Figure 6
Target Ags must be expressed on the same cell to observe bystander immunosuppression. (A) RNA encoding the A2-SC9 TCRs was transfected into Tregs, and the ability of these cells to bind A2-SC9 tetramer was measured the following day by flow cytometry. (B) Same as panel A except TCR encoding RNA was not added before the transfection (mock control). (C) RNA encoding the A2-SL9 TCRs was transfected into a mixture of CD4 and CD8 Teffs, and the ability of these cells to bind A2-SL9 tetramer was measured the following day by flow cytometry. (D) Same as panel C except TCR encoding RNA was not added before the transfection (mock control). (E) A2-SL9 Teffs were mixed with the indicated ratios of mock-transfected, polyclonal Tregs. These T-cell mixtures were then incubated with an equal number of K.A2.SL9 and K.A2.NY-ESO aAPCs. The final ratio of T cells to aAPCs was 1. (F) A2-SL9 Teffs were mixed with the indicated ratios of A2-SC9–transfected Tregs. These T-cell mixtures were then incubated with an equal number of K.A2.SL9 and K.A2.NY-ESO aAPCs. The final ratio of T cells to aAPCs was 1. (G) A2-SL9 Teffs were mixed with the indicated ratios of mock-transfected, polyclonal Tregs. These T-cell mixtures were then incubated with an equal number of K.A2.SL9.NY-ESO aAPCs. The final ratio of T cells to aAPCs was 1. (H) A2-SL9 effectors were mixed with the indicated ratios of A2-SC9–transfected Tregs. These T-cell mixtures were then incubated with an equal number of K.A2.SL9.NY-ESO aAPCs. The final ratio of T cells to aAPCs was 1. A cartoon denoting the cell mixtures is displayed below each data panel. The percent suppression was calculated as described in “In vitro suppression assay.” A negative value indicates that more cell divisions were measured in these conditions relative to the control without Tregs.

Target Ags must be expressed on the same cell to observe bystander immunosuppression. (A) RNA encoding the A2-SC9 TCRs was transfected into Tregs, and the ability of these cells to bind A2-SC9 tetramer was measured the following day by flow cytometry. (B) Same as panel A except TCR encoding RNA was not added before the transfection (mock control). (C) RNA encoding the A2-SL9 TCRs was transfected into a mixture of CD4 and CD8 Teffs, and the ability of these cells to bind A2-SL9 tetramer was measured the following day by flow cytometry. (D) Same as panel C except TCR encoding RNA was not added before the transfection (mock control). (E) A2-SL9 Teffs were mixed with the indicated ratios of mock-transfected, polyclonal Tregs. These T-cell mixtures were then incubated with an equal number of K.A2.SL9 and K.A2.NY-ESO aAPCs. The final ratio of T cells to aAPCs was 1. (F) A2-SL9 Teffs were mixed with the indicated ratios of A2-SC9–transfected Tregs. These T-cell mixtures were then incubated with an equal number of K.A2.SL9 and K.A2.NY-ESO aAPCs. The final ratio of T cells to aAPCs was 1. (G) A2-SL9 Teffs were mixed with the indicated ratios of mock-transfected, polyclonal Tregs. These T-cell mixtures were then incubated with an equal number of K.A2.SL9.NY-ESO aAPCs. The final ratio of T cells to aAPCs was 1. (H) A2-SL9 effectors were mixed with the indicated ratios of A2-SC9–transfected Tregs. These T-cell mixtures were then incubated with an equal number of K.A2.SL9.NY-ESO aAPCs. The final ratio of T cells to aAPCs was 1. A cartoon denoting the cell mixtures is displayed below each data panel. The percent suppression was calculated as described in “In vitro suppression assay.” A negative value indicates that more cell divisions were measured in these conditions relative to the control without Tregs.

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