Your search keyword '"Bovine immunodeficiency virus"' showing total 14 results

1. Conserved Interaction of Lentiviral Vif Molecules with HIV-1 Gag and Differential Effects of Species-Specific Vif on Virus Production

Author

Wenying Gao, Hong Wang, Xiao Fang Yu, Limian Ling, Shaohua Wang, Wenwen Zheng, Wei Wei, Yajuan Rui, Zhaolong Li, and Xing Su

Subjects

Models, Molecular, 0301 basic medicine, Immunodeficiency Virus, Bovine, viruses, Immunology, Virus Replication, medicine.disease_cause, gag Gene Products, Human Immunodeficiency Virus, Microbiology, Virus, 03 medical and health sciences, Transduction (genetics), Species Specificity, Virology, vif Gene Products, Human Immunodeficiency Virus, medicine, Humans, Protein Interaction Domains and Motifs, Amino Acid Sequence, Conserved Sequence, biology, virus diseases, Bovine immunodeficiency virus, biochemical phenomena, metabolism, and nutrition, Simian immunodeficiency virus, biology.organism_classification, Viral infectivity factor, Virus-Cell Interactions, Ubiquitin ligase, HEK293 Cells, 030104 developmental biology, Viral replication, Capsid, Insect Science, HIV-1, biology.protein, Protein Processing, Post-Translational

Abstract

The virion infectivity factor (Vif) open reading frame is conserved among most lentiviruses. Vif molecules contribute to viral replication by inactivating host antiviral factors, the APOBEC3 cytidine deaminases. However, various species of lentiviral Vif proteins have evolved different strategies for overcoming host APOBEC3. Whether different species of lentiviral Vif proteins still preserve certain common features has not been reported. Here, we show for the first time that diverse lentiviral Vif molecules maintain the ability to interact with the human immunodeficiency virus type 1 (HIV-1) Gag precursor (Pr55 Gag ) polyprotein. Surprisingly, bovine immunodeficiency virus (BIV) Vif, but not HIV-1 Vif, interfered with HIV-1 production and viral infectivity even in the absence of APOBEC3. Further analysis revealed that BIV Vif demonstrated an enhanced interaction with Pr55 Gag compared to that of HIV-1 Vif, and BIV Vif defective for the Pr55 Gag interaction lost its ability to inhibit HIV-1. The C-terminal region of capsid (CA) and the p2 region of Pr55 Gag , which are important for virus assembly and maturation, were involved in the interaction. Transduction of CD4 + T cells with BIV Vif blocked HIV-1 replication. Thus, the conserved Vif-Pr55 Gag interaction provides a potential target for the future development of antiviral strategies. IMPORTANCE The conserved Vif accessory proteins of primate lentiviruses HIV-1, simian immunodeficiency virus (SIV), and BIV all form ubiquitin ligase complexes to target host antiviral APOBEC3 proteins for degradation, with different cellular requirements and using different molecular mechanisms. Here, we demonstrate that BIV Vif can interfere with HIV-1 Gag maturation and suppress HIV-1 replication through interaction with the precursor of the Gag (Pr55 Gag ) of HIV-1 in virus-producing cells. Moreover, the HIV-1 and SIV Vif proteins are conserved in terms of their interactions with HIV-1 Pr55 Gag although HIV-1 Vif proteins bind Pr55 Gag less efficiently than those of BIV Vif. Our research not only sheds new light on this feature of these conserved lentiviral Vif proteins but also provides a formerly unrecognized target for the development of antiviral strategies. Since increasing the Vif-Pr55 Gag interaction could potentially suppress virus proliferation, this approach could offer a new strategy for the development of HIV inhibitors.

Published

2017

2. Core-Binding Factor Subunit Beta Is Not Required for Non-Primate Lentiviral Vif-Mediated APOBEC3 Degradation

Author

Youwei Ai, Dantong Zhu, Cuihui Wang, Chao Su, Jian Ma, Jianzhang Ma, and Xiaojun Wang

Subjects

Feline immunodeficiency virus, Gene Products, vif, viruses, Immunology, Microbiology, Core Binding Factor beta Subunit, Virus, Cytosine Deaminase, Equine infectious anemia, Retrovirus, Cytidine Deaminase, Virology, Humans, APOBEC Deaminases, Caprine arthritis encephalitis virus, DNA Primers, Base Sequence, biology, Reverse Transcriptase Polymerase Chain Reaction, Lentivirus, virus diseases, Bovine immunodeficiency virus, biochemical phenomena, metabolism, and nutrition, biology.organism_classification, Viral infectivity factor, Virus-Cell Interactions, HEK293 Cells, Insect Science, Proteolysis

