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      HIV-1 Vpr interacts with the nuclear transport pathway to promote macrophage infection.

      Genes & development
      Cell Nucleus, metabolism, virology, Cells, Cultured, Fluorescent Antibody Technique, Indirect, G2 Phase, genetics, Gene Products, vpr, physiology, HIV-1, pathogenicity, HeLa Cells, Humans, Macrophages, Nuclear Envelope, Nuclear Proteins, Point Mutation, RNA, Messenger, analysis, T-Lymphocytes, Yeasts, alpha Karyopherins, beta Karyopherins, vpr Gene Products, Human Immunodeficiency Virus

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          Abstract

          HIV-1 Vpr promotes nuclear entry of viral nucleic acids in nondividing macrophages and also causes a G2 cell-cycle arrest. Consistent with its role in nuclear transport, we show Vpr localizes to the nuclear envelope in both human and yeast cells. Like the importin-beta subunit of the nuclear import receptor, Vpr also interacts with the yeast importin-alpha subunit and nucleoporins. Moreover, overexpression of either Vpr or importin-beta in yeast blocks nuclear transport of mRNAs. A mutant form of Vpr (Vpr F34I) that does not localize at the nuclear envelope, or bind to importin-alpha and nucleoporins, renders HIV-1 incapable of infecting macrophages efficiently. Vpr F34I, however, still causes a G2 arrest, demonstrating that the dual functions of Vpr are genetically separable. Our data suggest Vpr functionally resembles importin-beta in nuclear import of the HIV-1 pre-integration complex and this function is essential for the role of Vpr in macrophage infection, but not G2 arrest.

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