DCregs generate alloreactive CD4+CD25+Foxp3+ TR cells from CD4+CD25− Foxp3− T cells in vitro. (A) CD4+CD25− T cells (2 × 105) obtained from B10.D2 mice were cultured with or without the irradiated DCs (2 × 104) obtained from BALB/c mice for 3 days, and the proliferative response was measured. The error bars indicate SD. *P < .01 compared with mDCs. Results of 4 replicated experiments were pooled. (B-D) CD4+CD25− T cells (5 × 106) obtained from B10.D2 mice were cultured with the irradiated DCs (5 × 105) obtained from BALB/c mice for 7 days, and CD4+ T cells were collected. (B,C) The expression of CD25 and Foxp3 on CD4+ T cells was analyzed by flow cytometry, and data are represented by a dot plot (B) and are expressed as% positive cells (C). The error bars indicate SD. *P < .01 compared with the CD4+ T cells primed with allogeneic mDCs by Student paired t test. Results of 4 replicated experiments were pooled. (D) CD4+CD25− T cells obtained from B10.D2 mice (5 × 104) were cultured with the irradiated mDCs (5 × 103) obtained from BALB/c mice in the presence of CD4+CD25+ T cells (6.25 × 103-5 × 104) obtained from B10.D2 mice or each culture for 3 days, and the proliferative response was measured. The error bars indicate SD. *P < .01 compared with CD4+CD25+ nTR cells by Student paired t test. Results of 4 replicated experiments were pooled. (E) CD4+CD25− T cells (106) obtained from B10.D2 mice and the irradiated DCregs (105) obtained from BALB/c mice were cocultured or placed separately in the presence or absence of anti–IL-10 mAb, anti–TGF-β mAb or control Ig for 7 days, and CD4+ T cells were collected. The expression of CD25 and Foxp3 on CD4+ T cells was analyzed by flow cytometry, and data are expressed as percentage of cells positive for both CD25 and Foxp3. The error bars indicate SD. *P < .01 compared with the primed CD4+ T cells primed with allogeneic DCregs by Student paired t test. Results of 3 replicated experiments were pooled.