Abstract

Viral infectivity factor (Vif) is required for lentivirus fitness and pathogenicity, except in equine infectious anemia virus (EIAV). Vif enhances viral infectivity by a Cullin5-Elongin B/C E3 complex to inactivate the host restriction factor APOBEC3. Core-binding factor subunit beta (CBF-β) is a cell factor that was recently shown to be important for the primate lentiviral Vif function. Non-primate lentiviral Vif also degrades APOBEC3 through the proteasome pathway. However, it is unclear whether CBF-β is required for the non-primate lentiviral Vif function. In this study, we demonstrated that the Vifs of non-primate lentiviruses, including feline immunodeficiency virus (FIV), bovine immunodeficiency virus (BIV), caprine arthritis encephalitis virus (CAEV), and maedi-visna virus (MVV), do not interact with CBF-β. In addition, CBF-β did not promote the stability of FIV, BIV, CAEV, and MVV Vifs. Furthermore, CBF-β silencing or overexpression did not affect non-primate lentiviral Vif-mediated APOBEC3 degradation. Our results suggest that non-primate lentiviral Vif induces APOBEC3 degradation through a different mechanism than primate lentiviral Vif. IMPORTANCE The APOBEC3 protein family members are host restriction factors that block retrovirus replication. Vif, an accessory protein of lentivirus, degrades APOBEC3 to rescue viral infectivity by forming Cullin5-Elongin B/C-based E3 complex. CBF-β was proved to be a novel regulator of primate lentiviral Vif function. In this study, we found that CBF-β knockdown or overexpression did not affect FIV Vif's function, which induced polyubiquitination and degradation of APOBEC3 by recruiting the E3 complex in a manner similar to that of HIV-1 Vif. We also showed that other non-primate lentiviral Vifs did not require CBF-β to degrade APOBEC3. CBF-β did not interact with non-primate lentiviral Vifs or promote their stability. These results suggest that a different mechanism exists for the Vif-APOBEC interaction and that non-primates are not suitable animal models for exploring pharmacological interventions that disrupt Vif–CBF-β interaction.

Published

2014

3. The Bovine Immunodeficiency Virus Rev Protein: Identification of a Novel Lentiviral Bipartite Nuclear Localization Signal Harboring an Atypical Spacer Sequence

Author

Andrea Gomez Corredor and Denis Archambault

Subjects

Signal peptide, Immunodeficiency Virus, Bovine, Nucleolus, viruses, Molecular Sequence Data, Nuclear Localization Signals, Immunology, Biology, Microbiology, Green fluorescent protein, Virology, Consensus sequence, Animals, Humans, NLS, Amino Acid Sequence, Peptide sequence, Cells, Cultured, Cell Nucleus, Bovine immunodeficiency virus, biology.organism_classification, Molecular biology, Genome Replication and Regulation of Viral Gene Expression, Gene Products, rev, Insect Science, Cell Nucleolus, Nuclear localization sequence

Abstract

The bovine immunodeficiency virus (BIV) Rev protein (186 amino acids [aa] in length) is involved in the nuclear exportation of partially spliced and unspliced viral RNAs. Previous studies have shown that BIV Rev localizes in the nucleus and nucleolus of infected cells. Here we report the characterization of the nuclear/nucleolar localization signals (NLS/NoLS) of this protein. Through transfection of a series of deletion mutants of BIV Rev fused to enhanced green fluorescent protein and fluorescence microscopy analyses, we were able to map the NLS region between aa 71 and 110 of the protein. Remarkably, by conducting alanine substitution of basic residues within the aa 71 to 110 sequence, we demonstrated that the BIV Rev NLS is bipartite, maps to aa 71 to 74 and 95 to 101, and is predominantly composed of arginine residues. This is the first report of a bipartite Rev (or Rev-like) NLS in a lentivirus/retrovirus. Moreover, this NLS is atypical, as the length of the sequence between the motifs composing the bipartite NLS, e.g., the spacer sequence, is 20 aa. Further mutagenesis experiments also identified the NoLS region of BIV Rev. It localizes mainly within the NLS spacer sequence. In addition, the BIV Rev NoLS sequence differs from the consensus sequence reported for other viral and cellular nucleolar proteins. In summary, we conclude that the nucleolar and nuclear localizations of BIV Rev are mediated via novel NLS and NoLS motifs.

