain II has already been assigned as the viral RNA dependent RNA polymerase, domain I and domain III were chosen for further characterization. Both domains were cloned, expressed and purified to homogeneity using recombinant baculovirus expression system. However, the recombinant domain III alone showed the NTPase activity where as neither domain I or III showed RTPase activity. This is expected since a part of the conserved RTPase motif was located in domain II in the multiple sequence alignment with other viral and yeast RTPases. In addition, the recombinant domain III also showed the characteristic enzyme-GMP complex formation but failed to be active in the indirect capping assay. Therefore, both domain II and domain III are likely to be involved in the co-transcriptional capping of viral mRNA. In support of this view, recent report in VSV suggests the presence of additional motif in domain II which is essential for viral mRNA capping. Preliminary evidence has been presented in the appendix section for the presence of N7 guanine methyl transferase activity with L protein although further experiments are needed to confirm this activity. 3. Role of host factor Ebp1 in negative sense RNA virus replication - a possible antagonist In recent years, many cellular factors such as actin, tubulin and profilin have been shown to be involved in viral transcription. Ebp1-ErbB3 binding protein was initially isolated as a cellular protein which binds to Influenza viral polymerase subunit PB1. Ebp1 selectively inhibits the influenza virus transcription in vitro whereas the cap binding and endonuclease activity of PB1 subunit of viral polymerase is unaffected. Till now there are no reports of the role of Ebp1 in non segmented negative sense RNA virus infection. The fifth chapter describes the role of Ebp1 in RPV infection and vice versa. RPV infection leads to down regulation of Ebp1 mRNA levels which in turn leads to decreased protein synthesis. Subsequently, it was found that Ebp1 interacts presumably with viral N protein, being a part of the viral RNP complex in both infected cells as well as in purified virion. Further, over expression of Ebp1 inhibits viral transcription and as a consequence the virus multiplication in vivo suggesting a mutual antagonism between virus and the host cell through Ebp1 protein.

Rinderpest Virus Transcription

RNA Polymerase

Virus Multiplication

Host Factor Ebp1

Rinderpest Virus L Protein

Viral mRNA Synthesis

Viral mRNA Capping

Rinderpest Virus (RPV)

Biochemical Genetics

Fluorescence nanoscopy in three dimensions / Fluoreszenz-Nanoskopie in drei Dimensionen

Geisler, Claudia

15 December 2009

No description available.

530 Physik

Mathematics and Computer Science

Mikroskopie

Hochauflösung

4Pi

PALM

SMS

photoschalten

microscopy

high resolution

4Pi

PALM

SMS

photoswitching

33.18

42.03

RPV 280: Mikroskop {Physik: Optik}

Methods to improve the sample quality of macromolecular complexes for structure determination by 3D Electron Cryo-Microscopy / Methoden zur Verbesserung der Probenqualität makromolekularer Komplexe zur Strukturbestimmung mittels 3D Kryo-Elektronenmikroskopie

Platzmann, Florian Peter

24 February 2012

No description available.

570 Biowissenschaften

Biologie

RPV 750

Kryo-Elektronenmikroskopie

Probenvorbereitung

Electron Cryo-Microscopy

sample preparation

42.03

42.13

Quantitation Strategies in Optically Sectioning Fluorescence Microscopy / Quantifizierungsstrategien in der optisch schnittbildenden Fluoreszenzmikroskopie

Weigel, Arwed

15 January 2009

No description available.

570 Biowissenschaften

Biologie

Fluoreszenzmikroskopie

optische Schnittbildung

strukturierte Beleuchtung

konfokale Mikroskopie

ApoTome

SIPchart

fluorescence microscopy

optical sectioning

structured illumination microscopy

confocal microscopy

ApoTome

SIPchart

42.03

RPV 280: Mikroskop {Physik: Optik}

Spektroskopie und Polarimetrie kleinskaliger magnetischer Strukturen der Sonnenoberfläche mit Methoden der Bildrekonstruktion / Spectroscopy and polarimetry of small-scale magnetic structures on the solar surface with image restoration techniques

Koschinsky, Markus

03 May 2001

No description available.

