Figure 5.
CD8+CD25+ thymocytes do not proliferate in MLCs and suppress the proliferation in MLCs of CD4+CD25- thymocytes via a contact-dependent mechanism. (A) Proliferative response of purified CD4+CD25-, CD4+CD25+, CD8+CD25-, or CD8+CD25+ human thymocytes to allogeneic stimulation. On day 5, cells were harvested and their proliferation assessed by measuring 3H-TdR uptake. Mean values (± SD) obtained in 9 separate experiments are reported. (B) Suppression by CD4+CD25+ or CD8+CD25+ thymocytes, but not by CD8+CD25- thymocytes, of the proliferative response of autologous CD4+CD25- thymocytes to allogeneic T-cell-depleted PBMNCs. On day 5, cells were harvested and proliferation assessed by measuring 3H-TdR uptake. Mean values (± SD) obtained in 9 separate experiments are reported. (C) Cell contact dependency of suppressive activity exerted by CD8+CD25+ thymocytes. CD4+CD25- thymocytes were stimulated with irradiated T-cell-depleted allogeneic PBMNCs in the lower chamber of a transwell plate in the absence or presence of CD8+CD25+ thymocytes, which were placed in the same chamber or in the top chamber. CD8+CD25+ thymocytes placed in the upper chamber were cultured in medium alone or stimulated with 106 irradiated T-cell-depleted allogeneic PBMNCs in the presence or absence of 5 × 105 CD4+CD25- cells. On day 5, cells present in the bottom chamber were harvested and their proliferation assessed by measuring 3H-TdR uptake. The mean values (± SD) obtained in 4 separate experiments are reported. *P < .01.

CD8+CD25+ thymocytes do not proliferate in MLCs and suppress the proliferation in MLCs of CD4+CD25- thymocytes via a contact-dependent mechanism. (A) Proliferative response of purified CD4+CD25-, CD4+CD25+, CD8+CD25-, or CD8+CD25+ human thymocytes to allogeneic stimulation. On day 5, cells were harvested and their proliferation assessed by measuring 3H-TdR uptake. Mean values (± SD) obtained in 9 separate experiments are reported. (B) Suppression by CD4+CD25+ or CD8+CD25+ thymocytes, but not by CD8+CD25- thymocytes, of the proliferative response of autologous CD4+CD25- thymocytes to allogeneic T-cell-depleted PBMNCs. On day 5, cells were harvested and proliferation assessed by measuring 3H-TdR uptake. Mean values (± SD) obtained in 9 separate experiments are reported. (C) Cell contact dependency of suppressive activity exerted by CD8+CD25+ thymocytes. CD4+CD25- thymocytes were stimulated with irradiated T-cell-depleted allogeneic PBMNCs in the lower chamber of a transwell plate in the absence or presence of CD8+CD25+ thymocytes, which were placed in the same chamber or in the top chamber. CD8+CD25+ thymocytes placed in the upper chamber were cultured in medium alone or stimulated with 106 irradiated T-cell-depleted allogeneic PBMNCs in the presence or absence of 5 × 105 CD4+CD25- cells. On day 5, cells present in the bottom chamber were harvested and their proliferation assessed by measuring 3H-TdR uptake. The mean values (± SD) obtained in 4 separate experiments are reported. *P < .01.

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