Published

2009

4. Important Role for the CA-NC Spacer Region in the Assembly of Bovine Immunodeficiency Virus Gag Protein

Author

James B. Whitney, Chen Liang, Jing Hu, Rodney S. Russell, and Xiaofeng Guo

Subjects

Immunodeficiency Virus, Bovine, Feline immunodeficiency virus, Visna virus, Recombinant Fusion Proteins, viruses, Amino Acid Motifs, Molecular Sequence Data, Immunology, Gene Products, gag, Replication, Microbiology, Virus, Equine infectious anemia, Capsid, Virology, Animals, Humans, Amino Acid Sequence, Nucleocapsid, Peptide sequence, biology, Virus Assembly, Cell Membrane, Bovine immunodeficiency virus, Group-specific antigen, biology.organism_classification, Molecular biology, Insect Science, COS Cells, Mutation, Cattle, HeLa Cells

Abstract

Lentiviral Gag proteins contain a short spacer sequence that separates the capsid (CA) from the downstream nucleocapsid (NC) domain. This short spacer has been shown to play an important role in the assembly of human immunodeficiency virus type 1 (HIV-1). We have now extended this finding to the CA-NC spacer motif within the Gag protein of bovine immunodeficiency virus (BIV). Mutation of this latter spacer sequence led to dramatic reductions in virus production, which was mainly attributed to the severely disrupted association of the mutated Gag with the plasma membrane, as shown by the results of membrane flotation assays and confocal microscopy. Detailed mutagenesis analysis of the BIV CA-NC spacer region for virus assembly determinants led to the identification of two key residues, L368 and M372, which are separated by three amino acids, 369-VAA-371. Incidentally, the same two residues are present within the HIV-1 CA-NC spacer region at positions 364 and 368 and have also been shown to be crucial for HIV-1 assembly. Regardless of this conservation between these two viruses, the BIV CA-NC spacer could not be replaced by its HIV-1 counterpart without decreasing virus production, as opposed to its successful replacement by the CA-NC spacer sequences from the nonprimate lentiviruses such as feline immunodeficiency virus (FIV), equine infectious anemia virus and visna virus, with the sequence from FIV showing the highest effectiveness in this regard. Taken together, these data suggest a pivotal role for the CA-NC spacer region in the assembly of BIV Gag; however, the mechanism involved therein may differ from that for the HIV-1 CA-NC spacer.

Published

2004

5. Replication of Human Immunodeficiency Viruses Engineered with Heterologous Tat-Transactivation Response Element Interactions

Author

Alan D. Frankel, Mark A. Wainberg, and Baode Xie

Subjects

Transcriptional Activation, Immunodeficiency Virus, Bovine, Cyclin T1, viruses, Molecular Sequence Data, Immunology, Replication, RNA polymerase II, Response Elements, Virus Replication, Microbiology, Virus, Cell Line, Transcription (biology), Virology, Humans, Amino Acid Sequence, HIV Long Terminal Repeat, Binding Sites, biology, RNA, Bovine immunodeficiency virus, biology.organism_classification, Viral replication, Insect Science, Gene Products, tat, HIV-1, biology.protein, RNA, Viral, tat Gene Products, Human Immunodeficiency Virus, Genetic Engineering

Abstract

Human immunodeficiency viruses (HIVs) and the related bovine lentiviruses bovine immunodeficiency virus (BIV) and Jembrana disease virus (JDV) utilize the viral Tat protein to activate viral transcription. The arginine-rich RNA-binding domains of the Tat proteins bind to their cognate transactivation response element (TAR) RNA hairpins located at the 5′ ends of the viral mRNAs, resulting in enhanced processivity of RNA polymerase II. It has previously been shown that HIV type 1 (HIV-1) Tat requires the cellular cyclin T1 protein for high-affinity RNA binding whereas BIV Tat and JDV Tat bind with high affinity on their own and adopt distinct β-hairpin conformations when complexed to RNA. Here we have engineered the BIV and JDV Tat-TAR interactions into HIV-1 and show that the heterologous interactions support viral replication, correlating well with their RNA-binding affinities. Viruses engineered with a variant TAR able to bind all three Tat proteins replicate efficiently with any of the proteins. In one virus containing a noncognate Tat-TAR pair that neither interacts nor efficiently replicates (HIV-1 TAR and BIV Tat), viral revertants were isolated in which TAR had become mutated to generate a functional BIV Tat binding site. Our results support the view that incremental changes to TAR structure can provide routes for evolving new Tat-TAR complexes while maintaining active viral replication.

