Figure 3
Significant increase in transcription frequency and intracellular protein expression of FoxP3 after allo-BMT using Cav-1−/− T cells. (A) BALB/c BM-derived DCs were irradiated with 40 Gy and cocultured with isolated WT or Cav-1−/− T cells (n = 4 per group). After 2 days of coculture, cells were harvested and applied to CD11c depletion. The CD11c− T-cell fraction was then further analyzed for differentially transcribed genes by microarray analysis. The RMA was calculated (mean ± SEM). (B) The RMA values for FoxP3 are selectively displayed (n = 4 per group). (C) BALB/c recipient mice were irradiated with a total of 9 Gy and subsequently transplanted with 5 × 106 BM plus 3 × 105 WT or Cav-1−/− T cells. Recipients were euthanized 7 days post–allo-BMT and analyzed by flow cytometry, using specific staining against CD4 and FoxP3. Relative Treg proportions of all CD4+ T cells in the spleen are shown (mean ± SEM; Cav-1+/+, n = 12 and Cav-1−/−, n = 14) (left). Absolute Treg numbers in the spleen are displayed (mean ± SEM; Cav-1+/+, n = 6 and Cav-1−/−, n = 6) (right). (D) Cav-1 expression in Treg cells was analyzed at day 7 after BMT. Teffs were obtained from sort-purified naive CD4+CD25−CD127+CD45RA+ T cells that have been stimulated with anti–CD3-loaded KT64/86 and expanded 7 to 8 days in vitro. The MFI was normalized to the value obtained for Treg cells derived from untreated WT mice. The dotted line indicates the background MFI for Cav-1 that is detected in Cav-1−/− Treg cells. RMA, robust multi-array average; stim, stimulated. *P < .05; ***P < .001.

Significant increase in transcription frequency and intracellular protein expression of FoxP3 after allo-BMT using Cav-1−/− T cells. (A) BALB/c BM-derived DCs were irradiated with 40 Gy and cocultured with isolated WT or Cav-1−/− T cells (n = 4 per group). After 2 days of coculture, cells were harvested and applied to CD11c depletion. The CD11c T-cell fraction was then further analyzed for differentially transcribed genes by microarray analysis. The RMA was calculated (mean ± SEM). (B) The RMA values for FoxP3 are selectively displayed (n = 4 per group). (C) BALB/c recipient mice were irradiated with a total of 9 Gy and subsequently transplanted with 5 × 106 BM plus 3 × 105 WT or Cav-1−/− T cells. Recipients were euthanized 7 days post–allo-BMT and analyzed by flow cytometry, using specific staining against CD4 and FoxP3. Relative Treg proportions of all CD4+ T cells in the spleen are shown (mean ± SEM; Cav-1+/+, n = 12 and Cav-1−/−, n = 14) (left). Absolute Treg numbers in the spleen are displayed (mean ± SEM; Cav-1+/+, n = 6 and Cav-1−/−, n = 6) (right). (D) Cav-1 expression in Treg cells was analyzed at day 7 after BMT. Teffs were obtained from sort-purified naive CD4+CD25CD127+CD45RA+ T cells that have been stimulated with anti–CD3-loaded KT64/86 and expanded 7 to 8 days in vitro. The MFI was normalized to the value obtained for Treg cells derived from untreated WT mice. The dotted line indicates the background MFI for Cav-1 that is detected in Cav-1−/− Treg cells. RMA, robust multi-array average; stim, stimulated. *P < .05; ***P < .001.

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