Fig. 6.
Fig. 6. Abolition of CTL activity in pfp−/− mice. CTL activity was determined by 51Cr release assay. (A) Equal numbers of splenic T cells from a 6-day primary MLR (B6 anti-B6D2F1) were used as effectors. (B) Splenocytes from day 7 posttransplant (n = 5/group) were counted, and equal numbers of T cells (CD4+ plus CD8+ cells adjusted according to FACS analysis) were used as effectors.51Cr-labeled p815 targets (H-2d) were coincubated with effectors for 4 hours, and 51Cr in the supernatants was determined by a γ-scintillation counter.

Abolition of CTL activity in pfp−/− mice. CTL activity was determined by 51Cr release assay. (A) Equal numbers of splenic T cells from a 6-day primary MLR (B6 anti-B6D2F1) were used as effectors. (B) Splenocytes from day 7 posttransplant (n = 5/group) were counted, and equal numbers of T cells (CD4+ plus CD8+ cells adjusted according to FACS analysis) were used as effectors.51Cr-labeled p815 targets (H-2d) were coincubated with effectors for 4 hours, and 51Cr in the supernatants was determined by a γ-scintillation counter.

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