Published

2003

6. Construction and Molecular Analysis of Gene Transfer Systems Derived from Bovine Immunodeficiency Virus

Author

Robert D. Berkowitz, Wei Yu Lin, Stan Tamaki, Gabor Veres, Andrea Coward, Karl Eckert, Heini Ilves, and Ivan Plavec

Subjects

Adult, Immunodeficiency Virus, Bovine, Gene Transfer, Horizontal, viruses, Genetic enhancement, Genetic Vectors, Immunology, Microbiology, Virus, Cell Line, Transduction (genetics), Virology, Animals, Humans, biology, Genetically modified virus, Virus Assembly, Terminal Repeat Sequences, Bovine immunodeficiency virus, Genetic Therapy, Gene Therapy, biology.organism_classification, Insect Science, Lentivirus, HIV-1, Pseudotyping, Cattle, Stem cell

Abstract

Because lentiviruses are able to infect nondividing cells, these viruses might be utilized in gene therapy applications where the target cell does not divide. However, it has been suggested that the introduction of primate lentivirus sequences, particularly those of human immunodeficiency virus, into human cells may pose a health risk for the patient. To avoid this concern, we have constructed gene transfer systems based on a nonprimate lentivirus, bovine immunodeficiency virus. A panel of vectors and packaging constructs was generated and analyzed in a transient expression system for virion production and maturation, vector expression and encapsidation, and envelope protein pseudotyping. Virion preparations were also analyzed for transduction efficiency in a panel of human and nonhuman primary cells and immortalized cell lines. The virion preparations transduced most of the target cell types, with efficiencies up to 90% and with titers of unconcentrated virus up to 5 × 10 5 infectious doses/ml. In addition, infection of nondividing human cells, including unstimulated hematopoietic stem cells and irradiated endothelial cells, was observed.

Published

2001

7. Differentiation of Two Bovine Lentiviruses by a Monoclonal Antibody on the Basis of Epitope Specificity

Author

H.C. Minocha, Sanjay Kapil, Ling Zheng, Charles E. Wood, Graham E. Wilcox, Thomas A. Loughin, and Shucheng Zhang

Subjects

Microbiology (medical), Immunodeficiency Virus, Bovine, medicine.drug_class, viruses, Clinical Biochemistry, Immunology, Cattle Diseases, Enzyme-Linked Immunosorbent Assay, Biology, Monoclonal antibody, Veterinary Immunology, Epitope, law.invention, Diagnosis, Differential, Epitopes, Immunoglobulin kappa-Chains, Mice, Capsid, Antigen, Antibody Specificity, Antigens, Neoplasm, law, Tumor Cells, Cultured, medicine, Animals, Immunology and Allergy, Mice, Inbred BALB C, Hybridomas, Errata, Antibodies, Monoclonal, Bovine immunodeficiency virus, biology.organism_classification, Fusion protein, Virology, Molecular biology, Lentivirus Infections, Recombinant DNA, biology.protein, Cattle, Antibody

Abstract

Bovine immunodeficiency virus (BIV) and Jembrana disease virus (JDV) are bovine lentiviruses that are closely related genetically. A recombinant fusion protein containing the capsid protein of BIV expressed in Escherichia coli was used to immunize mice and produce monoclonal antibodies. Six hybridomas specific for BIV capsid protein were identified, and one antibody, designated 10H1, was characterized further. Competitive binding assays were performed to analyze the topography of antigenic determinants by enzyme-linked immunosorbent assay and demonstrated the existence of at least three distinct antigenic determinants on capsid protein. The monoclonal antibody reacted specifically with both BIV capsid and the recombinant fusion protein in Western immunoblot analyses. However, it did not react with the recombinant capsid fusion protein of JDV, indicating that BIV contains at least one unique epitope in the capsid protein that is absent in JDV. Further mapping of the epitope by chemical cleavage analysis identified that the epitope is located at the 6.4-kDa N terminus of the 29-kDa capsid protein. This monoclonal antibody assay will be valuable for distinguishing the two closely related lentiviruses by Western blotting.

