Figure 7
Figure 7. Reversal of Treg-induced senescence by TLR8 ligand and MAPK inhibitors in vivo. (A) Colocalization of adoptively transferred naive CD8+ T cells and CD4+CD25hiFoxP3+ Treg cells in Rag1−/− mice. Naive CD8+ T cells (5 × 106/mouse) and CD4+CD25hiFoxP3+ Treg cells (5 × 106/mouse) were injected intravenously into Rag1−/− mice. Blood, lymph nodes (LN), and spleens (SP) were harvested from the mice on days 1 and 2 after injection. Cells were purified and analyzed for CD4+ and CD8+ T-cell populations using FACS with anti–human CD4 and CD8 Abs. (B) Increased SA-β-Gal+ cell populations were induced markedly in naive CD8+ T cells after cotransfer with CD4+CD25hiFoxP3+ Treg cells, whereas cotransfer with CD4+CD25− T cells did not induce increased senescent CD8+ T cells. (C) The purified CD8+ T cells cotransferred with CD4+CD25hiFoxP3+ Treg cells had potent suppressive activity on the proliferation of responding CD4+ T cells. Naive CD8+ T cells (5 × 106/mouse), CD4+CD25hiFoxP3+ Treg cells (3 × 106/mouse), and CD4+CD25− T cells (3 × 106/mouse) were preactivated with anti-CD3 Ab and adoptively cotransferred into Rag1−/− mice. Blood, lymph nodes, and spleens were harvested at 12 days after injection. The transferred human CD8+ T cells were isolated for subsequent SA-β-Gal staining (B) and 3H-thymidine incorporation (C) assays. *P < .05 and **P < .01 compared with the groups cotransferred with CD4+CD25− T cells or alone. (D-E) Pretreatment of CD4+CD25hiFoxP3+ Treg cells with poly-G3 or naive T cells with ERK and p38 inhibitors before coinjection was able to block significantly the induction of senescence and reverse the suppressive activity in transferred naive CD8+ T cells. Naive CD8+ T cells were pretreated with ERK and p38 inhibitors and/or CD4+CD25hiFoxp3+ Treg were pretreated with poly-G3 or poly-T3 (control) for 2 days before cotransfer. The transferred human CD8+ T cells in different organs were isolated at 12 days after injection for subsequent SA-β-Gal staining (D) and 3H-thymidine incorporation (E) assays. *P < .05 and **P < .01 compared with the medium-only and poly-T3 groups.

Reversal of Treg-induced senescence by TLR8 ligand and MAPK inhibitors in vivo. (A) Colocalization of adoptively transferred naive CD8+ T cells and CD4+CD25hiFoxP3+ Treg cells in Rag1−/− mice. Naive CD8+ T cells (5 × 106/mouse) and CD4+CD25hiFoxP3+ Treg cells (5 × 106/mouse) were injected intravenously into Rag1−/− mice. Blood, lymph nodes (LN), and spleens (SP) were harvested from the mice on days 1 and 2 after injection. Cells were purified and analyzed for CD4+ and CD8+ T-cell populations using FACS with anti–human CD4 and CD8 Abs. (B) Increased SA-β-Gal+ cell populations were induced markedly in naive CD8+ T cells after cotransfer with CD4+CD25hiFoxP3+ Treg cells, whereas cotransfer with CD4+CD25 T cells did not induce increased senescent CD8+ T cells. (C) The purified CD8+ T cells cotransferred with CD4+CD25hiFoxP3+ Treg cells had potent suppressive activity on the proliferation of responding CD4+ T cells. Naive CD8+ T cells (5 × 106/mouse), CD4+CD25hiFoxP3+ Treg cells (3 × 106/mouse), and CD4+CD25 T cells (3 × 106/mouse) were preactivated with anti-CD3 Ab and adoptively cotransferred into Rag1−/− mice. Blood, lymph nodes, and spleens were harvested at 12 days after injection. The transferred human CD8+ T cells were isolated for subsequent SA-β-Gal staining (B) and 3H-thymidine incorporation (C) assays. *P < .05 and **P < .01 compared with the groups cotransferred with CD4+CD25 T cells or alone. (D-E) Pretreatment of CD4+CD25hiFoxP3+ Treg cells with poly-G3 or naive T cells with ERK and p38 inhibitors before coinjection was able to block significantly the induction of senescence and reverse the suppressive activity in transferred naive CD8+ T cells. Naive CD8+ T cells were pretreated with ERK and p38 inhibitors and/or CD4+CD25hiFoxp3+ Treg were pretreated with poly-G3 or poly-T3 (control) for 2 days before cotransfer. The transferred human CD8+ T cells in different organs were isolated at 12 days after injection for subsequent SA-β-Gal staining (D) and 3H-thymidine incorporation (E) assays. *P < .05 and **P < .01 compared with the medium-only and poly-T3 groups.

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