530 Physik

Mathematics and Computer Science

Spektroskopie

Interferometrie

Polarimetrie

Speckle

Phase Diversity

seeing

Sun

granulation

magnetic fields

plage

pore

sunspot

Fabry-Perot-interferometer

image processing

image reconstruction

image restoration

spectroscopy

interferometry

polarimetry

speckle

phase diversity

seeing

Sun

granulation

magnetic fields

plage

pore

sunspot

Fabry-Perot-interferometer

image processing

image reconstruction

image restoration

33.18

39.51

TGC 100: Sonnenbeobachtung {Astronomie}

TGC 740: Sonnenatmosphäre

RPV 000: Instrumentelle Optik {Physik}

RPV 800: Interferometrie {Physik}

RR 000: Spektroskopie {Physik}

TGC 100: Sonnenbeobachtung {Astronomie}

TGC 300: Sonnenspektrum {Astronomie}

TGC 500: Sonnenaktivität {Astronomie}

TGC 520: Sonnenflecken {Astronomie}

TGC 540: Sonnenfackeln {Astronomie}

RPC 000: Wellenoptik {Physik}

RPV 200: Optische Instrumente {Physik}

RPV 260: Fernrohr

Teleskop {Physik: Optik}

RPV 340: Filter {Physik: Optik}

RPV 360: Interferometer {Physik: Optik}

TCG 000: Astronomische Optik

TCG 200

Mikrostrukturelle Untersuchungen an Mangan-dotiertem Galliumnitrid mittels fortgeschrittener Methoden der hochauflösenden und analytischen Transmissionselektronenmikroskopie / Microstructural investigations of Manganese-doped Gallium Nitride by modern methods of high resolution and analytical transmission electron microscopy

Niermann, Tore

30 October 2006

No description available.

530 Physik

Mathematics and Computer Science

Transmissionselektronenmikroskopie

Mikrostruktur

Kristalldefekte

Galliumnitrid

Mangan

Transmission electron microscopy

microstructure

crystal defects

Gallium Nitride

Manganese

33.05

33.61

RPV 750: Elektronenmikroskopie {Physik}

Molecular dynamics of clathrin proteins at endocytic sites studied with evanescent-wave microscopy / Untersuchung der molekularen Dynamik von Clathrin mit Totalreflektionsmikroskopie

Loerke, Dinah

12 February 2004

No description available.

530 Physik

Mathematics and Computer Science

Clathrin

light chain

heavy chain

FRAP

Photobleichen

Austausch

Totalreflektion

Fluoreszenz

Mikroskopie

clathrin

light chain

heavy chain

FRAP

photobleaching

exchange

evanescent

fluorescence microscopy

33.05

42.03

42.12

RPV 720: Mikroskopie {Physik}

WC 000: Biophysik

Identification of the Minimal Domain of RNA Trihosphastase Activity in the L Protien of Rinderpest Virus and Charecterization of its Enzymatic Activities

Singh, Piyush Kumar

January 2013

Morbilliviruses belong to the family Paramyxoviridae of the Mononegavirale order of viruses. The Mononegavirale order contains viruses which contain negatively-polar, non-segmented and single stranded RNA genomes. This order contains some of most lethal pathogens known to the humankind. Ebola virus and Marburg virus are perhaps the most lethal human pathogens. Rinderpest virus, declared eradicated in 2011, was known to be the most significant cattle killer. Similarly the Canine distemper virus and Rabies virus, two topmost canine pathogens belong to this order. The L protein in the viruses of Morbillivirus genus harbours the viral RNA-dependent RNA polymerase that replicates and transcribes the viral genome and also all the mRNA capping enzymes, viz. RNA 5’ triphosphatase, guanylyltransferase, RNA (guanine-7-)methyltransferase and RNA 5’ cap-dependent (2’-oxo-)methyltransferase. Moreover this protein can act as a protein kinase that can regulate the function of P protein which serves as a switch between transcription and replication. mRNA capping is necessary for the virus for the purpose of exploiting host cellular machinery towards viral protein synthesis. The Rinderpest virus L protein serves as a model to study the capping enzymes of Morbillivirus. RNA triphosphatase (RTPase), the first enzyme of the capping cascade had earlier been located on the L protein. The RTPase minimal domain on the L protein was identified earlier by sequence homology studies done with RTPase proteins of Baculovirus and Vaccinia virus and cloned. The bacterially expressed recombinant domain was shown to possess RTPase activity. The enzymatic activity was characterized and the RTPase was found to be a metal-dependent enzyme which is highly specific to capping viral mRNA. Further characterization of the domain revealed that the domain also possesses nucleotide triphosphatase (NTPase), tripolyphosphatase and pyrophosphatase activities. Two site-directed mutants in motif-A of the domain: E1645A and E1647A were also tested and were found to be essential for the RTPase and NTPase activity. It was also recognized through these mutant studies that the active sites of RTPase and NTPase activities are partially overlapping. Earlier work done with Vesicular stomatitis virus capping enzymes showed that the Rhabdoviridae family of viruses follow unconventional capping pathway utilizing an enzyme polyribonucleotidyltransferase (PRNTase) which transfers GDP to 5’-monophosphated RNA. Characterization of the RTPase activity which converts 5’-triphosphated RNA into 5’-diphosphated RNA is an evidence for the morbilliviruses utilizing the conventional eukaryotic capping cascade. The results show that Paramyxoviridae do not follow unconventional capping pathway for the mRNA capping as has been the paradigm in the past decade.

