Your search keyword '"Weisberg AS"' showing total 122 results

1. Inactivation of Genes by Frameshift Mutations Provides Rapid Adaptation of an Attenuated Vaccinia Virus

Author

Erik K. Zhivkoplias, Bernard Moss, Andrea S. Weisberg, and Tatiana G. Senkevich

Subjects

viruses, Immunology, Adaptation, Biological, Gene Dosage, Vaccinia virus, Virus Replication, Microbiology, Virus, Cell Line, Frameshift mutation, Viral Proteins, chemistry.chemical_compound, Serial passage, Virology, Chlorocebus aethiops, Animals, Orthopoxvirus, Frameshift Mutation, Gene, Recombination, Genetic, Base Sequence, Whole Genome Sequencing, biology, Myxoma virus, Epithelial Cells, biology.organism_classification, Recombinant Proteins, Genetic Diversity and Evolution, chemistry, Viral replication, Codon, Nonsense, Insect Science, Viral evolution, Genetic Fitness, Rabbits, Vaccinia, Transcription Factors

Abstract

Unlike RNA viruses, most DNA viruses replicate their genomes with high-fidelity polymerases that rarely make base substitution errors. Nevertheless, experimental evolution studies have revealed rapid acquisition of adaptive mutations during serial passage of attenuated vaccinia virus (VACV). One way in which adaptation can occur is by an accordion mechanism in which the gene copy number increases followed by base substitutions and, finally, contraction of the gene copy number. Here, we show rapid acquisition of multiple adaptive mutations mediated by a gene-inactivating frameshift mechanism during passage of an attenuated VACV. Attenuation had been achieved by exchanging the VACV A8R intermediate transcription factor gene with the myxoma virus ortholog. A total of seven mutations in six different genes occurred in three parallel passages of the attenuated virus. The most frequent mutations were single-nucleotide insertions or deletions within runs of five to seven As or Ts, although a deletion of 11 nucleotides also occurred, leading to frameshifts and premature stop codons. During 10 passage rounds, the attenuated VACV was replaced by the mutant viruses. At the end of the experiment, virtually all remaining viruses had one fixed mutation and one or more additional mutations. Although nucleotide substitutions in the transcription apparatus accounted for two low-frequency mutations, frameshifts in genes encoding protein components of the mature virion, namely, A26L, G6R, and A14.5L, achieved 74% to 98% fixation. The adaptive role of the mutations was confirmed by making recombinant VACV with A26L or G6R or both deleted, which increased virus replication levels and decreased particle/PFU ratios. IMPORTANCE Gene inactivation is considered to be an important driver of orthopoxvirus evolution. Whereas cowpox virus contains intact orthologs of genes present in each orthopoxvirus species, numerous genes are inactivated in all other members of the genus. Inactivation of additional genes can occur upon extensive passaging of orthopoxviruses in cell culture leading to attenuation in vivo, a strategy for making vaccines. Whether inactivation of multiple viral genes enhances replication in the host cells or has a neutral effect is unknown in most cases. Using an experimental evolution protocol involving serial passages of an attenuated vaccinia virus, rapid acquisition of inactivating frameshift mutations occurred. After only 10 passage rounds, the starting attenuated vaccinia virus was displaced by viruses with one fixed mutation and one or more additional mutations. The high frequency of multiple inactivating mutations during experimental evolution simulates their acquisition during normal evolution and extensive virus passaging to make vaccine strains.

Published

2020

2. Inactivation of Genes by Frameshift Mutations Provides Rapid Adaptation of an Attenuated Vaccinia Virus

Author

Senkevich, Tatiana G., primary, Zhivkoplias, Erik K., additional, Weisberg, Andrea S., additional, and Moss, Bernard, additional

Published

2020

3. Human Papillomavirus 16 Capsids Mediate Nuclear Entry during Infection

Author

Douglas R. Lowy, Yuk Ying S. Pang, Patricia M. Day, Michelle Hughes, Cynthia D. Thompson, John T. Schiller, and Andrea S. Weisberg

Subjects

viruses, Immunology, Biology, Microbiology, Virus, Cell Line, chemistry.chemical_compound, Capsid, Viral entry, Virology, Animals, Humans, Mitosis, Host cell nucleus, Cell Nucleus, Human papillomavirus 16, Papillomavirus Infections, Oncogene Proteins, Viral, Virus Internalization, Virus-Cell Interactions, Cell biology, Vesicular transport protein, Disease Models, Animal, Microscopy, Electron, chemistry, Insect Science, Capsid Proteins, Nuclear localization sequence, DNA

Abstract

Infectious human papillomavirus 16 (HPV16) L1/L2 pseudovirions were found to remain largely intact during vesicular transport to the nucleus. By electron microscopy, capsids with a diameter of 50 nm were clearly visible within small vesicles attached to mitotic chromosomes and to a lesser extent within interphase nuclei, implying nuclear disassembly. By confocal analysis, it was determined that nuclear entry of assembled L1 is dependent upon the presence of the minor capsid protein, L2, but independent of encapsidated DNA. We also demonstrate that L1 nuclear localization and mitotic chromosome association can occur in vivo in the murine cervicovaginal challenge model of HPV16 infection. These findings challenge the prevailing concepts of PV uncoating and disassembly. More generally, they document that a largely intact viral capsid can enter the nucleus within a transport vesicle, establishing a novel mechanism by which a virus accesses the nuclear cellular machinery. IMPORTANCE Papillomaviruses (PVs) comprise a large family of nonenveloped DNA viruses that include HPV16, among other oncogenic types, the causative agents of cervical cancer. Delivery of the viral DNA into the host cell nucleus is necessary for establishment of infection. This was thought to occur via a subviral complex following uncoating of the larger viral capsid. In this study, we demonstrate that little disassembly of the PV capsid occurs prior to nuclear delivery. These surprising data reveal a previously unrecognized viral strategy to access the nuclear replication machinery. Understanding viral entry mechanisms not only increases our appreciation of basic cell biological pathways but also may lead to more effective antiviral interventions.

Published

2019

4. Retrograde Transport from Early Endosomes to the trans -Golgi Network Enables Membrane Wrapping and Egress of Vaccinia Virus Virions

Author

Bernard Moss, Andrea S. Weisberg, Jeffrey L. Americo, and Gilad Sivan

Subjects

0301 basic medicine, Endosome, viruses, Immunology, Vaccinia virus, Endosomes, Biology, Endocytosis, Microbiology, Exocytosis, Cell membrane, 03 medical and health sciences, symbols.namesake, Virology, medicine, Humans, Monkeypox virus, Virus Release, Secretory pathway, Microscopy, Confocal, Cell Membrane, Virion, Biological Transport, Golgi apparatus, Virus-Cell Interactions, Cell biology, Microscopy, Electron, 030104 developmental biology, Secretory protein, medicine.anatomical_structure, Insect Science, symbols, HeLa Cells, trans-Golgi Network

Abstract

The anterograde pathway, from the endoplasmic reticulum through the trans -Golgi network to the cell surface, is utilized by trans -membrane and secretory proteins. The retrograde pathway, which directs traffic in the opposite direction, is used following endocytosis of exogenous molecules and recycling of membrane proteins. Microbes exploit both routes: viruses typically use the anterograde pathway for envelope formation prior to exiting the cell, whereas ricin and Shiga-like toxins and some nonenveloped viruses use the retrograde pathway for cell entry. Mining a human genome-wide RNA interference (RNAi) screen revealed a need for multiple retrograde pathway components for cell-to-cell spread of vaccinia virus. We confirmed and extended these results while discovering that retrograde trafficking was required for virus egress rather than entry. Retro-2, a specific retrograde trafficking inhibitor of protein toxins, potently prevented spread of vaccinia virus as well as monkeypox virus, a human pathogen. Electron and confocal microscopy studies revealed that Retro-2 prevented wrapping of virions with an additional double-membrane envelope that enables microtubular transport, exocytosis, and actin polymerization. The viral B5 and F13 protein components of this membrane, which are required for wrapping, normally colocalize in the trans -Golgi network. However, only B5 traffics through the secretory pathway, suggesting that F13 uses another route to the trans -Golgi network. The retrograde route was demonstrated by finding that F13 was largely confined to early endosomes and failed to colocalize with B5 in the presence of Retro-2. Thus, vaccinia virus makes novel use of the retrograde transport system for formation of the viral wrapping membrane. IMPORTANCE Efficient cell-to-cell spread of vaccinia virus and other orthopoxviruses depends on the wrapping of infectious particles with a double membrane that enables microtubular transport, exocytosis, and actin polymerization. Interference with wrapping or subsequent steps results in severe attenuation of the virus. Some previous studies had suggested that the wrapping membrane arises from the trans -Golgi network, whereas others suggested an origin from early endosomes. Some nonenveloped viruses use retrograde trafficking for entry into the cell. In contrast, we provided evidence that retrograde transport from early endosomes to the trans -Golgi network is required for the membrane-wrapping step in morphogenesis of vaccinia virus and egress from the cell. The potent in vitro inhibition of this step by the drug Retro-2 suggests that derivatives with enhanced pharmacological properties might serve as useful antipoxviral agents.

