an initial in vitro investigation into the potential therapeutic use of supt1 cells to prevent aids in hiv-seropositive individuals体外初步调查的潜在治疗用途supt1细胞在hiv-seropositive个人预防艾滋病.pdfVIP
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an initial in vitro investigation into the potential therapeutic use of supt1 cells to prevent aids in hiv-seropositive individuals体外初步调查的潜在治疗用途supt1细胞在hiv-seropositive个人预防艾滋病
An Initial In Vitro Investigation into the Potential
Therapeutic Use of SupT1 Cells to Prevent AIDS in HIV-
Seropositive Individuals
Jonathan Fior*
Section of Infectious Diseases and Immunopathology, Department of Clinical Sciences, Luigi Sacco Hospital, University of Milan, Milan, Italy
Abstract
HIV infection usually leads to a progressive decline in number and functionality of CD4+ T lymphocytes, resulting in AIDS
development. In this study, I investigated the strategy of using inoculated SupT1 cells to move infection from HIV-1 X4
strains toward the inoculated cells, which should theoretically prevent infection and depletion of normal CD4+ T cells,
preventing the development of AIDS-related pathologies. Interestingly, the persistent in vitro replication in SupT1 cells
renders the virus less cytopathic and more sensitive to antibody-mediated neutralization, suggesting that replication of
the virus in the inoculated SupT1 cells may have a vaccination effect in the long run. In order to mimic the scenario of a
therapy in which SupT1 cells are inoculated in an HIV-seropositive patient, I used infected SupT1/PBMC cocultures and a
series of control experiments. Infections were done with equal amounts of the wild type HIV-1 LAI virus. The SupT1
CD4+CD8+ T cell population was distinguished from the PBMC CD4+CD8 2 T cell population by FACS analysis. The results
of this study show that the virus-mediated killing of primary CD4+ T cells in the SupT1/PBMC cocultures was significantly
delayed, suggesting that the preferential infection of SupT1 cells can induce the virus to spare primary CD4+ T cells from
infection and depletion. The preferential infection of SupT1 cells can be explained by the higher viral tropism for the
SupT1 cell line. In conclusion, this study demonstrates that it’s possible in an in vitro system to use Su
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