Rinderpest Virus (RPV)

Viral Replication

Viral Transcription

Viral Structure

Viral RNA Synthesis

Morbilliviruses

Rinderpest Virus L Protein

Viral Proteins - Synthesis

Viruses - Reproduction

Viral Proteins

Viruses - RNA Capping

Viral Genome Organization

Viral RNA

L Protein

Virology

Experimental and numerical studies on the micromechanical crystal plasticity behavior of an RPV steel / Etudes expérimentales et numériques de plasticité cristalline d’un acier de cuve

Shi, Qiwei

23 April 2018

Cette thèse vise à étudier le comportement mécanique de l’acier de cuve 16MND5 (ou A508cl3 pour la norme anglaise) à l’échelle de la microstructure en croisant des approches expérimentale et numérique. Plusieurs contributions au développement de l’essai de traction in-situ à l’intérieur de MEB ont été apportées. En premier, les biais de mesure de différentes modalités (BSE, EBSD et SE) d’acquisition d’images sous MEB ont été caractérisés et corrigés. Les images MEB de différentes modalités ont été corrélées de façon précise afin de décrire la topographie de l’éprouvette. Les images d’orientation cristallographique (EBSD) ont été corrélées afin de révéler la rotation cristalline et les champs de déplacement de surface au long de la traction. La déformation élastique de l’éprouvette a été mesurée par corrélation intégrée des images de diffraction électronique à haute-résolution. Les microstructures fines de l’éprouvette à trois dimensions après déformation ont été mesurées par FIB-EBSD. L’essai a également été simulé par calcul de plasticité cristalline sur un maillage 3D, basé sur les microstructures mesurées dans la configuration déformée. Un algorithme a été proposé pour estimer la configuration initiale de l’éprouvette et identifier les paramètres de loi de plasticité en procédant par itérations. Un cas test synthétique 2D a été employé pour valider la faisabilité de l’algorithme. Deux lois de plasticité cristalline ont été testées sur le maillage 3D: dynamique des dislocations des cristaux cubiques centrés, et une version modifiée de la loi Méric-Cailletaud. Pour cette dernière loi, deux jeux de paramètres ont été identifiés pour les ferrites et bainites par recalage des éléments finis. / The PhD project is devoted to the study of the mechanical response of the reactor pressure vessel steel A508cl3 (or 16MND5 in French nomenclature) at the microscopic scale by experimental analyses and numerical simulations. Different aspects of in-situ tests inside an SEM chamber have been considered. First, the characterization and corrections of bias and uncertainties of different SEM imaging modalities (SE, BSE, and EBSD) have been performed. Precise registrations of SEM images in different modalities have been developed in order to give a comprehensive description of the sample surface topographies. Crystallographic orientation maps (from EBSD analyses) are registered to measure the crystal rotation and displacement fields along the tensile test. The elastic deformations of the surface are assessed by integrated correlation of high-resolution electron diffraction images. The 3D microstructure of the analyzed sample is revealed a posteriori by combining FIB milling andEBSD images.The experimental test is also simulated by crystal plasticity calculations on a 3D mesh created according to the 3D microstructure observed in the deformed configuration. An algorithm has been proposed to estimate its initial configuration and to identify the plastic parameters iteratively. A synthetic 2D model has been used to prove its feasibility. Two crystal plasticity laws have been validated on the 3D mesh, namely dislocation dynamics for body-centered cubic crystals and a modified version of Méric-Cailletaud model. In thepresent work finite element model updating was used to provide two sets of parameters (for ferrite and bainite) for the latter law.

Plasticité cristalline

Acier de cuve

Recalage de modèles éléments finis

Corrélation d'images numériques

Microscope électronique à balayage

Rotation cristalline

Crystal plasticity

RPV steel

Finite element model updating

Digital image correlation

Scanning electron microscope

Crystal rotation

Fast STED Microscopy / Schnelle STED-Mikroskopie

Lauterbach, Marcel

15 December 2009

No description available.

530 Physik

Mathematics and Computer Science

Schnelle STED-Mikroskopie

Strahlabtastung

Neurotransmittervesikel

Vesikel

Kolloide

Kolloidkristalle

Monolage

in vivo STED-Mikroskopie

Zweifarben-STED-Mikroskopie

Mehrfarbige STED-Mikroskopie

TIMP-1

CD-63

Integrin

Mitochondrien

TOM

Proteinverteilung

Geschichte der Beugungsgrenze

Abbe

Auflösung

Fast STED Microscopy

beam-scanning

beamscanning

neurotransmitter vesicles

neurotransmittervesicles

colloids

colloidal crystals

monolayer

in vivo STED microscopy

two-color STED microscopy

TIMP-1

CD63

Integrin

mitochondria

TOM

protein distribution

history of diffraction

Abbe

resolution

42.12

33.18

42.03

50.37

RPV 280: Mikroskop {Physik: Optik}

RPV 720: Mikroskopie {Physik}

WC 100: Biophysikalische Methoden

MED 272: Biophysik {Medizin}

AHI 470