Figure 2.
Figure 2. CD8+ T cells from male H-Y mice possess a high activation threshold due to a defect in TCR signal transduction. (A) Purified CD8+ T cells (1 × 104) from female H-2b H-Y (CD8hi), male H-2b H-Y (CD8lo), or male H-2b/d H-Y (CD8int) mice were cultured with irradiated B6-Tap-1-/- splenocytes (5 × 105) ± IL-2 and the indicated concentration of H-Y peptide. Proliferation was determined after 3 days, and the error bars represent the standard deviation of triplicate cultures. (B) Western blot analysis of CD8hi, CD8int, and CD8lo cells immediately ex vivo or after stimulation for 10 minutes with anti-CD3 (10 μg/mL) or PMA (25 ng/mL) and ionomycin (500 ng/mL). Blots were probed with antiphospho-ZAP-70 and phospho-ERK and then stripped and reprobed with antibodies to unphosphorylated ZAP-70 and ERK2.

CD8+ T cells from male H-Y mice possess a high activation threshold due to a defect in TCR signal transduction. (A) Purified CD8+ T cells (1 × 104) from female H-2b H-Y (CD8hi), male H-2b H-Y (CD8lo), or male H-2b/d H-Y (CD8int) mice were cultured with irradiated B6-Tap-1-/- splenocytes (5 × 105) ± IL-2 and the indicated concentration of H-Y peptide. Proliferation was determined after 3 days, and the error bars represent the standard deviation of triplicate cultures. (B) Western blot analysis of CD8hi, CD8int, and CD8lo cells immediately ex vivo or after stimulation for 10 minutes with anti-CD3 (10 μg/mL) or PMA (25 ng/mL) and ionomycin (500 ng/mL). Blots were probed with antiphospho-ZAP-70 and phospho-ERK and then stripped and reprobed with antibodies to unphosphorylated ZAP-70 and ERK2.

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