Published

2016

5. Human Papillomavirus 16 Capsids Mediate Nuclear Entry during Infection

Author

Day, Patricia M., primary, Weisberg, Andrea S., additional, Thompson, Cynthia D., additional, Hughes, Michelle M., additional, Pang, Yuk Ying, additional, Lowy, Douglas R., additional, and Schiller, John T., additional

Published

2019

6. Identification of Vaccinia Virus Replisome and Transcriptome Proteins by Isolation of Proteins on Nascent DNA Coupled with Mass Spectrometry

Author

Bernard Moss, George C. Katsafanas, Andrea S. Weisberg, Tatiana G. Senkevich, and Lisa R. Olano

Subjects

0301 basic medicine, Proteome, Transcription, Genetic, viruses, Immunology, Vaccinia virus, Biology, Virus Replication, Microbiology, Mass Spectrometry, Cell Line, 03 medical and health sciences, chemistry.chemical_compound, Antigens, Neoplasm, Proliferating Cell Nuclear Antigen, Virology, Chlorocebus aethiops, Animals, Humans, Telomere-binding protein, chemistry.chemical_classification, DNA ligase, Staining and Labeling, 030102 biochemistry & molecular biology, Gene Expression Profiling, Topoisomerase, DNA replication, DNA-Directed RNA Polymerases, Deoxyuridine, Molecular biology, Genome Replication and Regulation of Viral Gene Expression, Nuclear DNA, Proliferating cell nuclear antigen, DNA-Binding Proteins, DNA Topoisomerases, Type II, 030104 developmental biology, chemistry, A549 Cells, Insect Science, DNA, Viral, biology.protein, Replisome, Click Chemistry, Transcriptome, DNA

Abstract

Poxviruses replicate within the cytoplasm and encode proteins for DNA and mRNA synthesis. To investigate poxvirus replication and transcription from a new perspective, we incorporated 5-ethynyl-2′-deoxyuridine (EdU) into nascent DNA in cells infected with vaccinia virus (VACV). The EdU-labeled DNA was conjugated to fluor- or biotin-azide and visualized by confocal, superresolution, and transmission electron microscopy. Nuclear labeling decreased dramatically after infection, accompanied by intense labeling of cytoplasmic foci. The nascent DNA colocalized with the VACV single-stranded DNA binding protein I3 in multiple puncta throughout the interior of factories, which were surrounded by endoplasmic reticulum. Complexes containing EdU-biotin-labeled DNA cross-linked to proteins were captured on streptavidin beads. After elution and proteolysis, the peptides were analyzed by mass spectrometry to identify proteins associated with nascent DNA. The known viral replication proteins, a telomere binding protein, and a protein kinase were associated with nascent DNA, as were the DNA-dependent RNA polymerase and intermediate- and late-stage transcription initiation and elongation factors, plus the capping and methylating enzymes. These results suggested that the replicating pool of DNA is transcribed and that few if any additional viral proteins directly engaged in replication and transcription remain to be discovered. Among the host proteins identified by mass spectrometry, topoisomerases IIα and IIβ and PCNA were noteworthy. The association of the topoisomerases with nascent DNA was dependent on expression of the viral DNA ligase, in accord with previous proteomic studies. Further investigations are needed to determine possible roles for PCNA and other host proteins detected. IMPORTANCE Poxviruses, unlike many well-characterized animal DNA viruses, replicate entirely within the cytoplasm of animal cells, raising questions regarding the relative roles of viral and host proteins. We adapted newly developed procedures for click chemistry and iPOND ( I solation of p roteins o n n ascent D NA) to investigate vaccinia virus (VACV), the prototype poxvirus. Nuclear DNA synthesis ceased almost immediately following VACV infection, followed swiftly by the synthesis of viral DNA within discrete cytoplasmic foci. All viral proteins known from genetic and proteomic studies to be required for poxvirus DNA replication were identified in the complexes containing nascent DNA. The additional detection of the viral DNA-dependent RNA polymerase and intermediate and late transcription factors provided evidence for a temporal coupling of replication and transcription. Further studies are needed to assess the potential roles of host proteins, including topoisomerases IIα and IIβ and PCNA, which were found associated with nascent DNA.

Published

2017

7. Deletion of the Vaccinia Virus I2 Protein Interrupts Virion Morphogenesis, Leading to Retention of the Scaffold Protein and Mislocalization of Membrane-Associated Entry Proteins

Author

Bernard Moss, Seong-In Hyun, and Andrea S. Weisberg

Subjects

0301 basic medicine, Scaffold protein, viruses, Immunology, Mutant, Morphogenesis, Vaccinia virus, Biology, Microbiology, Virus, Cell Line, 03 medical and health sciences, chemistry.chemical_compound, Virology, Humans, Viral Structural Proteins, Virus Assembly, Structure and Assembly, Molecular biology, Transmembrane protein, Transmembrane domain, 030104 developmental biology, chemistry, Membrane protein, Insect Science, Vaccinia, Gene Deletion

Abstract

The I2L open reading frame of vaccinia virus (VACV) encodes a conserved 72-amino-acid protein with a putative C-terminal transmembrane domain. Previous studies with a tetracycline-inducible mutant demonstrated that I2-deficient virions are defective in cell entry. The purpose of the present study was to determine the step of replication or entry that is affected by loss of the I2 protein. Fluorescence microscopy experiments showed that I2 colocalized with a major membrane protein of immature and mature virions. We generated a cell line that constitutively expressed I2 and allowed construction of the VACV I2L deletion mutant vΔI2. As anticipated, vΔI2 was unable to replicate in cells that did not express I2. Unexpectedly, morphogenesis was interrupted at a stage after immature virion formation, resulting in the accumulation of dense spherical particles instead of brick-shaped mature virions with well-defined core structures. The abnormal particles retained the D13 scaffold protein of immature virions, were severely deficient in the transmembrane proteins that comprise the entry fusion complex (EFC), and had increased amounts of unprocessed membrane and core proteins. Total lysates of cells infected with vΔI2 also had diminished EFC proteins due to instability attributed to their hydrophobicity and failure to be inserted into viral membranes. A similar instability of EFC proteins had previously been found with unrelated mutants blocked earlier in morphogenesis that also accumulated viral membranes retaining the D13 scaffold. We concluded that I2 is required for virion morphogenesis, release of the D13 scaffold, and the association of EFC proteins with viral membranes. IMPORTANCE Poxviruses comprise a large family that infect vertebrates and invertebrates, cause disease in both in humans and in wild and domesticated animals, and are being engineered as vectors for vaccines and cancer therapy. In addition, investigations of poxviruses have provided insights into many aspects of cell biology. The I2 protein is conserved in all poxviruses that infect vertebrates, suggesting an important role. The present study revealed that this protein is essential for vaccinia virus morphogenesis and that its absence results in an accumulation of deformed virus particles retaining the scaffold protein and deficient in surface proteins needed for cell entry.

Published

2017

8. Analysis of Viral Membranes Formed in Cells Infected by a Vaccinia Virus L2-Deletion Mutant Suggests Their Origin from the Endoplasmic Reticulum

Author

Bernard Moss, Andrea S. Weisberg, Liliana Maruri-Avidal, and Himani Bisht

Subjects

Immunology, Vaccinia virus, Biology, Endoplasmic Reticulum, Microbiology, Cell Line, Viral Matrix Proteins, Cell membrane, Viral entry, Virology, medicine, Viral structural protein, Humans, Viroplasm, Sequence Deletion, Viral matrix protein, Virus Assembly, Endoplasmic reticulum, Cell Membrane, Viral membrane, Molecular biology, Virus-Cell Interactions, Cell biology, medicine.anatomical_structure, Insect Science, Membrane biogenesis

Abstract

Assembly of the poxvirus immature virion (IV) membrane is a poorly understood event that occurs within the cytoplasm. At least eight viral proteins participate in formation of the viral membrane. Of these, A14, A17, and D13 are structural components whereas A6, A11, F10, H7, and L2 participate in membrane biogenesis. L2, the object of this study, is conserved in all chordopoxviruses, expressed early in infection, and associated with the endoplasmic reticulum (ER) throughout the cell and at the edges of crescent-shaped IV precursors. Previous studies with an inducible L2 mutant revealed abortive formation of the crescent membrane. However, possible low-level L2 synthesis under nonpermissive conditions led to ambiguity in interpretation. Here, we constructed a cell line that expresses L2, which allowed the creation of an L2-deletion mutant. In noncomplementing cells, replication was aborted prior to formation of mature virions and two types of aberrant structures were recognized. One consisted of short crescents, at the surface of dense masses of viroplasm, which were labeled with antibodies to the A11, A14, A17, and D13 proteins. The other structure consisted of “empty” IV-like membranes, also labeled with antibodies to the viral proteins, which appeared to be derived from adjacent calnexin-containing ER. A subset of 25 proteins examined, exemplified by components of the entry-fusion complex, were greatly diminished in amount. The primary role of L2 may be to recruit ER and modulate its transformation to viral membranes in juxtaposition with the viroplasm, simultaneously preventing the degradation of viral proteins dependent on viral membranes for stability.

Published

2013

9. Participation of Vaccinia Virus L2 Protein in the Formation of Crescent Membranes and Immature Virions

Author

Andrea S. Weisberg, Bernard Moss, Liliana Maruri-Avidal, and Arban Domi

Subjects

Genes, Viral, Molecular Sequence Data, Immunology, Mutant, Vaccinia virus, Viral Plaque Assay, Biology, Microbiology, Virus, Cell Line, Viral Proteins, Microscopy, Electron, Transmission, Virology, Humans, Viroplasm, Poxviridae, Amino Acid Sequence, Orthopoxvirus, Genes, Essential, Structure and Assembly, Virus Assembly, Virion, Virion membrane, Viral membrane, biology.organism_classification, Molecular biology, Cytoplasm, Insect Science, Sequence Alignment, Gene Deletion

Abstract

Morphogenesis of vaccinia virus begins with the appearance of crescent-shaped membrane precursors of immature virions in cytoplasmic factories. During the initial characterization of the product of the L2R reading frame, we discovered that it plays an important role in crescent formation. The L2 protein was expressed early in infection and was associated with the detergent-soluble membrane fraction of mature virions, consistent with two potential membrane-spanning domains. All chordopoxviruses have L2 homologs, suggesting an important function. Indeed, we were unable to isolate an infectious L2R deletion mutant. Consequently, we constructed an inducible mutant with a conditional lethal phenotype. When L2 expression was repressed, proteolytic processing of the major core proteins and the A17 protein, which is an essential component of the immature virion membrane, failed to occur, suggesting an early block in viral morphogenesis. At 8 h after infection in the presence of inducer, immature and mature virions were abundantly seen by electron microscopy. In contrast, those structures were rare in the absence of inducer and were replaced by large, dense aggregates of viroplasm. A minority of these aggregates had short spicule-coated membranes, which resembled the beginnings of crescent formation, at their periphery. These short membrane segments at the edge of the dense viroplasm increased in number at later times, and some immature virions were seen. Although the L2 protein was not detected under nonpermissive conditions, minute amounts could account for stunted and delayed viral membrane formation. These findings suggested that L2 is required for the formation or elongation of crescent membranes.