Published

2001

8. Cloning of the Bovine Immunodeficiency Virus gag Gene and Development of a Recombinant-Protein-Based Enzyme-Linked Immunosorbent Assay

Author

Sanjay Kapil, Ling Zheng, Charles E. Wood, Thomas A. Loughin, Michelle Swanson, Ron Snider, Jinghua Liao, and H.C. Minocha

Subjects

Microbiology (medical), Immunodeficiency Virus, Bovine, medicine.drug_class, Clinical Biochemistry, Immunology, Gene Products, gag, Enzyme-Linked Immunosorbent Assay, medicine.disease_cause, Monoclonal antibody, Sensitivity and Specificity, law.invention, Antigen, law, medicine, Animals, Immunology and Allergy, Cloning, Molecular, Escherichia coli, Expression vector, biology, Bovine immunodeficiency virus, Group-specific antigen, biology.organism_classification, Virology, Molecular biology, Recombinant Proteins, biology.protein, Recombinant DNA, Cattle, Microbial Immunology, Antibody

Abstract

An enzyme-linked immunosorbent assay (ELISA) was established for the rapid detection of specific bovine immunodeficiency virus (BIV) antibodies in cattle, using recombinant Gag protein as an antigen. The gag coding region from BIV was cloned into an expression vector, pQE32, which expressed high levels of recombinant protein from Escherichia coli . The ELISA was standardized by a checkerboard titration against known BIV-positive and -negative sera from cattle and a monoclonal antibody to the Gag protein. A total of 139 cattle serum samples, from the diagnostic laboratory at Kansas State University, Manhattan, and from the Dairy Station, Louisiana State University, Baton Rouge, were compared by ELISA and immunoblot assays for the detection of BIV-specific antibodies. Of 26 cattle sera samples which tested positive using the immunoblot assay, 23 were positive by ELISA, thus establishing a strong correlation between the two tests. The sensitivity and specificity of ELISA relative to immunoblotting were 0.88 and 0.93, respectively. ELISA proved to be as specific as immunoblotting but was much less time-consuming and easier to perform.

Published

2000

9. Jembrana Disease Virus Tat Can Regulate Human Immunodeficiency Virus (HIV) Long Terminal Repeat-Directed Gene Expression and Can Substitute for HIV Tat in Viral Replication

Author

Hexin Chen, Graham E. Wilcox, Steven E Fong, Charles E. Wood, and Jun He

Subjects

Gene Expression Regulation, Viral, Transcriptional Activation, viruses, Molecular Sequence Data, Immunology, Replication, Gene Expression, Virus Replication, Binding, Competitive, Microbiology, Virus, Transactivation, Proviruses, Virology, Animals, Humans, Cells, Cultured, Phylogeny, HIV Long Terminal Repeat, Binding Sites, Base Sequence, biology, Genetic Complementation Test, virus diseases, Bovine immunodeficiency virus, Transfection, biology.organism_classification, Molecular biology, Long terminal repeat, Viral replication, Insect Science, Gene Products, tat, Lentivirus, HIV-1, Lentiviruses, Bovine, Leukocytes, Mononuclear, Nucleic Acid Conformation, RNA, Viral, Cattle, tat Gene Products, Human Immunodeficiency Virus

Abstract

Jembrana disease virus (JDV) is a bovine lentivirus genetically similar to bovine immunodeficiency virus; it causes an acute and sometimes fatal disease in infected animals. This virus carries a very potent Tat that can strongly activate not only its own long terminal repeat (LTR) but also the human immunodeficiency virus (HIV) LTR. In contrast, HIV Tat cannot reciprocally activate the JDV LTR (H. Chen, G. E. Wilcox, G. Kertayadnya, and C. Wood, J. Virol. 73:658–666, 1999). This indicates that in transactivation JDV Tat may utilize a mechanism similar to but not the same as that of the HIV Tat. To further study the similarity of JDV and HIVtatin transactivation, we first tested the responses of a series of HIV LTR mutants to the JDV Tat. Cross-transactivation of HIV LTR by JDV Tat was impaired by mutations that disrupted the HIV type 1 transactivation response element (TAR) RNA stem-loop structure. Our results demonstrated that JDV Tat, like HIV Tat, transactivated the HIV LTR at least partially in a TAR-dependent manner. However, the sequence in the loop region of TAR was not as critical for the function of JDV Tat as it was for HIV Tat. The competitive inhibition of Tat-induced transactivation by the truncated JDV or HIV Tat, which consisted only of the activation domain, suggested that similar cellular factors were involved in both JDV and HIV Tat-induced transactivation. Based on the one-round transfection assay with HIVtatmutant proviruses, the cotransfected JDVtatplasmid can functionally complement the HIVtatdefect. To further characterize the effect of JDV Tat on HIV, a stable chimeric HIV carrying the JDVtatgene was generated. This chimeric HIV replicated in a T-cell line, C8166, and in peripheral blood mononuclear cells, which suggested that JDV Tat can functionally substitute for HIV Tat. Further characterization of this chimeric virus will help to elucidate how JDV Tat functions and to explain the differences between HIV and JDV Tat transactivation.

