Literature DB >> 23115284

Comprehensive mutational analysis reveals p6Gag phosphorylation to be dispensable for HIV-1 morphogenesis and replication.

Benjamin Radestock1, Ivonne Morales, Sheikh Abdul Rahman, Sonja Radau, Bärbel Glass, René Peiman Zahedi, Barbara Müller, Hans-Georg Kräusslich.   

Abstract

The structural polyprotein Gag of human immunodeficiency virus type 1 (HIV-1) is necessary and sufficient for formation of virus-like particles. Its C-terminal p6 domain harbors short peptide motifs that facilitate virus release from the plasma membrane and mediate incorporation of the viral Vpr protein. p6 has been shown to be the major viral phosphoprotein in HIV-1-infected cells and virions, but the sites and functional relevance of p6 phosphorylation are not clear. Here, we identified phosphorylation of several serine and threonine residues in p6 in purified virus preparations using mass spectrometry. Mutation of individual candidate phosphoacceptor residues had no detectable effect on virus assembly, release, and infectivity, however, suggesting that phosphorylation of single residues may not be functionally relevant. Therefore, a comprehensive mutational analysis was conducted changing all potentially phosphorylatable amino acids in p6, except for a threonine that is part of an essential peptide motif. To avoid confounding changes in the overlapping pol reading frame, mutagenesis was performed in a provirus with genetically uncoupled gag and pol reading frames. An HIV-1 derivative carrying 12 amino acid changes in its p6 region, abolishing all but one potential phosphoacceptor site, showed no impairment of Gag assembly and virus release and displayed only very subtle deficiencies in viral infectivity in T-cell lines and primary lymphocytes. All mutations were stable over 2 weeks of culture in primary cells. Based on these findings, we conclude that phosphorylation of p6 is dispensable for HIV-1 assembly, release, and infectivity in tissue culture.

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Year:  2012        PMID: 23115284      PMCID: PMC3554071          DOI: 10.1128/JVI.02162-12

Source DB:  PubMed          Journal:  J Virol        ISSN: 0022-538X            Impact factor:   5.103


  48 in total

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Authors:  W J Godinez; M Lampe; S Wörz; B Müller; R Eils; K Rohr
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5.  Proteomic analysis of the yeast mitochondrial outer membrane reveals accumulation of a subclass of preproteins.

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6.  Highly selective enrichment of phosphorylated peptides from peptide mixtures using titanium dioxide microcolumns.

Authors:  Martin R Larsen; Tine E Thingholm; Ole N Jensen; Peter Roepstorff; Thomas J D Jørgensen
Journal:  Mol Cell Proteomics       Date:  2005-04-27       Impact factor: 5.911

7.  Double-labelled HIV-1 particles for study of virus-cell interaction.

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8.  Solution structure of the human immunodeficiency virus type 1 p6 protein.

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Journal:  J Biol Chem       Date:  2005-10-17       Impact factor: 5.157

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Authors:  Lars-Anders Carlson; John A G Briggs; Bärbel Glass; James D Riches; Martha N Simon; Marc C Johnson; Barbara Müller; Kay Grünewald; Hans-Georg Kräusslich
Journal:  Cell Host Microbe       Date:  2008-12-11       Impact factor: 21.023

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  14 in total

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Journal:  J Virol       Date:  2015-07-15       Impact factor: 5.103

2.  The nucleocapsid domain of Gag is dispensable for actin incorporation into HIV-1 and for association of viral budding sites with cortical F-actin.

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3.  Phosphorylation Requirement of Murine Leukemia Virus p12.

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4.  Mass spectrometry-based proteomic approaches for discovery of HIV-host interactions.

Authors:  Yang Luo; Mark A Muesing
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5.  Re-visiting the functional Relevance of the highly conserved Serine 40 Residue within HIV-1 p6(Gag).

Authors:  Benjamin Radestock; Robin Burk; Barbara Müller; Hans-Georg Kräusslich
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6.  The phosphorylation of HIV-1 Gag by atypical protein kinase C facilitates viral infectivity by promoting Vpr incorporation into virions.

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7.  Mutation of the highly conserved Ser-40 of the HIV-1 p6 gag protein to Phe causes the formation of a hydrophobic patch, enhances membrane association, and polyubiquitination of Gag.

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8.  Proteolysis of mature HIV-1 p6 Gag protein by the insulin-degrading enzyme (IDE) regulates virus replication in an Env-dependent manner.

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9.  HIV-1 Gag Recruits Oligomeric Vpr via Two Binding Sites in p6, but Both Mature p6 and Vpr Are Rapidly Lost upon Target Cell Entry.

Authors:  Madushi Wanaguru; Kate N Bishop
Journal:  J Virol       Date:  2021-08-10       Impact factor: 5.103

10.  Glutamic Acid Residues in HIV-1 p6 Regulate Virus Budding and Membrane Association of Gag.

Authors:  Melanie Friedrich; Christian Setz; Friedrich Hahn; Alina Matthaei; Kirsten Fraedrich; Pia Rauch; Petra Henklein; Maximilian Traxdorf; Torgils Fossen; Ulrich Schubert
Journal:  Viruses       Date:  2016-04-25       Impact factor: 5.048

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