ABSTRACT
Human immunodeficiency virus (HIV) has a small genome and therefore relies heavily on the host cellular machinery to replicate. Identifying which host proteins and complexes come into physical contact with the viral proteins is crucial for a comprehensive understanding of how HIV rewires the host's cellular machinery during the course of infection. Here we report the use of affinity tagging and purification mass spectrometry to determine systematically the physical interactions of all 18 HIV-1 proteins and polyproteins with host proteins in two different human cell lines (HEK293 and Jurkat). Using a quantitative scoring system that we call MiST, we identified with high confidence 497 HIV-human protein-protein interactions involving 435 individual human proteins, with â¼40% of the interactions being identified in both cell types. We found that the host proteins hijacked by HIV, especially those found interacting in both cell types, are highly conserved across primates. We uncovered a number of host complexes targeted by viral proteins, including the finding that HIV protease cleaves eIF3d, a subunit of eukaryotic translation initiation factor 3. This host protein is one of eleven identified in this analysis that act to inhibit HIV replication. This data set facilitates a more comprehensive and detailed understanding of how the host machinery is manipulated during the course of HIV infection.
Subject(s)
HIV-1/chemistry , HIV-1/metabolism , Host-Pathogen Interactions , Human Immunodeficiency Virus Proteins/metabolism , Protein Interaction Mapping/methods , Protein Interaction Maps/physiology , Affinity Labels , Amino Acid Sequence , Conserved Sequence , Eukaryotic Initiation Factor-3/chemistry , Eukaryotic Initiation Factor-3/metabolism , HEK293 Cells , HIV Infections/metabolism , HIV Infections/virology , HIV Protease/metabolism , HIV-1/physiology , Human Immunodeficiency Virus Proteins/analysis , Human Immunodeficiency Virus Proteins/chemistry , Human Immunodeficiency Virus Proteins/isolation & purification , Humans , Immunoprecipitation , Jurkat Cells , Mass Spectrometry , Protein Binding , Reproducibility of Results , Virus ReplicationABSTRACT
Genome-wide siRNA screens have identified host cell factors important for efficient HIV infection, among which are nuclear pore proteins such as RanBP2/Nup358 and the karyopherin Transportin-3/TNPO3. Analysis of the roles of these proteins in the HIV replication cycle suggested that correct trafficking through the pore may facilitate the subsequent integration step. Here we present data for coupling between these steps by demonstrating that depletion of Transportin-3 or RanBP2 altered the terminal step in early HIV replication, the selection of chromosomal sites for integration. We found that depletion of Transportin-3 and RanBP2 altered integration targeting for HIV. These knockdowns reduced HIV integration frequency in gene-dense regions and near gene-associated features, a pattern that differed from that reported for depletion of the HIV integrase binding cofactor Psip1/Ledgf/p75. MLV integration was not affected by the Transportin-3 knockdown. Using siRNA knockdowns and integration targeting analysis, we also implicated several additional nuclear proteins in proper target site selection. To map viral determinants of integration targeting, we analyzed a chimeric HIV derivative containing MLV gag, and found that the gag replacement phenocopied the Transportin-3 and RanBP2 knockdowns. Thus, our data support a model in which Gag-dependent engagement of the proper transport and nuclear pore machinery mediate trafficking of HIV complexes to sites of integration.
Subject(s)
HIV/physiology , Host-Pathogen Interactions/physiology , Molecular Chaperones/metabolism , Nuclear Pore Complex Proteins/metabolism , beta Karyopherins/metabolism , Gene Expression Regulation, Viral , Gene Knockdown Techniques , HEK293 Cells , Humans , Molecular Chaperones/genetics , Nuclear Pore Complex Proteins/genetics , RNA, Small Interfering/genetics , Virus Replication , beta Karyopherins/genetics , gag Gene Products, Human Immunodeficiency Virus/genetics , gag Gene Products, Human Immunodeficiency Virus/metabolismABSTRACT
Lentiviruses such as HIV-1 traverse nuclear pore complexes (NPC) and infect terminally differentiated non-dividing cells, but how they do this is unclear. The cytoplasmic NPC protein Nup358/RanBP2 was identified as an HIV-1 co-factor in previous studies. Here we report that HIV-1 capsid (CA) binds directly to the cyclophilin domain of Nup358/RanBP2. Fusion of the Nup358/RanBP2 cyclophilin (Cyp) domain to the tripartite motif of TRIM5 created a novel inhibitor of HIV-1 replication, consistent with an interaction in vivo. In contrast to CypA binding to HIV-1 CA, Nup358 binding is insensitive to inhibition with cyclosporine, allowing contributions from CypA and Nup358 to be distinguished. Inhibition of CypA reduced dependence on Nup358 and the nuclear basket protein Nup153, suggesting that CypA regulates the choice of the nuclear import machinery that is engaged by the virus. HIV-1 cyclophilin-binding mutants CA G89V and P90A favored integration in genomic regions with a higher density of transcription units and associated features than wild type virus. Integration preference of wild type virus in the presence of cyclosporine was similarly altered to regions of higher transcription density. In contrast, HIV-1 CA alterations in another patch on the capsid surface that render the virus less sensitive to Nup358 or TRN-SR2 depletion (CA N74D, N57A) resulted in integration in genomic regions sparse in transcription units. Both groups of CA mutants are impaired in replication in HeLa cells and human monocyte derived macrophages. Our findings link HIV-1 engagement of cyclophilins with both integration targeting and replication efficiency and provide insight into the conservation of viral cyclophilin recruitment.