Published

2011

10. Congregation of Orthopoxvirus Virions in Cytoplasmic A-Type Inclusions Is Mediated by Interactions of a Bridging Protein (A26p) with a Matrix Protein (ATIp) and a Virion Membrane-Associated Protein (A27p)

Author

Amanda R. Howard, Bernard Moss, and Andrea S. Weisberg

Subjects

Cytoplasmic inclusion, viruses, Immunology, Vaccinia virus, medicine.disease_cause, Microbiology, Cell Line, Inclusion Bodies, Viral, Viral Proteins, Virology, Chlorocebus aethiops, Protein Interaction Mapping, medicine, Animals, Humans, Poxviridae, Orthopoxvirus, Viral matrix protein, biology, Structure and Assembly, Virus Assembly, Cowpox virus, Virion membrane, Membrane Proteins, virus diseases, biology.organism_classification, Cell biology, Virion assembly, Insect Science, Raccoonpox virus, Carrier Proteins, Viral Fusion Proteins, Protein Binding

Abstract

Some orthopoxviruses, e.g., the cowpox, ectromelia, and raccoonpox viruses, form large, discrete cytoplasmic inclusions within which mature virions (MVs) are embedded by a process called occlusion. These inclusions, which may protect occluded MVs in the environment, are composed of aggregates of the A-type inclusion protein (ATIp), which is truncated in orthopoxviruses such as vaccinia virus (VACV) and variola virus that fail to form inclusions. In addition to an intact ATIp, occlusion requires the A26 protein (A26p). Although VACV contains a functional A26p, determined by complementation of a cowpox virus occlusion-defective mutant, its role in occlusion was unknown. We found that restoration of the full-length ATI gene was sufficient for VACV inclusion formation and the ensuing occlusion of MVs. A26p was present in inclusions even when virion assembly was inhibited, suggesting a direct interaction of A26p with ATIp. Analysis of a panel of ATIp mutants indicated that the C-terminal repeat region was required for inclusion formation and the N-terminal domain for interaction with A26p and occlusion. A26p is tethered to MVs via interaction with the A27 protein (A27p); A27p was not required for association of A26p with ATIp but was necessary for occlusion. In addition, the C-terminal domain of A26p, which mediates A26p-A27p interactions, was necessary but insufficient for occlusion. Taken together, the data suggest a model for occlusion in which A26p has a bridging role between ATIp and A27p, and A27p provides a link to the MV membrane.

Published

2010

11. Vaccinia Virus L1 Protein Is Required for Cell Entry and Membrane Fusion

Author

Himani Bisht, Bernard Moss, and Andrea S. Weisberg

Subjects

Indoles, Genes, Viral, viruses, Green Fluorescent Proteins, Immunology, Vaccinia virus, Virus Replication, Membrane Fusion, Microbiology, Virus, Cell Fusion, chemistry.chemical_compound, Viral entry, Virology, Humans, Poxviridae, Orthopoxvirus, Fluorescent Antibody Technique, Indirect, Fluorescent Dyes, Cell fusion, biology, Viral Core Proteins, Virion, Virion membrane, Membrane Proteins, Hydrogen-Ion Concentration, biology.organism_classification, Virus-Cell Interactions, DNA-Binding Proteins, Viral replication, chemistry, Insect Science, Mutation, Vaccinia, HeLa Cells

Abstract

Genetic and biochemical studies have provided evidence for an entry/fusion complex (EFC) comprised of at least eight viral proteins (A16, A21, A28, G3, G9, H2, J5, and L5) that together with an associated protein (F9) participates in entry of vaccinia virus (VACV) into cells. The genes encoding these proteins are conserved in all poxviruses, are expressed late in infection, and are components of the mature virion membrane but are not required for viral morphogenesis. In addition, all but one component has intramolecular disulfides that are formed by the poxvirus cytoplasmic redox system. The L1 protein has each of the characteristics enumerated above except that it has been reported to be essential for virus assembly. To further investigate the role of L1, we constructed a recombinant VACV (vL1Ri) that inducibly expresses L1. In the absence of inducer, L1 synthesis was repressed and vL1Ri was unable to form plaques or produce infectious progeny. Unexpectedly, assembly and morphogenesis appeared normal and the noninfectious virus particles were indistinguishable from wild-type VACV as determined by transmission electron microscopy and analysis of the component polypeptides. Notably, the L1-deficient virions were able to attach to cells but the cores failed to penetrate into the cytoplasm. In addition, cells infected with vL1Ri in the absence of inducer did not form syncytia following brief low-pH treatment even though extracellular virus was produced. Coimmunoprecipitation experiments demonstrated that L1 interacted with the EFC and indirectly with F9, suggesting that L1 is an additional component of the viral entry apparatus.

Published

2008

12. Vaccinia Virus E2L Null Mutants Exhibit a Major Reduction in Extracellular Virion Formation and Virus Spread

Author

Bernard Moss, Andrea S. Weisberg, and Arban Domi

Subjects

DNA Replication, viruses, Immunology, Mutant, Vaccinia virus, Biology, Virus Replication, Microbiology, Virus, Cell Line, chemistry.chemical_compound, Viral Envelope Proteins, Virology, Chlorocebus aethiops, Extracellular, Animals, Poxviridae, Orthopoxvirus, Gene, Structure and Assembly, Virion, biology.organism_classification, Molecular biology, Viral replication, chemistry, Insect Science, DNA, Viral, Mutation, Vaccinia

Abstract

The vaccinia virus E2L (VACWR058) gene is conserved in all sequenced chordopoxviruses and is predicted to encode an 86-kDa protein with no recognizable functional motifs or nonpoxvirus homologs. Although the region immediately upstream of the open reading frame lacked optimal consensus promoter motifs, expression of the E2 protein occurred after viral DNA replication. Transfection studies, however, indicated that the promoter was weak compared to well-characterized intermediate and late promoters. The E2 protein was present in mature virions purified from infected cells but was more abundant in extracellular enveloped forms. Despite the conservation of the E2L gene in chordopoxviruses, deletion mutants could be isolated from both the WR and IHD-J strains of vaccinia virus. These null mutants produced very small plaques in all cell lines tested, reduced amounts of mature infectious virions, and very low numbers of extracellular virions. Nevertheless, viral protein synthesis appeared qualitatively and quantitatively normal. The defect in extracellular virus formation was corroborated by electron microscopy, which also showed some aberration in the wrapping of virions by cisternal membranes. Extracellular virions that did form, however, were able to induce actin tail formation.

Published

2008

13. Identification of Vaccinia Virus Replisome and Transcriptome Proteins by Isolation of Proteins on Nascent DNA Coupled with Mass Spectrometry

Author

Senkevich, Tatiana G., primary, Katsafanas, George C., additional, Weisberg, Andrea, additional, Olano, Lisa R., additional, and Moss, Bernard, additional

Published

2017

14. Deletion of the Vaccinia Virus I2 Protein Interrupts Virion Morphogenesis, Leading to Retention of the Scaffold Protein and Mislocalization of Membrane-Associated Entry Proteins

Author

Hyun, Seong-In, primary, Weisberg, Andrea, additional, and Moss, Bernard, additional

Published

2017

15. Sequence-Independent Targeting of Transmembrane Proteins Synthesized within Vaccinia Virus Factories to Nascent Viral Membranes

Author

Bernard Moss, Matloob Husain, and Andrea S. Weisberg

Subjects

Models, Molecular, Indoles, Viral protein, viruses, Molecular Sequence Data, Immunology, Vaccinia virus, Biology, medicine.disease_cause, Microbiology, Viral Matrix Proteins, Virology, Viral structural protein, medicine, Humans, Immunoprecipitation, Amino Acid Sequence, Fluorescent Antibody Technique, Indirect, Microscopy, Immunoelectron, Integral membrane protein, Fluorescent Dyes, Microscopy, Confocal, Viral matrix protein, Virion, Membrane Proteins, STIM1, Viral membrane, Transmembrane protein, Virus-Cell Interactions, Transmembrane domain, Biochemistry, Insect Science, HeLa Cells

Abstract

The primary membrane of vaccinia virus, as well as those of other poxviruses, forms within a discrete cytoplasmic factory region. We recently determined the existence of an operative pathway from the endoplasmic reticulum within the virus factory to nascent viral membranes and demonstrated that a viral protein could be diverted from this pathway to Golgi membranes by the addition of COPII-binding sites (M. Husain, A. S. Weisberg, and B. Moss, Proc. Natl. Acad. Sci. USA, 103: 19506-19511, 2006). Here we describe an investigation of the structural features that are required for transit of proteins to the viral membrane. Deletion of either the N-terminal domain or the C-terminal cytoplasmic tail from the conserved A9 protein did not prevent its incorporation into viral membranes, whereas deletion of the transmembrane domain resulted in its distribution throughout the cytoplasm. Nevertheless, replacement of the A9 transmembrane domain with the corresponding region of a nonpoxvirus transmembrane protein or of a vaccinia virus extracellular envelope protein allowed viral membrane targeting, indicating no requirement for a specific amino acid sequence. Remarkably, the epitope-tagged A9 transmembrane domain alone, as well as a heterologous transmembrane domain lacking a poxvirus sequence, was sufficient for viral membrane association. The data are consistent with a sequence-independent pathway in which transmembrane proteins that are synthesized within the virus factory and lack COPII or other binding sites that enable conventional endoplasmic reticulum exiting are incorporated into nascent viral membranes.

Published

2007

16. Human papillomavirus type 16 (HPV16) capsids mediate nuclear entry during infection.

Author

Day, Patricia M., Weisberg, Andrea S., Thompson, Cynthia D., Hughes, Michelle M., Yuk Ying Pang, Lowy, Douglas R., and Schiller, John T.

