Figure 6
Figure 6. Short-term activation of allogeneic T cells with a CD28-SA in vitro protects from aGVHD while maintaining GVT activity. (A) Increased frequencies and (B) activated phenotype of Foxp3+ Treg cells after CD28-SA stimulation of whole LN cells in vitro. Numbers represent the percentages of Foxp3+ cells as indicated by the marker. (C) Lethally irradiated BALB/c mice were reconstituted with 107 C57BL/6 TCD BM cells either alone or together with 5 × 105 CD4+ or 4 × 105 Treg cell–depleted CD4+ cells (n = 10) characterized in panel A. P values compare (C) survival curves or (D) clinical scores from animals after transfer of cultured CD4+ cells versus Treg cell–depleted CD4+ cells. Data from 2 individual experiments were pooled. BALB/c recipient mice received BCL1 lymphoma cells followed by TCD BM cells only or TCD BM cells together with either (E) 5 × 105 or (F) 5 × 104 fresh T cells or the same numbers of T cells isolated from whole LN cell cultures stimulated in vitro with a CD28-SA for 4 days. Data from 2 experiments were pooled (n = 12; 5 × 104 T cells [fresh], n = 11), and P values were obtained comparing T-cell recipients with the TCD BM only group. Numbers in parentheses indicate animals with end-stage lymphoma/animals analyzed).

Short-term activation of allogeneic T cells with a CD28-SA in vitro protects from aGVHD while maintaining GVT activity. (A) Increased frequencies and (B) activated phenotype of Foxp3+ Treg cells after CD28-SA stimulation of whole LN cells in vitro. Numbers represent the percentages of Foxp3+ cells as indicated by the marker. (C) Lethally irradiated BALB/c mice were reconstituted with 107 C57BL/6 TCD BM cells either alone or together with 5 × 105 CD4+ or 4 × 105 Treg cell–depleted CD4+ cells (n = 10) characterized in panel A. P values compare (C) survival curves or (D) clinical scores from animals after transfer of cultured CD4+ cells versus Treg cell–depleted CD4+ cells. Data from 2 individual experiments were pooled. BALB/c recipient mice received BCL1 lymphoma cells followed by TCD BM cells only or TCD BM cells together with either (E) 5 × 105 or (F) 5 × 104 fresh T cells or the same numbers of T cells isolated from whole LN cell cultures stimulated in vitro with a CD28-SA for 4 days. Data from 2 experiments were pooled (n = 12; 5 × 104 T cells [fresh], n = 11), and P values were obtained comparing T-cell recipients with the TCD BM only group. Numbers in parentheses indicate animals with end-stage lymphoma/animals analyzed).

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