Subject(s)
Capsid Proteins/metabolism , Cell Nucleus/virology , Cyclophilin A/metabolism , HIV Infections/metabolism , HIV-1/physiology , Virus Replication , Active Transport, Cell Nucleus/physiology , Blotting, Western , Cell Line , Cell Nucleus/metabolism , HeLa Cells , Humans , Macrophages/metabolism , Macrophages/virology , Molecular Chaperones/metabolism , Nuclear Pore Complex Proteins/metabolism , Reverse Transcriptase Polymerase Chain Reaction , Virus Replication/physiologyABSTRACT
Human genetic diseases have been successfully corrected by integration of functional copies of the defective genes into human cells, but in some cases integration of therapeutic vectors has activated proto-oncogenes and contributed to leukemia. For this reason, extensive efforts have focused on analyzing integration site populations from patient samples, but the most commonly used methods for recovering newly integrated DNA suffer from severe recovery biases. Here, we show that a new method based on phage Mu transposition in vitro allows convenient and consistent recovery of integration site sequences in a form that can be analyzed directly using DNA barcoding and pyrosequencing. The method also allows simple estimation of the relative abundance of gene-modified cells from human gene therapy subjects, which has previously been lacking but is crucial for detecting expansion of cell clones that may be a prelude to adverse events.
Subject(s)
Gene Targeting , Genetic Therapy , Sequence Analysis, DNA/methods , Bacteriophage mu/genetics , Cell Line , Humans , Polymerase Chain ReactionABSTRACT
Some of the earliest studies of retroviral integration targeting reported that sites of gammaretroviral DNA integration were positively correlated with DNase I-hypersensitive sites in chromatin. This led to the suggestion that open chromatin was favorable for integration. More recent deep sequencing experiments confirmed that gammaretroviral integration sites and DNase I cleavage sites are associated in genome-wide surveys. Paradoxically, in vitro studies of integration show that nucleosomal DNA is actually favored over naked DNA, raising the question of whether integration target DNA in chromosomes is wrapped in nucleosomes or nucleosome free. In this study we examined gammaretroviral integration by infecting primary human CD4(+) T lymphocytes with a murine leukemia virus (MLV)-based retroviral vector or xenotropic murine leukemia virus-related virus (XMRV), and isolated 32,585 unique integration sites using ligation-mediated PCR and 454 pyrosequencing. CD4(+) T lymphocytes were chosen for study because of the particularly dense genome-wide mapping of chromatin features available for comparison. Analysis relative to predicted nucleosome positions showed that gammaretroviruses direct integration into outward-facing major grooves on nucleosome-wrapped DNA, similar to the integration pattern of HIV. Also, a suite of histone modifications correlated with gene activity are positively associated with integration by both MLV and XMRV. Thus, we conclude that favored integration near DNase I-hypersensitive sites does not imply that integration takes place exclusively in nucleosome-free regions.
Subject(s)
DNA, Viral/genetics , Gammaretrovirus/genetics , Nucleosomes/genetics , Virus Integration , Acetylation , CD4-Positive T-Lymphocytes/cytology , Histones/metabolism , Humans , Transduction, GeneticABSTRACT
Many viral fusion proteins are primed by proteolytic cleavage near their fusion peptides. While the coronavirus (CoV) spike (S) protein is known to be cleaved at the S1/S2 boundary, this cleavage site is not closely linked to a fusion peptide. However, a second cleavage site has been identified in the severe acute respiratory syndrome CoV (SARS-CoV) S2 domain (R797). Here, we investigated whether this internal cleavage of S2 exposes a viral fusion peptide. We show that the residues immediately C-terminal to the SARS-CoV S2 cleavage site SFIEDLLFNKVTLADAGF are very highly conserved across all CoVs. Mutagenesis studies of these residues in SARS-CoV S, followed by cell-cell fusion and pseudotyped virion infectivity assays, showed a critical role for residues L803, L804, and F805 in membrane fusion. Mutation of the most N-terminal residue (S798) had little or no effect on membrane fusion. Biochemical analyses of synthetic peptides corresponding to the proposed S2 fusion peptide also showed an important role for this region in membrane fusion and indicated the presence of alpha-helical structure. We propose that proteolytic cleavage within S2 exposes a novel internal fusion peptide for SARS-CoV S, which may be conserved across the Coronaviridae.