Published

2000

10. Characterization of bovine immunodeficiency virus rev cDNAs and identification and subcellular localization of the Rev protein

Author

M S Oberste, J D Greenwood, Kunio Nagashima, J C Williamson, Terry D. Copeland, and Matthew A. Gonda

Subjects

Immunodeficiency Virus, Bovine, DNA, Complementary, Genes, Viral, Visna virus, viruses, Immunoelectron microscopy, Molecular Sequence Data, Immunology, Virus Replication, Microbiology, Virology, Complementary DNA, Gene expression, Amino Acid Sequence, Cloning, Molecular, Peptide sequence, DNA Primers, Viral Structural Proteins, Messenger RNA, Base Sequence, biology, Nuclear Proteins, Bovine immunodeficiency virus, rev Gene Products, Human Immunodeficiency Virus, Phosphoproteins, biology.organism_classification, Molecular biology, Gene Products, rev, Insect Science, RNA splicing, HIV-1, Peptides, Sequence Alignment, Research Article

Abstract

One of the six putative accessory genes of bovine immunodeficiency virus (BIV) is similar to those identified as rev in the human immunodeficiency virus and visna virus genomes. To further analyze the BIV rev gene locus, protein, and function, rev cDNAs were cloned and characterized. BIV rev mRNA is derived from the full-length transcript by multiple splicing events and consists of three exons, including the untranslated leader sequence and two coding exons. BIV rev cDNA was expressed in bacteria and in a mammalian in vitro translation expression system. A 23-kDa Rev protein (p23rev) was immunologically detected in lysates from both systems by using an antiserum made to a synthetic Rev peptide. Recombinant p23rev made in bacteria was purified and used to make a polyvalent antiserum. Antisera to Rev peptide and recombinant p23rev immunoprecipitated p23rev from BIV-infected mammalian cells but not from virions. A mammalian expression vector using the BIV rev cDNA was constructed; p23rev was immunoprecipitated with anti-Rev serum from 32P-labeled lysates of monkey cells transfected with this plasmid, demonstrating that BIV Rev is phosphorylated. Immunofluorescence and immunoelectron microscopy with anti-BIV Rev antisera localized Rev in the nucleus and, particularly, in the nucleoli of BIV-infected cells. In functional studies, the expression of BIV Rev was shown to positively regulate the appearance both of Gag protein, which is translated from the unspliced primary viral transcript, and of singly spliced env mRNA but not that of the multiply spliced tat mRNA. These results demonstrate that BIV Rev activity correlates with the known function of lentivirus Rev proteins.

Published

1993

11. Isolation and characterization of new wild-type isolates of bovine lentivirus

Author

David L. Suarez, Charles E. Wood, M J VanDerMaaten, and C A Whetstone

Subjects

Neutrophils, Molecular Sequence Data, Immunology, Cattle Diseases, Buffy coat, Biology, Polymerase Chain Reaction, Microbiology, Virus, law.invention, law, Virology, Animals, Lymphocytes, Polymerase chain reaction, Jembrana disease, Syncytium, Base Sequence, Lentivirus, Bovine immunodeficiency virus, Lentivirus Infections, biology.organism_classification, Genes, pol, Oligodeoxyribonucleotides, Insect Science, Florida, biology.protein, Cattle, Female, Antibody, Research Article