Subjects

*CAPSIDS, *ELECTRON microscopy, *INFECTION, *CHROMOSOMES

Abstract

Infectious HPV16 L1/L2 pseudovirions were found to remain largely intact during vesicular transport to the nucleus. By electron microscopy, capsids with a diameter of 50 nm were clearly visible within small vesicles attached to mitotic chromosomes and to a lesser extent within interphase nuclei, implying nuclear disassembly. By confocal analysis, it was determined that nuclear entry of assembled L1 is dependent upon the presence of the minor capsid protein, L2, but independent of encapsidated DNA. We also demonstrate that L1 nuclear localization and mitotic chromosome association can occur in vivo in the murine cervicovaginal challenge model of HPV16 infection. These findings challenge the prevailing concepts of PV uncoating and disassembly. More generally, they document that a largely intact viral capsid can enter the nucleus within a transport vesicle, establishing a novel mechanism by which a virus accesses the nuclear cellular machinery. [ABSTRACT FROM AUTHOR]

Published

2019

17. Vaccinia Virus Nonstructural Protein Encoded by the A11R Gene Is Required for Formation of the Virion Membrane

Author

Bernard Moss, Andrea S. Weisberg, and Wolfgang Resch

Subjects

Gene Expression Regulation, Viral, Vesicle-associated membrane protein 8, viruses, Immunology, Vaccinia virus, Protein Serine-Threonine Kinases, Viral Nonstructural Proteins, Biology, Virus Replication, Microbiology, Virus, Cell Line, Open Reading Frames, Viral Proteins, VP40, Virology, Viral factory, Viral structural protein, Animals, Humans, Orthopoxvirus, Phosphorylation, Base Sequence, Structure and Assembly, Virus Assembly, Gene Expression Regulation, Developmental, Viral membrane, biology.organism_classification, Molecular biology, Molecular Weight, Microscopy, Electron, Viral replication, Insect Science, DNA, Viral, Protein Processing, Post-Translational, HeLa Cells

Abstract

The vaccinia virus A11R gene has orthologs in all known poxvirus genomes, and the A11 protein has been previously reported to interact with the putative DNA packaging protein A32 in a yeast two-hybrid screen. Using antisera raised against A11 peptides, we show that the A11 protein was (i) expressed at late times with an apparent mass of 40 kDa, (ii) not incorporated into virus particles, (iii) phosphorylated independently of the viral F10 kinase, (iv) coimmunoprecipitated with A32, and (v) localized to the viral factory. To determine the role of the A11 protein and test whether it is indeed involved in DNA packaging, we constructed a recombinant vaccinia virus with an inducible A11R gene. This recombinant was dependent on inducer for single-cycle growth and plaque formation. In the absence of inducer, viral late proteins were produced at normal levels, but proteolytic processing and other posttranslational modifications of some proteins were inhibited, suggesting a block in virus particle assembly. Consistent with this observation, electron microscopy of cells infected in the absence of inducer showed virus factories with abnormal electron-dense viroplasms and intermediate density regions associated with membranes and containing the D13 protein. However, no viral membrane crescents, immature virions, or mature virions were produced. The requirement for nonvirion protein A11 in order to make normal viral membranes was an unexpected and exciting finding, since neither the origin of these membranes nor their mechanism of formation in the cytoplasm of infected cells is understood.

Published

2005

18. Vaccinia Virus Mutants with Alanine Substitutions in the Conserved G5R Gene Fail To Initiate Morphogenesis at the Nonpermissive Temperature

Author

Flávio Guimarães da Fonseca, Bernard Moss, M.F. Caeiro, and Andrea S. Weisberg

Subjects

DNA Replication, Cytoplasm, Genes, Viral, Transcription, Genetic, viruses, Molecular Sequence Data, Immunology, Mutant, Replication, Vaccinia virus, Viral Plaque Assay, Protein Serine-Threonine Kinases, Biology, Microbiology, Virus, Cell Line, Conserved sequence, Open Reading Frames, Viral Proteins, chemistry.chemical_compound, Viral Envelope Proteins, Virology, Morphogenesis, Humans, Amino Acid Sequence, Orthopoxvirus, Gene, Conserved Sequence, Genes, Essential, Viral Core Proteins, Virus Assembly, Temperature, DNA replication, Membrane Proteins, Viral membrane, biology.organism_classification, Molecular biology, DNA-Binding Proteins, Amino Acid Substitution, chemistry, Protein Biosynthesis, Insect Science, DNA, Viral, Mutation, Vaccinia, Protein Processing, Post-Translational

Abstract

The initial characterization of the product of the vaccinia virus G5R gene, which is conserved in all poxviruses sequenced to date, is described. The G5 protein was detected in the core fraction of purified virions, and transcription and translation of the G5R open reading frame occurred early in infection, independently of DNA replication. Attempts to delete the G5R gene and isolate a replication-competent virus were unsuccessful, suggesting that G5R encodes an essential function. We engineered vaccinia virus mutants with clusters of charged amino acids changed to alanines and determined that several were unable to replicate at 40°C but grew well at 37°C. At the nonpermissive temperature, viral gene expression and DNA replication and processing were unperturbed. However, tyrosine phosphorylation and proteolytic cleavage of the A17 membrane protein and proteolytic cleavage of core proteins were inhibited at 40°C, suggesting an assembly defect. The cytoplasm of cells that had been infected at the nonpermissive temperature contained large granular areas devoid of cellular organelles or virus structures except for occasional short crescent-shaped membranes and electron-dense lacy structures. The temperature-sensitive phenotype of the G5R mutants closely resembled the phenotypes of vaccinia virus mutants carrying conditionally lethal F10R protein kinase and H5R mutations. F10, although required for phosphorylation of A17 and viral membrane formation, was synthesized by the G5R mutants under nonpermissive conditions. An intriguing possibility is that G5 participates in the formation of viral membranes, a poorly understood event in poxvirus assembly.

Published

2004

19. Evidence for an Essential Catalytic Role of the F10 Protein Kinase in Vaccinia Virus Morphogenesis

Author

Andrea S. Weisberg, Patricia Szajner, and Bernard Moss

Subjects

Gene Expression Regulation, Viral, Isopropyl Thiogalactoside, Immunology, Vaccinia virus, Protein Serine-Threonine Kinases, Biology, Virus Replication, Microbiology, Catalysis, Virus, Cell Line, Viral Proteins, Virology, Morphogenesis, Humans, Inducer, Orthopoxvirus, Protein kinase A, Recombination, Genetic, Kinase, Virus Assembly, Structure and Assembly, Viral membrane, biology.organism_classification, Molecular biology, Viral replication, Insect Science, Mutation, Phosphorylation, HeLa Cells, Plasmids

Abstract

Temperature-sensitive mutants of vaccinia virus, with genetic changes that map to the open reading frame encoding the F10 protein kinase, exhibit a defect at an early stage of viral morphogenesis. To further study the role of the enzyme, we constructed recombinant vaccinia virus vF10V5i, which expresses inducible V5 epitope-tagged F10 and is dependent on a chemical inducer for plaque formation and replication. In the absence of inducer, viral membrane formation was delayed and crescents and occasional immature forms were detected only late in infection. When the temperature was raised from 37 to 39°C, the block in membrane formation persisted throughout the infection. The increased stringency may be explained by a mild temperature sensitivity of the wild-type F10 kinase, which reduced the activity of the very small amount expressed in the absence of inducer, or by the thermolability of an unphosphorylated kinase substrate or uncomplexed F10-interacting protein. Further analyses demonstrated that tyrosine and threonine phosphorylation of the A17 membrane component was inhibited in the absence of inducer. The phosphorylation defect could be overcome by transfection of plasmids that express wild-type F10, but not by plasmids that express F10 with single amino acid substitutions that abolished catalytic activity. Although the mutated forms of F10 were stable and concentrated in viral factories, only the wild-type protein complemented the assembly and replication defects of vF10V5i in the absence of inducer. These studies provide evidence for an essential catalytic role of the F10 kinase in vaccinia virus morphogenesis.

Published

2004

20. Physical and Functional Interactions between Vaccinia Virus F10 Protein Kinase and Virion Assembly Proteins A30 and G7

Author

Patricia Szajner, Andrea S. Weisberg, and Bernard Moss

Subjects

Gene Expression Regulation, Viral, Threonine, Immunoprecipitation, Viral protein, Immunology, Vaccinia virus, Protein Serine-Threonine Kinases, Biology, medicine.disease_cause, Microbiology, Cell Line, Viral Proteins, Viral Envelope Proteins, Virology, medicine, Animals, Humans, Phosphorylation, Microscopy, Immunoelectron, Protein kinase A, Microscopy, Confocal, Kinase, Structure and Assembly, Viral Core Proteins, Virus Assembly, Autophosphorylation, Virion, Precipitin Tests, Molecular biology, Cell biology, Membrane protein, Virion assembly, Insect Science, Tyrosine, Rabbits, HeLa Cells

Abstract

An early step in vaccinia virus morphogenesis, the association of crescent membranes with electron-dense granular material, is perturbed when expression of the viral protein encoded by the A30L or G7L open reading frame is repressed. Under these conditions, we found that phosphorylation of the A17 membrane protein, which is mediated by the F10 kinase, was severely reduced. Furthermore, A30 and G7 stimulated F10-dependent phosphorylation of A17 in the absence of other viral late proteins. Evidence for physical interactions between A30, G7, and F10 was obtained by their coimmunoprecipitation with antibody against A30 or F10. In addition, phosphorylation of A30 was dependent on the F10 kinase and autophosphorylation of F10 was stimulated by A30 and G7. Nevertheless, the association of A30, G7, and F10 occurred even with mutated, catalytically inactive forms of F10. Just as A30 and G7 are mutually dependent on each other for stability, F10 was nearly undetectable in the absence of A30 and G7. The reverse is not true, however, as repression of F10 did not diminish A30 or G7. Interaction of F10 with A30 and G7 presumably occurred within the virus factory areas of the cytoplasm, where each was concentrated. F10 localized predominantly in the cortical region of immature virions, beneath the membrane where A17 is located. F10 remained associated with the particulate core fraction of mature virions after treatment with a nonionic detergent and reducing agent. The formation of protein complexes such as the one involving A30, G7, and F10 may be a mechanism for the regulated packaging and processing of virion components.

