Figure 1.
Figure 1. Autologous fibroblasts infected with AD169 or RV798 can be used as stimulator cells to quantitate CMV-specific CD8+ T cells by cytokine flow cytometry. Fibroblasts were infected with AD169 or RV798 for 4, 16, 24, and 48 hours and then used to stimulate autologous PBMCs or whole blood in a CFC assay. CD8+ T cells that produced IFNγ were identified within the lymphocyte gate (based on forward/side scatter) by 2-color staining with anti-CD8 and anti–IFNγ monoclonal antibodies. The data shown are the results for donor 1 and are representative of the results obtained in 5 donors. (A) Frequency of CD8+ T cells induced to produce IFNγ after stimulation with mock-infected fibroblasts. (B) Frequency of CD8+ T cells induced to produce IFNγ after stimulation with fibroblasts infected with AD169 for various times. (C) Frequency of CD8+ T cells induced to produce IFNγ after stimulation with fibroblasts infected with RV798 for various times.

Autologous fibroblasts infected with AD169 or RV798 can be used as stimulator cells to quantitate CMV-specific CD8+ T cells by cytokine flow cytometry. Fibroblasts were infected with AD169 or RV798 for 4, 16, 24, and 48 hours and then used to stimulate autologous PBMCs or whole blood in a CFC assay. CD8+ T cells that produced IFNγ were identified within the lymphocyte gate (based on forward/side scatter) by 2-color staining with anti-CD8 and anti–IFNγ monoclonal antibodies. The data shown are the results for donor 1 and are representative of the results obtained in 5 donors. (A) Frequency of CD8+ T cells induced to produce IFNγ after stimulation with mock-infected fibroblasts. (B) Frequency of CD8+ T cells induced to produce IFNγ after stimulation with fibroblasts infected with AD169 for various times. (C) Frequency of CD8+ T cells induced to produce IFNγ after stimulation with fibroblasts infected with RV798 for various times.

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