Abstract

Two new isolates of bovine lentivirus, also known as bovine immunodeficiency-like virus (BIV), were obtained from a seropositive cattle herd in Florida. This is the first report of new isolates of BIV since the original BIV strain, R29, was isolated in 1969. The two new BIV isolates were derived from blood buffy coat cells cocultivated in vitro with fetal bovine lung cell cultures. The new isolates differed in vitro from the original R29 isolate in replication and syncytium formation in fetal bovine lung cells. Both new isolates were confirmed as BIV by immunofluorescence assay, Western blotting (immunoblotting), and polymerase chain reaction. Sequence analyses of the polymerase chain reaction pol gene product showed 92.6 and 93.6% homology to the published nucleotide sequence of BIV R29-127, a molecular clone derived from BIV R29. Each of the new BIV isolates was inoculated into two calves, and virus was recovered between 5 and 10 days postinoculation (p.i.), with BIV seroconversion between 10 and 21 days p.i. Virus was recoverable and antibody was detectable for at least 4 months p.i. Two calves developed a transiently elevated mononuclear cell count, similar to what was reported for BIV R29 in the original experimental calf inoculations. No other clinical abnormalities were observed.

Published

1993

12. Immunological characterization of the gag gene products of bovine immunodeficiency virus

Author

M Y Hu, G J Tobin, Matthew A. Gonda, J K Battles, and Lynn Rasmussen

Subjects

Immunodeficiency Virus, Bovine, Antigenicity, viruses, Blotting, Western, Molecular Sequence Data, Immunology, Gene Products, gag, Biology, Microbiology, Epitope, Virus, law.invention, Open Reading Frames, law, Virology, Escherichia coli, Leukocytes, Animals, Amino Acid Sequence, Cloning, Molecular, Peptide sequence, Cells, Cultured, Base Sequence, Bovine immunodeficiency virus, Group-specific antigen, biology.organism_classification, Genes, gag, Molecular biology, Recombinant Proteins, Fusion Proteins, gag-pol, Capsid, Insect Science, HIV-1, Recombinant DNA, Nucleic Acid Conformation, RNA, Viral, Cattle, Peptides, Plasmids, Research Article

Abstract

The bovine immunodeficiency virus (BIV) gag gene encodes a 53-kDa precursor (Pr53gag) that is involved in virus particle assembly and is further processed into the putative matrix (MA), capsid (CA), and nucleocapsid (NC) functional domains in the mature virus. Gag determinants are also found in the Gag-Pol polyprotein precursor. To immunologically identify the major precursors and processed products of the BIV gag gene, monospecific rabbit sera to recombinant BIV MA protein and Pr53gag and peptides predicted to correspond to the CA and NC proteins and the MA-CA cleavage site were developed and used in immunoprecipitations and immunoblots of BIV antigens. Monospecific antisera to native and recombinant human immunodeficiency virus type 1 proteins were also used to identify analogous BIV Gag proteins and to determine whether cross-reactive epitopes were present in the BIV Gag precursors or processed products. The BIV MA, CA, and NC Gag proteins were identified as p16, p26, and p13, respectively. In addition to BIV Pr53gag, the major Gag precursor, two other Gag-related precursors of 170 and 49 kDa were identified that have been designated pPr170gag-pol and Pr49gag, respectively; pPr170gag-pol is the Gag-Pol polyprotein precursor, and Pr49gag is the transframe Gag precursor present in pPr170gag-pol. Several alternative Gag cleavage products were also observed, including p23, which contains CA and NC determinants, and p10, which contains a peptide sequence conserved in the CA proteins of most lentiviruses. The monospecific antisera to human immunodeficiency virus type 1 CA (p24) and NC (p7) proteins showed cross-reactivity to and aided in the identification of analogous BIV proteins. Based on the present data, a scheme for the processing of BIV Gag precursors is proposed.

Published

1992

13. Selection of TAR RNA-Binding Chameleon Peptides by Using a Retroviral Replication System

Author

Mark A. Wainberg, Alan D. Frankel, Valerie Calabro, and Baode Xie

Subjects

viruses, Immunology, Molecular Sequence Data, Replication, Arginine, Virus Replication, Microbiology, Cell Line, Mice, Structure-Activity Relationship, Retrovirus, Peptide Library, Virology, Animals, Combinatorial Chemistry Techniques, Humans, Amino Acid Sequence, Peptide library, Gene, HIV Long Terminal Repeat, biology, Lentivirus, RNA, Bovine immunodeficiency virus, RNA-Binding Proteins, biology.organism_classification, Viral replication, Viral Regulatory Proteins, Insect Science, Viral evolution, Gene Products, tat, HIV-1, Nucleic Acid Conformation, RNA, Viral, Cattle, tat Gene Products, Human Immunodeficiency Virus, Peptides