Published

2004

21. Mapping and Functional Analysis of Interaction Sites within the Cytoplasmic Domains of the Vaccinia Virus A33R and A36R Envelope Proteins

Author

Andrea S. Weisberg, Brian M. Ward, and Bernard Moss

Subjects

Genes, Viral, Immunology, Mutant, Vaccinia virus, Viral Plaque Assay, Biology, Recombinant virus, Microbiology, Cell Line, Viral Envelope Proteins, Two-Hybrid System Techniques, Virology, Humans, Binding site, Microscopy, Immunoelectron, Gene, Actin, Sequence Deletion, Recombination, Genetic, Viral Structural Proteins, Binding Sites, Membrane Glycoproteins, Microscopy, Confocal, Base Sequence, Structure and Assembly, Molecular biology, Protein Structure, Tertiary, Phenotype, Membrane protein, Cytoplasm, Insect Science, DNA, Viral, Bacterial outer membrane, HeLa Cells

Abstract

Incorporation of the vaccinia virus A36R protein into the outer membrane of intracellular enveloped virions (IEV) is dependent on expression of the A33R protein. Possible interactions of the 200-amino-acid cytoplasmic domain of the A36R protein with itself or with the cytoplasmic domain of the A33R, A34R, B5R, or F12L IEV membrane protein was investigated by using the yeast two-hybrid system. A strong interaction was detected only between the cytoplasmic domains of the A36R and A33R proteins. Upon further analyses, the interaction site was mapped to residues 91 to 111 of the A36R protein. To investigate the role of the A36R:A33R interaction during viral infection, five recombinant vaccinia viruses containing B5R-GFP as a marker were constructed. Four had the full-length A36R gene replaced with various-length C-terminal truncations of A36R, of which two contained residues 91 to 111 and two were missing this region. The fifth recombinant virus had an A33R gene with most of the 40-amino-acid cytoplasmic tail deleted. Residues 91 to 111 of A36R and the cytoplasmic tail of A33R were required for a strong interaction between the two proteins during viral infection and for maximal amounts of A36R protein on IEV. Mutants lacking these regions of A33R or A36R formed IEV that exhibited only short sporadic intracellular movement, displayed no actin tails, and formed small plaques on cell monolayers equivalent to those of an A36R deletion mutant and smaller than those formed by point mutations that specifically abrogate actin tail formation. The A33R interaction site of the A36R protein is highly conserved among orthopoxviruses and may overlap binding sites for cellular proteins needed for microtubular movement and actin tail formation.

Published

2003

22. Isolation of Enzymatically Active Replication Complexes from Feline Calicivirus-Infected Cells

Author

Mark H. Fogg, Craig E. Cameron, Gaël Belliot, Kim Y. Green, Mariam Wagner, Ellie Ehrenfeld, Aaron Mory, Stanislav V. Sosnovtsev, Andrea S. Weisberg, and Tanaji Mitra

Subjects

Viral protein, viruses, Immunology, Replication, Biology, Virus Replication, medicine.disease_cause, Antiviral Agents, Microbiology, Virus, Cell Line, Viral Proteins, Virology, medicine, Animals, Northern blot, Protein Precursors, Caliciviridae Infections, Feline calicivirus, Brefeldin A, Cell Membrane, Membrane Proteins, RNA, biology.organism_classification, Molecular biology, Viral replication, Capsid, Biochemistry, Membrane protein, Insect Science, Cats, RNA, Viral, Calicivirus, Feline

Abstract

A membranous fraction that could synthesize viral RNA in vitro in the presence of magnesium salt, ribonucleotides, and an ATP-regenerating system was isolated from feline calicivirus (FCV)-infected cells. The enzymatically active component of this fraction was designated FCV replication complexes (RCs), by analogy to other positive-strand RNA viruses. The newly synthesized RNA was characterized by Northern blot analysis, which demonstrated the production of both full-length (8.0-kb) and subgenomic-length (2.5-kb) RNA molecules similar to those synthesized in FCV-infected cells. The identity of the viral proteins associated with the fraction was investigated. The 60-kDa VP1 major capsid protein was the most abundant viral protein detected. VP2, a minor structural protein encoded by open reading frame 3 (ORF3), was also present. Nonstructural proteins associated with the fraction included the precursor polypeptides Pro-Pol (76 kDa) and p30-VPg (43 kDa), as well as the mature nonstructural proteins p32 (derived from the N-terminal region of the ORF1 polyprotein), p30 (the putative “3A-like” protein), and p39 (the putative nucleoside triphosphatase). The isolation of enzymatically active RCs containing both viral and cellular proteins should facilitate efforts to dissect the contributions of the virus and the host to FCV RNA replication.

Published

2002

23. Vaccinia Virus A30L Protein Is Required for Association of Viral Membranes with Dense Viroplasm To Form Immature Virions

Author

Elizabeth J. Wolffe, Bernard Moss, Patricia Szajner, and Andrea S. Weisberg

Subjects

Isopropyl Thiogalactoside, Transcription, Genetic, viruses, Immunoelectron microscopy, Immunology, Mutant, Vaccinia virus, Biology, Virus Replication, Microbiology, Virus, chemistry.chemical_compound, Viral Envelope Proteins, Virology, Virus maturation, Humans, Viroplasm, Gene, Virus Assembly, Virion, Molecular biology, Virus-Cell Interactions, Cell biology, chemistry, Viral replication, Insect Science, Vaccinia, HeLa Cells

Abstract

The previously uncharacterized A30L gene of vaccinia virus has orthologs in all vertebrate poxviruses but no recognizable nonpoxvirus homologs or functional motifs. We determined that the A30L gene was regulated by a late promoter and encoded a protein of approximately 9 kDa. Immunoelectron microscopy of infected cells indicated that the A30L protein was associated with viroplasm enclosed by crescent and immature virion membranes. The A30L protein was also present in mature virions and was partially released by treatment with a nonionic detergent and reducing agent, consistent with a location in the matrix between the core and envelope. To determine the role of the A30L protein, we constructed a stringent conditional lethal mutant with an inducible A30L gene. In the absence of inducer, synthesis of viral early and late proteins occurred but the proteolytic processing of certain core proteins was inhibited, suggesting an assembly block. Inhibition of virus maturation was confirmed by electron microscopy. Under nonpermissive conditions, we observed aberrant large, dense, granular masses of viroplasm with clearly defined margins; viral crescent membranes that appeared normal except for their location at a distance from viroplasm; empty immature virions; and an absence of mature virions. The data indicated that the A30L protein is needed for vaccinia virus morphogenesis, specifically the association of the dense viroplasm with viral membranes.

Published

2001

24. A Glutaredoxin, Encoded by the G4L Gene of Vaccinia Virus, Is Essential for Virion Morphogenesis

Author

Christine L. White, Bernard Moss, and Andrea S. Weisberg

Subjects

Gene Expression Regulation, Viral, Genes, Viral, viruses, Immunology, Mutant, Vaccinia virus, Biology, Virus Replication, Recombinant virus, Microbiology, Virus, Late protein, chemistry.chemical_compound, Virology, Glutaredoxin, Gene, Glutaredoxins, Structure and Assembly, Virion, Proteins, Molecular biology, Microscopy, Electron, Viral replication, chemistry, Insect Science, Vaccinia, Oxidoreductases

Abstract

Vaccinia virus encodes two glutaredoxins, O2L and G4L, both of which exhibit thioltransferase and dehydroascorbate reductase activities in vitro. Although O2L was previously found to be dispensable for virus replication, we now show that G4L is necessary for virion morphogenesis. RNase protection and Western blotting assays indicated that G4L was expressed at late times after infection and was incorporated into mature virus particles. Attempts to isolate a mutant virus with a deleted G4L gene were unsuccessful, suggesting that the protein was required for virus replication. This interpretation was confirmed by the construction and characterization of a conditional lethal recombinant virus with an inducible copy of the G4L gene replacing the original one. Expression of G4L was proportional to the concentration of inducer, and the amount of glutaredoxin could be varied from barely detectable to greater than normal amounts of protein. Immunogold labeling revealed that the induced G4L protein was associated with immature and mature virions and adjacent cytoplasmic depots. In the absence of inducer, the production of infectious virus was severely inhibited, though viral late protein synthesis appeared unaffected except for decreased maturation-dependent proteolytic processing of certain core components. Electron microscopy of cells infected under nonpermissive conditions revealed an accumulation of crescent membranes on the periphery of electron-dense globular masses but few mature particles. We concluded that the two glutaredoxin homologs encoded by vaccinia virus have different functions and that G4L has a role in virion morphogenesis, perhaps by acting as a redox protein.

