Role of human immunodeficiency virus replication in defective in vitro growth of hematopoietic progenitors

  • F Louache
    INSERM U. 91, CNRS UA 607, Hopital Henri Mondor, Creteil, France.
  • A Henri
    INSERM U. 91, CNRS UA 607, Hopital Henri Mondor, Creteil, France.
  • A Bettaieb
    INSERM U. 91, CNRS UA 607, Hopital Henri Mondor, Creteil, France.
  • E Oksenhendler
    INSERM U. 91, CNRS UA 607, Hopital Henri Mondor, Creteil, France.
  • G Raguin
    INSERM U. 91, CNRS UA 607, Hopital Henri Mondor, Creteil, France.
  • M Tulliez
    INSERM U. 91, CNRS UA 607, Hopital Henri Mondor, Creteil, France.
  • W Vainchenker
    INSERM U. 91, CNRS UA 607, Hopital Henri Mondor, Creteil, France.

書誌事項

公開日
1992-12-15
DOI
  • 10.1182/blood.v80.12.2991.2991
公開者
American Society of Hematology

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説明

<jats:title>Abstract</jats:title> <jats:p>A number of hematologic abnormalities, including cytopenias, have been observed in patients with human immunodeficiency virus (HIV) infection. To elucidate their mechanisms, a group of 27 patients with HIV-1 infection was studied. In all patients, a marked reduction of in vitro colony formation by erythroid, granulomacrophagic, and megakaryocytic bone marrow progenitors was observed in comparison to normal donors. HIV-1 infection of marrow progenitors was investigated in studying individual colonies with the polymerase chain reaction (PCR) technique. No HIV-1 DNA could be detected in these colonies, suggesting either that marrow progenitors were not infected or that infected progenitors were not able to generate colonies in vitro. The addition of antisense oligonucleotides directed against HIV tat or nef sequences in the culture medium led to a significant increase in colony formation, suggesting that HIV replication in hematopoietic progenitors could be responsible for their defective growth. However, no HIV-1-infected colonies could be detected by PCR after the antisense treatment, indicating that the increase in colony number was not due to the proliferation and differentiation of infected progenitors but to an inhibition of HIV replication in an accessory cell. This last hypothesis was further confirmed by the absence of effects of antisense oligomers on the plating efficiency of hematopoietic progenitors grown from CD34+ cells. These data indicate that hematologic abnormalities of HIV-infected patients cannot be explained by a direct infection of hematopoietic progenitor cells and suggest that a defective modulation of progenitor cell growth by HIV replication outside these cells might play a role in these abnormalities.</jats:p>

収録刊行物

  • Blood

    Blood 80 (12), 2991-2999, 1992-12-15

    American Society of Hematology

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