Abstract

The interaction between the arginine-rich motif (ARM) of the human immunodeficiency virus (HIV) Tat protein and TAR RNA is essential for Tat activation and viral replication. Two related lentiviruses, bovine immunodeficiency virus (BIV) and Jembrana disease virus (JDV), also require Tat ARM-TAR interactions to mediate activation, but the viruses have evolved different RNA-binding strategies. Interestingly, the JDV ARM can act as a “chameleon,” adopting both the HIV and BIV TAR binding modes. To examine how RNA-protein interactions may evolve in a viral context and possibly to identify peptides that recognize HIV TAR in novel ways, we devised a retroviral system based on HIV replication to amplify and select for RNA binders. We constructed a combinatorial peptide library based on the BIV Tat ARM and identified peptides that, like the JDV Tat ARM, also function through HIV TAR, revealing unexpected sequence characteristics of an RNAbinding chameleon. The results suggest that a retroviral screening approach may help identify high-affinity TAR binders and may provide new insights into the evolution of RNA-protein interactions. Many complex retroviruses, including the human immunodeficiency viruses (HIV) and related lentiviruses, encode RNA-binding proteins that regulate viral gene expression. While some RNA-binding domains may have been coopted from cellular genes, others may have arisen de novo and evolved in the viral context. The arginine-rich motif (ARM), found in several viral regulatory proteins, is a small (20 amino acids) RNA-binding domain that is a particularly attractive candidate for the viral evolution model. It has been shown in several cases that short peptides corresponding only to the ARM bind RNA with high affinity and specificity, typically using few types of amino acids other than arginine to recognize their RNA sites (18, 38). In principle, the relative simplicity of the ARM might allow specific RNA-binding domains to evolve rapidly in the context of an error-prone retrovirus and potentially to coevolve with its RNA target. Studies with the HIV and related lentiviral Tat proteins, described below, support such a view.

Published

2004

14. Envelope Glycoprotein Cytoplasmic Domains from Diverse Lentiviruses Interact with the Prenylated Rab Acceptor

Author

David T. Evans, Karl C. Tillman, and Ronald C. Desrosiers

Subjects

Feline immunodeficiency virus, viruses, Immunology, Molecular Sequence Data, Retroviridae Proteins, Vesicular Transport Proteins, Gp41, medicine.disease_cause, Virus Replication, Microbiology, Cell Line, Prenylation, Viral Envelope Proteins, GTP-Binding Proteins, Virology, Two-Hybrid System Techniques, medicine, Humans, Amino Acid Sequence, Cellular localization, Membrane Glycoproteins, biology, Lentivirus, Bovine immunodeficiency virus, virus diseases, Membrane Proteins, Simian immunodeficiency virus, biology.organism_classification, Virus-Cell Interactions, Insect Science, Simian Immunodeficiency Virus, Rab, Carrier Proteins, Protein Binding

Abstract

Lentivirus envelope glycoproteins have unusually long cytoplasmic domains compared to those of other retroviruses. To identify cellular binding partners of the simian immunodeficiency virus (SIV) envelope transmembrane protein (gp41) cytoplasmic domain (CD), we performed a yeast two-hybrid screen of a phytohemagglutinin-activated human T-cell cDNA library with the SIV gp41 CD. The majority of positive clones (50 of 54) encoded the prenylated Rab acceptor (PRA1). PRA1 is a 21-kDa protein associated with Golgi membranes that binds to prenylated Rab proteins in their GTP-bound state. While the cellular function of PRA1 is presently unknown, this protein appears to participate in intracellular vesicular trafficking, based on its cellular localization and ability to bind multiple members of the Rab protein family. Mammalian two-hybrid assays confirmed the interaction between the SIV gp41 CD and PRA1. Furthermore, gp41 sequences important for PRA1 binding were mapped to a central leucine-rich, amphipathic α-helix in the SIV gp41 cytoplasmic tail. Although the human immunodeficiency virus (HIV-1) gp41 CD failed to interact with PRA1 in the yeast two-hybrid system, its interaction with PRA1 was significantly better than that of the SIV gp41 CD in mammalian two-hybrid assays. Interestingly, PRA1 also interacted with the Env CDs of HIV-2, bovine immunodeficiency virus, equine infectious anemia virus, and feline immunodeficiency virus. Thus, PRA1 associates with envelope glycoproteins from widely divergent lentiviruses.

Published

2002