Published

2000

25. Effects of Deletion or Stringent Repression of the H3L Envelope Gene on Vaccinia Virus Replication

Author

Elizabeth J. Wolffe, Andrea S. Weisberg, Flávio Guimarães da Fonseca, and Bernard Moss

Subjects

Endosome, viruses, Immunology, Vaccinia virus, Viral Plaque Assay, Biology, Virus Replication, Giant Cells, Microbiology, Virus, Cell Line, chemistry.chemical_compound, Viral Envelope Proteins, Virology, Viral factory, Extracellular, Animals, Humans, Viral Structural Proteins, Virus Assembly, Structure and Assembly, Virion, Hydrogen-Ion Concentration, Molecular biology, Microscopy, Electron, Phenotype, Membrane, chemistry, Viral replication, Cytoplasm, Insect Science, Vaccinia, Carrier Proteins, Gene Deletion, HeLa Cells

Abstract

Poxviruses are the largest and most complex of all animal viruses. The first visible step in the assembly of vaccinia virus, the prototype poxvirus, is the formation of crescent membranes within viral factory areas of the cytoplasm (8). The crescents enclose electron-dense material to become spherical immature virions (IV) that progress into infectious intracellular mature virions (IMV). Some IMV are then wrapped by a double layer of membranes, derived from the trans-Golgi or endosomal cisternae, and migrate to the periphery of the cell where the outermost viral and plasma membranes may fuse (15, 17, 21, 35, 38). Virus spread is mediated largely by extracellular particles, which have one more membrane than the IMV, and are called cell-associated extracellular enveloped virions (CEV) if they remain adherent and extracellular enveloped virions (EEV) if they are detached from the cell surface (2, 4, 5, 24). Vaccinia virus mutants provide powerful tools for analyzing the sequential steps in membrane formation and morphogenesis. For example, studies with mutants indicated that (i) the F10L protein kinase is required for formation of the first viral membranes (39, 43); (ii) small vesicles that may be precursors of the viral membranes accumulate in the absence of A17L and A14L expression (28, 29, 40, 47); (iii) D13L expression is needed for coating the viral membranes to form crescents (50); (iv) IV accumulate when expression of L1R is blocked (25); (v) IMV remain largely unwrapped by cisternae when A27R (27), F13L (3), and B5R (12, 45) are not expressed; and (vi) actin tail formation is dependent on synthesis of proteins encoded by A33R, A34R, and A36R genes (30, 33, 46, 49). We recently initiated investigations of the role of the H3L protein, an immunodominant component of IMV membranes (18, 37, 51), and presented evidence that it is anchored to the surfaces of IMV by a C-terminal hydrophobic tail that can mediate posttranslational membrane insertion (7). As a continuation of that study we constructed two vaccinia virus mutants, one with the H3L open reading frame (ORF) deleted and the other with the H3L ORF stringently repressed, and found that immature viral forms accumulated, with a corresponding reduction in infectious virions, under conditions in which H3L was not expressed.

Published

2000

26. Retrograde Transport from Early Endosomes to the trans -Golgi Network Enables Membrane Wrapping and Egress of Vaccinia Virus Virions

Author

Sivan, Gilad, primary, Weisberg, Andrea S., additional, Americo, Jeffrey L., additional, and Moss, Bernard, additional

Published

2016

27. The Envelope Protein Encoded by the A33R Gene Is Required for Formation of Actin-Containing Microvilli and Efficient Cell-to-Cell Spread of Vaccinia Virus

Author

Bernard Moss, Elizabeth J. Wolffe, Andrea S. Weisberg, and Rachel L. Roper

Subjects

Intracellular Fluid, Genes, Viral, Immunology, Mutant, Fluorescent Antibody Technique, Gene Expression, Vaccinia virus, Viral Plaque Assay, Biology, Microbiology, Virus, Viral Envelope Proteins, Viral envelope, Virology, Animal Viruses, Gene expression, Centrifugation, Density Gradient, Extracellular, Humans, Cloning, Molecular, Gene, Actin, Glycoproteins, Microvilli, Virion, Actin cytoskeleton, Molecular biology, Actins, Culture Media, Actin Cytoskeleton, Phenotype, Mutagenesis, Insect Science, Gene Deletion, HeLa Cells

Abstract

The vaccinia virus (VV) A33R gene encodes a highly conserved 23- to 28-kDa glycoprotein that is specifically incorporated into the viral outer envelope. The protein is expressed early and late after infection, consistent with putative early and late promoter sequences. To determine the role of the protein, two inducible A33R mutants were constructed, one with the late promoter and one with the early and late A33R promoter elements. Decreased A33R expression was associated with small plaques that formed comets in liquid medium. Using both an antibiotic resistance gene and a color marker, an A33R deletion mutant, vA33Δ, was isolated, indicating that the A33R gene is not essential for VV replication. The plaques formed by vA33Δ, however, were tiny, indicating that the A33R protein is necessary for efficient cell-to-cell spread. Rescue of the large-plaque phenotype was achieved by inserting a new copy of the A33R gene into the thymidine kinase locus, confirming the specific genetic basis of the phenotype. Although there was a reduction in intracellular virus formed in cells infected with vA33Δ, the amount of infectious virus in the medium was increased. The virus particles in the medium had the buoyant density of extracellular enveloped viruses (EEV). Additionally, amounts of vA33Δ cell-associated extracellular enveloped viruses (CEV) were found to be normal. Immunogold electron microscopy of cells infected with vA33Δ demonstrated the presence of the expected F13L and B5R proteins in wrapping membranes and EEV; however, fully wrapped vA33Δ intracellular enveloped viruses (IEV) were rare compared to partially wrapped particles. Specialized actin tails that propel IEV particles to the periphery and virus-tipped microvilli (both common in wild-type-infected cells) were absent in cells infected with vA33Δ. This is the first deletion mutant in a VV envelope gene that produces at least normal amounts of fully infectious EEV and CEV and yet has a small-plaque phenotype. These data support a new model for VV spread, emphasizing the importance of virus-tipped actin tails.

Published

1998

28. Repression of the A8L Gene, Encoding the Early Transcription Factor 82-Kilodalton Subunit, Inhibits Morphogenesis of Vaccinia Virions

Author

Xiaolei Hu, Lawrence J. Carroll, Bernard Moss, Andrea S. Weisberg, and Elizabeth J. Wolffe

Subjects

Gene Expression Regulation, Viral, Isopropyl Thiogalactoside, RFC5, Genes, Viral, Protein Conformation, Protein subunit, Immunology, Vaccinia virus, Biology, medicine.disease_cause, Microbiology, Virus, Cell Line, Late protein, Viral Proteins, Virology, Animal Viruses, Escherichia coli, medicine, Animals, Humans, Inducer, Gene, DNA Primers, Recombination, Genetic, Mutation, Microscopy, Confocal, Base Sequence, Molecular biology, DNA-Binding Proteins, Molecular Weight, Microscopy, Electron, Lac Operon, Viral replication, Insect Science, DNA, Viral, HeLa Cells, Transcription Factors

Abstract

The vaccinia virus early transcription factor (VETF) is a DNA binding protein comprised of 70- and 82-kDa subunits encoded by the D6R and A8L genes, respectively. A previous investigation suggested a novel role for the 70-kDa subunit in the morphogenesis of vaccinia virus particles. The principal objectives of the present study were to determine if the 82-kDa subunit of VETF is also required for morphogenesis and, if so, whether the block occurs before or after the incorporation of the genome into the assembling virus particle. To address these and other questions, we constructed and characterized a conditionally lethal recombinant vaccinia virus in which the A8L gene is stringently repressed by the Escherichia coli lac operator system. The amount of 82-kDa protein synthesized could be regulated by the amount of inducer: from undetectable to higher than normal levels. Virus replication, as determined by plaque formation or virus yield upon synchronous infection, was dependent on inducer. Nevertheless, de novo synthesis of the 82-kDa subunit was not required for viral early, intermediate, and late gene expression or DNA replication. Overexpression of the A8L gene alone, produced by high concentrations of inducer, inhibited viral late protein synthesis, whereas overexpression of the D6R gene alone or both VETF genes simultaneously had little inhibitory effect. Laser confocal fluorescence and quantitative electron microscopic analyses revealed that immature and DNA-containing intermediate stage particles accumulated in the absence of inducer, indicating that the A8L protein has a role in morphogenesis of the core and subsequent events.

Published

1998

29. Association of the vaccinia virus A11 protein with the endoplasmic reticulum and crescent precursors of immature virions

Author

Liliana Maruri-Avidal, Bernard Moss, and Andrea S. Weisberg

Subjects

Scaffold protein, Viral protein, Immunology, Vaccinia virus, Plasma protein binding, Biology, medicine.disease_cause, Endoplasmic Reticulum, Virus Replication, Microbiology, Cell Line, Viral Proteins, Microscopy, Electron, Transmission, Virology, medicine, Viroplasm, Humans, Endoplasmic reticulum, Virus Assembly, Structure and Assembly, Virion, Molecular biology, Cell biology, Viral replication, Cytoplasm, Insect Science, Cell fractionation, Protein Binding

Abstract

The apparent de novo formation of viral membranes within cytoplasmic factories is a mysterious, poorly understood first step in poxvirus morphogenesis. Genetic studies identified several viral proteins essential for membrane formation and the assembly of immature virus particles. Their repression results in abortive replication with the accumulation of dense masses of viroplasm. In the present study, we further characterized one of these proteins, A11, and investigated its association with cellular and viral membranes under normal and abortive replication conditions. We discovered that A11 colocalized in cytoplasmic factories with the endoplasmic reticulum (ER) and L2, another viral protein required for morphogenesis. Confocal microscopy and subcellular fractionation indicated that A11 was not membrane associated in uninfected cells, whereas L2 still colocalized with the ER. Cell-free transcription and translation experiments indicated that both A11 and L2 are tail-anchored proteins that associate posttranslationally with membranes and likely require specific cytoplasmic targeting chaperones. Transmission electron microscopy indicated that A11, like L2, associated with crescent membranes and immature virions during normal infection and with vesicles and tubules near masses of dense viroplasm during abortive infection in the absence of the A17 or A14 protein component of viral membranes. When the synthesis of A11 was repressed, “empty” immature-virion-like structures formed in addition to masses of viroplasm. The immature-virion-like structures were labeled with antibodies to A17 and to the D13 scaffold protein and were closely associated with calnexin-labeled ER. These studies revealed similarities and differences between A11 and L2, both of which may be involved in the recruitment of the ER for virus assembly.

