Figure 2
Figure 2. APC-expressed C3 and DAF influence T-cell apoptosis after antigen stimulation. (A) Flow cytometry plots showing annexin V staining of CFSE-labeled Mar T cells on day 3 after stimulation with WT, Daf1−/−, C3−/−, or Daf1/C3−/− macrophages plus HYDby peptide. Percentages of annexin V+ cells are given in the upper left. Data are representative of 4 individual experiments. *P < .05 versus WT APCs. Similar results were found when TUNEL staining was used as a readout (Figure S2). (B) Percentage of annexin V+ polyclonal H-2b T cells on day 4 of in vitro culture with allogeneic H-2d WT, Daf1−/−, or C3−/− macrophages. Values are means plus or minus SD of 3 individual experiments. *P < .05. (C) CFSE-labeled WT or C3−/− H-2d T cells were stimulated in vitro with WT, C3−/−, or Daf1/C3−/− allogeneic H-2b macrophages for 4 days and stained with annexin V. Values are means plus or minus SD of 3 individual experiments. *P < .05 versus WT T cells. (D) Flow cytometry plots depicting annexin V+ Mar T cells in the spleens of recipient mice on day 3 after adoptive transfer (10 × 106 Mar T cells per mouse) into groups of male WT, Daf1−/−, or C3−/− recipients (n = 3 per group). *P < .05 versus WT APCs. (E) Groups of male bone marrow chimeric mice (n = 3) were injected with 5 × 106 CFSE-labeled Mar T cells and Vβ6+ splenic Mar cells were assayed for apoptosis by annexin V staining on day 3. *P < .05 versus WT→WT controls.

APC-expressed C3 and DAF influence T-cell apoptosis after antigen stimulation. (A) Flow cytometry plots showing annexin V staining of CFSE-labeled Mar T cells on day 3 after stimulation with WT, Daf1−/−, C3−/−, or Daf1/C3−/− macrophages plus HYDby peptide. Percentages of annexin V+ cells are given in the upper left. Data are representative of 4 individual experiments. *P < .05 versus WT APCs. Similar results were found when TUNEL staining was used as a readout (Figure S2). (B) Percentage of annexin V+ polyclonal H-2b T cells on day 4 of in vitro culture with allogeneic H-2d WT, Daf1−/−, or C3−/− macrophages. Values are means plus or minus SD of 3 individual experiments. *P < .05. (C) CFSE-labeled WT or C3−/− H-2d T cells were stimulated in vitro with WT, C3−/−, or Daf1/C3−/− allogeneic H-2b macrophages for 4 days and stained with annexin V. Values are means plus or minus SD of 3 individual experiments. *P < .05 versus WT T cells. (D) Flow cytometry plots depicting annexin V+ Mar T cells in the spleens of recipient mice on day 3 after adoptive transfer (10 × 106 Mar T cells per mouse) into groups of male WT, Daf1−/−, or C3−/− recipients (n = 3 per group). *P < .05 versus WT APCs. (E) Groups of male bone marrow chimeric mice (n = 3) were injected with 5 × 106 CFSE-labeled Mar T cells and Vβ6+ splenic Mar cells were assayed for apoptosis by annexin V staining on day 3. *P < .05 versus WT→WT controls.

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