Fig. 4.
Fig. 4. Selectivity of Fas-mediated apoptosis in cultures of lymphocytes from HIV-1–infected patients. (A) Fas-related apoptosis of CD4+ cells in culture of lymphocytes from patients with HIV-1 infection. Samples of lymphocytes from HIV-1–infected patients were untreated (ø) or cocultivated with CH11 MoAb (F ) for 3 days. The number of apoptotic cells were determined using two-color flow cytometry. Apoptotic cells were detected using TdT reaction; phenotype of cells was determined using CD4 or CD8 MoAb. Cells were gated to include only either CD4+ or CD8+ cells. The standard deviation of the mean is seen in brackets. (B) CD4/CD8 ratio of lymphocytes cocultivated with CH11 MoAb. Samples of PBMCs from the HIV-1–infected patients who were either untreated or cocultivated with CH11 MoAb. Columns represent the CD4+/CD8+ ratio of untreated (ø) and CH11-treated cells (F ). The standard deviation of the mean is shown in brackets.

Selectivity of Fas-mediated apoptosis in cultures of lymphocytes from HIV-1–infected patients. (A) Fas-related apoptosis of CD4+ cells in culture of lymphocytes from patients with HIV-1 infection. Samples of lymphocytes from HIV-1–infected patients were untreated (ø) or cocultivated with CH11 MoAb (F ) for 3 days. The number of apoptotic cells were determined using two-color flow cytometry. Apoptotic cells were detected using TdT reaction; phenotype of cells was determined using CD4 or CD8 MoAb. Cells were gated to include only either CD4+ or CD8+ cells. The standard deviation of the mean is seen in brackets. (B) CD4/CD8 ratio of lymphocytes cocultivated with CH11 MoAb. Samples of PBMCs from the HIV-1–infected patients who were either untreated or cocultivated with CH11 MoAb. Columns represent the CD4+/CD8+ ratio of untreated (ø) and CH11-treated cells (F ). The standard deviation of the mean is shown in brackets.

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