Published

2013

30. Vaccinia virus L2 protein associates with the endoplasmic reticulum near the growing edge of crescent precursors of immature virions and stabilizes a subset of viral membrane proteins

Author

Andrea S. Weisberg, Liliana Maruri-Avidal, and Bernard Moss

Subjects

Cytoplasm, Immunology, Blotting, Western, Vaccinia virus, Biology, Endoplasmic Reticulum, Virus Replication, Microbiology, Viral Matrix Proteins, Virology, Calnexin, Vaccinia, Humans, Protein disulfide-isomerase, Viral matrix protein, Protein Stability, Endoplasmic reticulum, Virus Assembly, Virion, Viral membrane, Molecular biology, Cell biology, Virus-Cell Interactions, Membrane protein, Viral replication, Insect Science, HeLa Cells

Abstract

The initial step in poxvirus morphogenesis, the formation of crescent membranes, occurs within cytoplasmic factories. L2 is one of several vaccinia virus proteins known to be necessary for formation of crescents and the only one synthesized early in infection. Virus replication was unaffected when the L2R open reading frame was replaced by L2R containing an N-terminal epitope tag while retaining the original promoter. L2 colocalized with the endoplasmic reticulum (ER) protein calnexin throughout the cytoplasm of infected and transfected cells. Topological studies indicated that the N terminus of L2 is exposed to the cytoplasm with the hydrophobic C terminus anchored in the ER. Using immunogold labeling and electron microscopy, L2 was detected in tubular membranes outside factories and inside factories near crescents and close to the edge or rim of crescents; a similar labeling pattern was found for the ER luminal protein disulfide isomerase (PDI). The phenotype of L2 conditional lethal mutants and the localization of L2 suggest that it participates in elongation of crescents by the addition of ER membrane to the growing edge. Small amounts of L2 and PDI were detected within immature and mature virions, perhaps trapped during assembly. The repression of L2, as well as A11 and A17, two other proteins that are required for viral crescent formation, profoundly decreased the stability of a subset of viral membrane proteins including those comprising the entry-fusion complex. To avoid degradation, these unstable membrane proteins may need to directly insert into the viral membrane or be rapidly shunted there from the ER.

Published

2011

31. Assembly and disassembly of the capsid-like external scaffold of immature virions during vaccinia virus morphogenesis

Author

Andrea S. Weisberg, Himani Bisht, Bernard Moss, and Patricia Szajner

Subjects

Immunology, Morphogenesis, Vaccinia virus, Biology, Microbiology, chemistry.chemical_compound, Viral Proteins, Capsid, Virology, Humans, Poxviridae, Orthopoxvirus, Particle Size, Virus Assembly, Structure and Assembly, Virion, Membrane Proteins, Immunogold labelling, biology.organism_classification, Molecular biology, Cell biology, Transmembrane domain, chemistry, Membrane protein, Insect Science, Capsid Proteins, Vaccinia, Protein Binding

Abstract

Infectious poxvirus particles are unusual in that they are brick shaped and lack symmetry. Nevertheless, an external honeycomb lattice comprised of a capsid-like protein dictates the spherical shape and size of immature poxvirus particles. In the case of vaccinia virus, trimers of 63-kDa D13 polypeptides form the building blocks of the lattice. In the present study, we addressed two questions: how D13, which has no transmembrane domain, associates with the immature virion (IV) membrane to form the lattice structure and how this scaffold is removed during the subsequent stage of morphogenesis. Interaction of D13 with the A17 membrane protein was demonstrated by immunoaffinity purification and Western blot analysis. In addition, the results of immunogold electron microscopy indicated a close association of A17 and D13 in crescents, as well as in vesicular structures when crescent formation was prevented. Further studies indicated that binding of A17 to D13 was abrogated by truncation of the N-terminal segment of A17. The N-terminal region of A17 was also required for the formation of crescent and IV structures. Disassembly of the D13 scaffold correlated with the processing of A17 by the I7 protease. When I7 expression was repressed, D13 was retained on aberrant virus particles. Furthermore, the morphogenesis of IVs to mature virions was blocked by mutation of the N-terminal but not the C-terminal cleavage site on A17. Taken together, these data indicate that A17 and D13 interactions regulate the assembly and disassembly of the IV scaffold.

Published

2009

32. Vaccinia virus entry into cells via a low-pH-dependent endosomal pathway

Author

Timothy R. Wagenaar, Andrea S. Weisberg, Alan C. Townsley, and Bernard Moss

Subjects

Cytoplasm, Time Factors, Endosome, viruses, Immunology, Vaccinia virus, Endosomes, Microbiology, Virus, Cell Line, Cell membrane, chemistry.chemical_compound, Viral entry, Virology, medicine, Humans, Poxviridae, Orthopoxvirus, Enzyme Inhibitors, Monensin, Microscopy, Confocal, biology, Ionophores, Cell Membrane, Bafilomycin, Hydrogen-Ion Concentration, biology.organism_classification, Cell biology, Virus-Cell Interactions, medicine.anatomical_structure, chemistry, Insect Science, Macrolides, Vaccinia, HeLa Cells

Abstract

Previous studies established that vaccinia virus could enter cells by fusion with the plasma membrane at neutral pH. However, low pH triggers fusion of vaccinia virus-infected cells, a hallmark of viruses that enter by the endosomal route. Here, we demonstrate that entry of mature vaccinia virions is accelerated by brief low-pH treatment and severely reduced by inhibitors of endosomal acidification, providing evidence for a predominant low-pH-dependent endosomal pathway. Entry of vaccinia virus cores into the cytoplasm, measured by expression of firefly luciferase, was increased more than 10-fold by exposure to a pH of 4.0 to 5.5. Furthermore, the inhibitors of endosomal acidification bafilomycin A1, concanamycin A, and monensin each lowered virus entry by more than 70%. This reduction was largely overcome by low-pH-induced entry through the plasma membrane, confirming the specificities of the drugs. Entry of vaccinia virus cores with or without brief low-pH treatment was visualized by electron microscopy of thin sections of immunogold-stained cells. Although some virus particles fused with the plasma membrane at neutral pH, 30 times more fusions and a greater number of cytoplasmic cores were seen within minutes after low-pH treatment. Without low-pH exposure, the number of released cores lagged behind the number of virions in vesicles until 30 min posttreatment, when they became approximately equal, perhaps reflecting the time of endosome acidification and virus fusion. The choice of two distinct pathways may contribute to the ability of vaccinia virus to enter a wide range of cells.

Published

2006

33. Deletion of the Vaccinia Virus I2 Protein Interrupts Virion Morphogenesis, Leading to Retention of the Scaffold Protein and Mislocalization of Membrane-Associated Entry Proteins.

Author

Seong-In Hyun, Weisberg, Andrea, and Mossa, Bernard

Subjects

*VACCINIA, *PROTEINS, *VIRION, *MORPHOGENESIS, *SCAFFOLD proteins, *C-terminal binding proteins

Abstract

The I2L open reading frame of vaccinia virus (VACV) encodes a conserved 72-amino-acid protein with a putative C-terminal transmembrane domain. Previous studies with a tetracycline-inducible mutant demonstrated that I2-deficient virions are defective in cell entry. The purpose of the present study was to determine the step of replication or entry that is affected by loss of the I2 protein. Fluorescence microscopy experiments showed that I2 colocalized with a major membrane protein of immature and mature virions. We generated a cell line that constitutively expressed I2 and allowed construction of the VACV I2L deletion mutant v▵I2. As anticipated, v▵I2 was unable to replicate in cells that did not express I2. Unexpectedly, morphogenesis was interrupted at a stage after immature virion formation, resulting in the accumulation of dense spherical particles instead of brick-shaped mature virions with welldefined core structures. The abnormal particles retained the D13 scaffold protein of immature virions, were severely deficient in the transmembrane proteins that comprise the entry fusion complex (EFC), and had increased amounts of unprocessed membrane and core proteins. Total lysates of cells infected with v▵I2 also had diminished EFC proteins due to instability attributed to their hydrophobicity and failure to be inserted into viral membranes. A similar instability of EFC proteins had previously been found with unrelated mutants blocked earlier in morphogenesis that also accumulated viral membranes retaining the D13 scaffold. We concluded that I2 is required for virion morphogenesis, release of the D13 scaffold, and the association of EFC proteins with viral membranes. [ABSTRACT FROM AUTHOR]

Published

2017

34. Vaccinia virus G7L protein Interacts with the A30L protein and is required for association of viral membranes with dense viroplasm to form immature virions

Author

Patricia Szajner, Howard Jaffe, Andrea S. Weisberg, and Bernard Moss

Subjects

Transcription, Genetic, viruses, Immunology, Mutant, Molecular Sequence Data, Vaccinia virus, Biology, Virus Replication, Microbiology, Epitope, Virus, Cell Line, chemistry.chemical_compound, Viral Envelope Proteins, Virology, Protein biosynthesis, Viroplasm, Humans, Amino Acid Sequence, Peptide sequence, Viral Core Proteins, Virus Assembly, Structure and Assembly, Virion, Molecular biology, Cell biology, Microscopy, Electron, Viral replication, chemistry, Insect Science, Protein Biosynthesis, Vaccinia, HeLa Cells

Abstract

The vaccinia virus A30L protein is required for the association of electron-dense, granular, proteinaceous material with the concave surfaces of crescent membranes, an early step in viral morphogenesis. For the identification of additional proteins involved in this process, we used an antibody to the A30L protein, or to an epitope appended to its C terminus, to capture complexes from infected cells. A prominent 42-kDa protein was resolved and identified by mass spectrometry as the vaccinia virus G7L protein. This previously uncharacterized protein was expressed late in infection and was associated with immature virions and the cores of mature particles. In order to study the role of the G7L protein, a conditional lethal mutant was made by replacing the G7L gene with an inducible copy. Expression of G7L and formation of infectious virus was dependent on the addition of inducer. Under nonpermissive conditions, morphogenesis was blocked and viral crescent membranes and immature virions containing tubular elements were separated from the electron-dense granular viroplasm, which accumulated in large spherical masses. This phenotype was identical to that previously obtained with an inducible, conditional lethal A30L mutant. Additional in vivo and in vitro experiments provided evidence for the direct interaction of the A30L and G7L proteins and demonstrated that the stability of each one was dependent on its association with the other.

