![Figure 3. Rras−/− splenic APCs and BM-DCs show impaired T-cell proliferation capacity. (A) Bulk splenic APCs (129Sv; n = 3) or (B) splenic DCs (129Sv; n = 4) from Rras+/+ or Rras−/− mice in different ratios were comixed with 2 × 105 T cells from WT Balb/c for 96 hours. Allogeneic T-cell proliferation was measured by adding [H3]-labeled thymidine for the last 16 hours, and the amount of incorporation was measured by a scintillation counter. Results represent triplicate measurements from a single experiment with data in panel A reproduced in 2 additional experiments. (C) A similar proliferation assay using WT T cells was conducted as in panels A and B, except that BM-DCs (129Sv) were used. Bars represent SD. (D) In vivo T-cell proliferation assays were performed. Rras+/+ or Rras−/− mice (129Sv) were injected intraperitoneally with PBS, 10 μg LPS, or 10 μg LPS and 1 mg OVA. Six hours after injection, splenic DCs were isolated and comixed with naive CFSE-labeled polyclonal syngeneic splenic T cells (129Sv) for 96 hours. CFSE+ staining was analyzed by flow cytometry to measure T-cell proliferation. All plots are gated for TCR+CD4+ cells. (E) Percentages from panel D for CFSE+ proliferating T cells are plotted. Results represent data from 2 independent experiments with Rras+/+ (n = 5) and Rras−/− (n = 6) mice. Bars represent median. ***P < .0005.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/119/7/10.1182_blood-2011-05-357319/4/zh89991185620003.jpeg?Expires=1724250738&Signature=Jgrn1ee9Pn99LGBnzBQwgnGdcuNODsGtDE6aGgcT0LMoFKCXAWAgRk3Cz2xktZbIBpW~uyyD2UBF8TW5O8bquu4IPZZ1GMUpDs2qRt3iIwruDmksvVmX1J~b2TM48VqZYFmyQPAVn8VJ4H3hxYXTcbJ6nbMcdi6G~JIDDD92OFV8lKPT4jKE358cktf0I1Gag8ZNgbHmsWKqzdNKbZ2I38BrFt0bbpE5y-df5MvL3mm98CmsgiKV626YO2BRtfSHwo7SYsn4UQzuisy6Te~xwcUD5GJkBeSXyaiGiYV85kb5zWgDrm1E3UxNCiYrIvBIFd8jqXVHvigelADUfrfnZw__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Rras−/− splenic APCs and BM-DCs show impaired T-cell proliferation capacity. (A) Bulk splenic APCs (129Sv; n = 3) or (B) splenic DCs (129Sv; n = 4) from Rras+/+ or Rras−/− mice in different ratios were comixed with 2 × 105 T cells from WT Balb/c for 96 hours. Allogeneic T-cell proliferation was measured by adding [H3]-labeled thymidine for the last 16 hours, and the amount of incorporation was measured by a scintillation counter. Results represent triplicate measurements from a single experiment with data in panel A reproduced in 2 additional experiments. (C) A similar proliferation assay using WT T cells was conducted as in panels A and B, except that BM-DCs (129Sv) were used. Bars represent SD. (D) In vivo T-cell proliferation assays were performed. Rras+/+ or Rras−/− mice (129Sv) were injected intraperitoneally with PBS, 10 μg LPS, or 10 μg LPS and 1 mg OVA. Six hours after injection, splenic DCs were isolated and comixed with naive CFSE-labeled polyclonal syngeneic splenic T cells (129Sv) for 96 hours. CFSE+ staining was analyzed by flow cytometry to measure T-cell proliferation. All plots are gated for TCR+CD4+ cells. (E) Percentages from panel D for CFSE+ proliferating T cells are plotted. Results represent data from 2 independent experiments with Rras+/+ (n = 5) and Rras−/− (n = 6) mice. Bars represent median. ***P < .0005.