Subject(s)
Membrane Glycoproteins/chemistry , Membrane Glycoproteins/physiology , Severe Acute Respiratory Syndrome/virology , Severe acute respiratory syndrome-related coronavirus/chemistry , Viral Envelope Proteins/chemistry , Viral Envelope Proteins/physiology , Virus Internalization , Amino Acid Sequence , Animals , Cell Fusion , Cell Line , Humans , Membrane Glycoproteins/genetics , Molecular Sequence Data , Peptides/chemistry , Peptides/genetics , Peptides/metabolism , Protein Structure, Tertiary , Severe acute respiratory syndrome-related coronavirus/genetics , Severe acute respiratory syndrome-related coronavirus/metabolism , Sequence Alignment , Spike Glycoprotein, Coronavirus , Viral Envelope Proteins/geneticsABSTRACT
Vesicular stomatitis virus (VSV) is a prototypic virus commonly used in studies of endocytosis and membrane trafficking. One proposed mechanism for VSV entry involves initial fusion with internal vesicles of multivesicular endosomes followed by back-fusion of these vesicles into the cytoplasm. One feature of endosomal internal vesicles is that they contain the lipid bis(monoacylglycero)phosphate (BMP). Here, we show that the presence of BMP significantly increases the rate of VSV G-mediated membrane fusion. The increased fusion was selective for VSV and was not evident for another enveloped virus, influenza virus. Our data provide a biological rationale for a two-step infection reaction during VSV entry, and suggest that BMP preferentially affects the ability of VSV G to mediate lipid mixing during membrane fusion.
Subject(s)
Endosomes/metabolism , Lysophospholipids/metabolism , Membrane Fusion , Monoglycerides/metabolism , Vesicular stomatitis Indiana virus/metabolism , Animals , Cell Line , Cholesterol/chemistry , Endosomes/chemistry , Endosomes/virology , Hydrogen-Ion Concentration , Lipids/chemistry , Liposomes/chemistry , Liposomes/metabolism , Lysophospholipids/chemistry , Membrane Glycoproteins/metabolism , Monoglycerides/chemistry , Phosphatidylcholines/chemistry , Phosphatidylserines/chemistry , Viral Envelope Proteins/metabolism , Virus InternalizationABSTRACT
Realizing the therapeutic potential of human induced pluripotent stem (iPS) cells will require robust, precise and safe strategies for genetic modification, as cell therapies that rely on randomly integrated transgenes pose oncogenic risks. Here we describe a strategy to genetically modify human iPS cells at 'safe harbor' sites in the genome, which fulfill five criteria based on their position relative to contiguous coding genes, microRNAs and ultraconserved regions. We demonstrate that â¼10% of integrations of a lentivirally encoded ß-globin transgene in ß-thalassemia-patient iPS cell clones meet our safe harbor criteria and permit high-level ß-globin expression upon erythroid differentiation without perturbation of neighboring gene expression. This approach, combining bioinformatics and functional analyses, should be broadly applicable to introducing therapeutic or suicide genes into patient-specific iPS cells for use in cell therapy.
Subject(s)
Genetic Engineering/methods , Induced Pluripotent Stem Cells/metabolism , Transgenes/genetics , beta-Globins/metabolism , beta-Thalassemia/therapy , Animals , Cell Differentiation , Cell Line , Erythroid Cells/cytology , Female , Gene Expression , Genetic Therapy/methods , Genetic Vectors , Genome, Human , Humans , Induced Pluripotent Stem Cells/cytology , Lentivirus/genetics , Lentivirus/metabolism , Male , Molecular Sequence Data , Transgenes/physiology , beta-Globins/genetics , beta-Thalassemia/genetics , beta-Thalassemia/metabolismABSTRACT
Members of the Rhabdoviridae infect a wide variety of animals and plants, and are the causative agents of many important diseases. Rhabdoviruses enter host cells following internalization into endosomes, with the glycoprotein (G protein) mediating both receptor binding to host cells and fusion with the cellular membrane. The recently solved crystal structure of vesicular stomatitis virus G has allowed considerable insight into the mechanism of rhabdovirus entry, in particular the low pH-dependent conformational changes that lead to fusion activation. Rhabdovirus entry shows several distinct features compared with other enveloped viruses; first, the entry process appears to consist of two distinct fusion events, initial fusion into vesicles within endosomes followed by back-fusion into the cytosol; second, the conformational changes in the G protein that lead to fusion activation are reversible; and third, the G protein is structurally distinct from other viral fusion proteins and is not proteolytically cleaved. The internalization and fusion mechanisms of rhabdoviruses are discussed in this article, with a focus on viral systems where the G protein has been studied extensively: vesicular stomatitis virus and rabies virus, as well as viral hemorrhagic septicemia virus.
ABSTRACT
Creating one-pot synthetic routes is a challenge that is already spawning new chemistry, enzymes, materials, and mechanistic insight. Through one-pot reactions, the chemical products that add value to our lives can be produced with less waste and greater economic benefits. Within this Emerging Area, we describe models for designing one-pot reactions as well as advanced catalysts created to facilitate their realization.