Published

2003

35. The vaccinia virus A33R protein provides a chaperone function for viral membrane localization and tyrosine phosphorylation of the A36R protein

Author

Andrea S. Weisberg, Bernard Moss, and Elizabeth J. Wolffe

Subjects

Vesicle-associated membrane protein 8, Endosome, viruses, Immunology, Vaccinia virus, Protein tyrosine phosphatase, Biology, Microbiology, Viral Envelope Proteins, Virology, Extracellular, Serine, Humans, Protein phosphorylation, Phosphorylation, Viral Structural Proteins, Structure and Assembly, Viral membrane, Molecular biology, Actins, Cell biology, Cytoplasm, Insect Science, Tyrosine, Intracellular, HeLa Cells, Molecular Chaperones

Abstract

Vaccinia virus, the prototypic member of the poxvirus family, is a complex enveloped DNA virus with antigenically distinct intracellular and extracellular infectious forms (1, 5). Although the majority of intracellular mature virions (IMV) reside in the cytoplasm until cell lysis, some are wrapped by additional membranes and transported to the cell surface. Two related types of extracellular virions have been identified: adherent cell-associated enveloped virions (CEV), which are needed for efficient cell-to-cell spread (4), and released extracellular enveloped virions (EEV), which promote long range dissemination (19). Although the mechanism of formation of IMV is still poorly understood, considerable progress has been made in identifying the cellular membranes and viral proteins required for extracellular virion formation. The double membranes that wrap IMV to form intracellular enveloped virions (IEV) are derived from late Golgi or endosomal cisternae (15, 25). IEV are transported to the cell periphery, where they acquire actin tails, similar to those made by other intracellular pathogens such as Listeria and Shigella spp., and form the tips of protruding microvilli (6, 14, 16, 27). Virions are externalized at the plasma membrane, apparently losing the outermost of the two IEV-specific membranes in the process. Six proteins, encoded by the F13L, B5R, A33R, A34R, A36R, and A56R open reading frames (ORFs), have been identified as constituents of the IEV or EEV membrane (8, 10, 17, 18, 20, 22, 29). Deletion of any of these ORFs, except for A56R, which encodes the viral hemagglutinin, yields a mutant with a small-plaque phenotype. Mutants with deleted F13L or B5R (3, 11, 30) ORFs have defects in membrane wrapping that lead to reduced production of CEV and EEV. The small-plaque phenotypes of A33R, A34R, or A36R deletion mutants, however, correlated with defects in actin tail formation rather than with reduced production of EEV (21, 24, 31, 33). The latter results indicated that actin tails were important for virus spread rather than for the egress of vaccinia virus. Based on the above observations, we proposed that the A33R, A34R, and A36R proteins interact to form a platform for nucleation of actin tails (33). While we were carrying out experiments to further investigate this hypothesis, evidence for physical associations among EEV proteins and between tyrosine-phosphorylated A36R protein and the cellular adapter protein Nck, leading to the recruitment of N-WASP to the site of actin assembly, was reported (12, 23). Here, we confirm interactions between the A33R and A36R proteins and demonstrate that both are phosphorylated predominantly on serine residues and that viral membrane localization and tyrosine phosphorylation of the A36R protein are dependent on expression of the A33R protein.

Published

2000

36. Vaccinia virus WR gene A5L is required for morphogenesis of mature virions

Author

Ollie Williams, Elizabeth J. Wolffe, Andrea S. Weisberg, and Michael Merchlinsky

Subjects

Genes, Viral, Viral protein, viruses, Immunology, Vaccinia virus, Biology, Recombinant virus, medicine.disease_cause, Virus Replication, Microbiology, Virus, Cell Line, Late protein, chemistry.chemical_compound, Open Reading Frames, Viral Proteins, Virology, medicine, Morphogenesis, Inducer, Gene, Structure and Assembly, Virion, Molecular biology, Viral replication, chemistry, Insect Science, DNA, Viral, Mutation, Vaccinia

Abstract

The vaccinia virus WR A5L open reading frame (corresponding to open reading frame A4L in vaccinia virus Copenhagen) encodes an immunodominant late protein found in the core of the vaccinia virion. To investigate the role of this protein in vaccinia virus replication, we have constructed a recombinant virus, vA5Li, in which the endogenous gene has been deleted and an inducible copy of the A5 gene dependent on isopropyl-β- d -thiogalactopyranoside (IPTG) for expression has been inserted into the genome. In the absence of inducer, the yield of infectious virus was dramatically reduced. However, DNA synthesis and processing, viral protein expression (except for A5), and early stages in virion formation were indistinguishable from the analogous steps in a normal infection. Electron microscopy revealed that the major vaccinia virus structural form present in cells infected with vA5Li in the absence of inducer was immature virions. Viral particles were purified from vA5Li-infected cells in the presence and absence of inducer. Both particles contained viral DNA and the full complement of viral proteins, except for A5, which was missing from particles prepared in the absence of inducer. The particles prepared in the presence of IPTG were more infectious than those prepared in its absence. The A5 protein appears to be required for the immature virion to form the brick-shaped intracellular mature virion.

Published

1999

37. Direct Formation of Vaccinia Virus Membranes from the Endoplasmic Reticulum in the Absence of the Newly Characterized L2-Interacting Protein A30.5

Author

Maruri-Avidal, Liliana, primary, Weisberg, Andrea S., additional, and Moss, Bernard, additional

Published

2013

38. Association of the Vaccinia Virus A11 Protein with the Endoplasmic Reticulum and Crescent Precursors of Immature Virions

Author

Maruri-Avidal, Liliana, primary, Weisberg, Andrea S., additional, and Moss, Bernard, additional

Published

2013

39. Vaccinia Virus A19 Protein Participates in the Transformation of Spherical Immature Particles to Barrel-Shaped Infectious Virions

Author

Satheshkumar, P. S., primary, Weisberg, A. S., additional, and Moss, B., additional

Published

2013

40. The A34R glycoprotein gene is required for induction of specialized actin-containing microvilli and efficient cell-to-cell transmission of vaccinia virus

Author

Bernard Moss, Ehud Katz, Elizabeth J. Wolffe, and Andrea S. Weisberg

Subjects

Viral protein, Phalloidine, viruses, Immunology, Vaccinia virus, Biology, medicine.disease_cause, Microbiology, Virus, chemistry.chemical_compound, Viral Envelope Proteins, Virology, Extracellular, medicine, Humans, Actin, Glycoproteins, chemistry.chemical_classification, Syncytium, Microvilli, Virion, Hydrogen-Ion Concentration, Molecular biology, Actins, Cell biology, Microscopy, Electron, chemistry, Insect Science, Vaccinia, Glycoprotein, Intracellular, HeLa Cells, Research Article

Abstract

The mechanisms allowing vaccinia virus to spread from cell to cell are incompletely understood. The A34R gene of vaccinia virus encodes a glycoprotein that is localized in the outer membranes of extracellular virions. The small-plaque phenotype of an A34R deletion mutant was similar to that of mutants with deletions in other envelope genes that fail to produce extracellular vaccinia virions. Transmission electron microscopy, however, revealed that the A34R mutant produced numerous extracellular particles that were labeled with antibodies to other outer-envelope proteins and with protein A-colloidal gold. Fluorescence and scanning electron microscopy indicated that expression of the A34R protein was necessary for detection of vaccinia virus-induced actin tails, which provide motility to the intracellular enveloped form of vaccinia virus, and of virus-tipped specialized microvilli that project from the cell. The ability of vaccinia virus-infected cells to form syncytia after a brief exposure to a pH below 6, known as fusion from within, failed to occur in the absence of expression of the A34R protein; nevertheless, purified A34R- virions were capable of mediating low-pH-induced fusion from without. The present study provides genetic and microscopic evidence for the involvement of a specific viral protein in the formation or stability of actin-containing microvilli and for a role of these structures in cell-to-cell spread rather than in formation of extracellular virions.

Published

1997

41. Analysis of Viral Membranes Formed in Cells Infected by a Vaccinia Virus L2-Deletion Mutant Suggests Their Origin from the Endoplasmic Reticulum

Author

Maruri-Avidal, Liliana, primary, Weisberg, Andrea S., additional, Bisht, Himani, additional, and Moss, Bernard, additional

Published

2012

42. Vaccinia Virus L2 Protein Associates with the Endoplasmic Reticulum near the Growing Edge of Crescent Precursors of Immature Virions and Stabilizes a Subset of Viral Membrane Proteins

Author

Maruri-Avidal, L., primary, Weisberg, A. S., additional, and Moss, B., additional

Published

2011

43. Participation of Vaccinia Virus L2 Protein in the Formation of Crescent Membranes and Immature Virions

Author

Maruri-Avidal, Liliana, primary, Domi, Arban, additional, Weisberg, Andrea S., additional, and Moss, Bernard, additional

Published

2011

44. Congregation of Orthopoxvirus Virions in Cytoplasmic A-Type Inclusions Is Mediated by Interactions of a Bridging Protein (A26p) with a Matrix Protein (ATIp) and a Virion Membrane-Associated Protein (A27p)

Author

Howard, Amanda R., primary, Weisberg, Andrea S., additional, and Moss, Bernard, additional

Published

2010

45. Assembly and Disassembly of the Capsid-Like External Scaffold of Immature Virions during Vaccinia Virus Morphogenesis

Author

Bisht, Himani, primary, Weisberg, Andrea S., additional, Szajner, Patricia, additional, and Moss, Bernard, additional

Published

2009

46. Vaccinia Virus H7 Protein Contributes to the Formation of Crescent Membrane Precursors of Immature Virions

Author

Satheshkumar, P. S., primary, Weisberg, Andrea, additional, and Moss, Bernard, additional

Published

2009

47. Vaccinia Virus L1 Protein Is Required for Cell Entry and Membrane Fusion

Author

Bisht, Himani, primary, Weisberg, Andrea S., additional, and Moss, Bernard, additional

Published

2008

48. Vaccinia Virus E2L Null Mutants Exhibit a Major Reduction in Extracellular Virion Formation and Virus Spread

Author

Domi, Arban, primary, Weisberg, Andrea S., additional, and Moss, Bernard, additional

Published

2008

49. Sequence-Independent Targeting of Transmembrane Proteins Synthesized within Vaccinia Virus Factories to Nascent Viral Membranes

Author

Husain, Matloob, primary, Weisberg, Andrea S., additional, and Moss, Bernard, additional

Published

2007

50. Vaccinia Virus Entry into Cells via a Low-pH-Dependent Endosomal Pathway

Author

Townsley, Alan C., primary, Weisberg, Andrea S., additional, Wagenaar, Timothy R., additional, and Moss, Bernard, additional

Published

2006