Figure 3
Figure 3. In vitro and in vivo cross-presentation of cell-associated, soluble, and viral antigens in Batf3-deficient mice. (A) Ly5.2+CD45RA− CD11c+Sirpα+ (top panels), CD11c+Sirpα−CD103− (CD8α+ equivalent; middle panels) and CD11c+Sirpα−CD103+ DCs (bottom panels) were purified from bone marrow cultures of Id2gfp/gfp(Ly5.2+)→Ly5.1 or Id2gfp/gfpBatf3−/−(Ly5.2+)→Ly5.1 chimeric mice that had been allowed to reconstitute for 10 weeks. Bone marrow was stimulated with Flt3L for 8 days with the addition of GM-CSF on day 6. FACS purified populations of DCs were cocultured with soluble OVA together with either CD8+ OT-I cells labeled with CellTracker Violet (CTV). Numbers represent the percentage of cells that have proliferated in response to exogenous antigen. Data are representative of bone marrow cells derived from 2 separate cohorts of Id2gfp/gfp(Ly5.2+)→Ly5.1 or Id2gfp/gfpBatf3−/−(Ly5.2+)→Ly5.1 chimeric mice and each DC subset analyses was performed in duplicate or triplicate within each experiment. (B) In vivo cross-presentation of soluble OVA (top panels). OVA-coated irradiated bm-1 splenocytes or soluble OVA was injected into recipient wild-type or Batf3−/− mice containing 1.5 × 106 CTV-labeled Ly5.1+ OT-I cells. After 3 days, the spleen was isolated and analyzed for proliferation by loss of CTV from Ly5.1+Vα2+CD8+ T cells. (C) Cross-presentation of cell-associated OVA in GVHD. Bm1.ActmOVA mice were irradiated and transplanted with 5 × 106 BM from either Id2-GFP or Id2 × Batf3−/− bone marrow, and 2 × 103 CD3+ T cells from Ly5.1 congenic mice. CSFE-labeled Ly5.1+ OT-I cells were adoptively transferred into mice on day 10 after transplantation and proliferation in the OVA-specific Vα2+ CD8+ T-cell population analyzed after 3 days. Data show representative proliferation profiles (left panels) and the mean number ± SD of Kb-OVA Vα2+ CD8+ T cells recovered per spleen (n = 8). NS, not significant. (D) Responses to HSV-1 virus infection. 1.5 × 106 CTV labeled Ly5.1+ HSV-1–specific (glycoprotein B, gB) CD8α+ T cells were adoptively transferred into wild-type or Batf3−/− mice 1 day before subcutaneous foot pad inoculation with HSV-1. After 3 days, the spleen was isolated and analyzed for proliferation by loss of CTV from Ly5.1+Vα2+CD8+ T cells. Data are representative of 3 experiments with 2 to 4 mice in each group for each experiment.

In vitro and in vivo cross-presentation of cell-associated, soluble, and viral antigens in Batf3-deficient mice. (A) Ly5.2+CD45RA CD11c+Sirpα+ (top panels), CD11c+SirpαCD103 (CD8α+ equivalent; middle panels) and CD11c+SirpαCD103+ DCs (bottom panels) were purified from bone marrow cultures of Id2gfp/gfp(Ly5.2+)→Ly5.1 or Id2gfp/gfpBatf3−/−(Ly5.2+)→Ly5.1 chimeric mice that had been allowed to reconstitute for 10 weeks. Bone marrow was stimulated with Flt3L for 8 days with the addition of GM-CSF on day 6. FACS purified populations of DCs were cocultured with soluble OVA together with either CD8+ OT-I cells labeled with CellTracker Violet (CTV). Numbers represent the percentage of cells that have proliferated in response to exogenous antigen. Data are representative of bone marrow cells derived from 2 separate cohorts of Id2gfp/gfp(Ly5.2+)→Ly5.1 or Id2gfp/gfpBatf3−/−(Ly5.2+)→Ly5.1 chimeric mice and each DC subset analyses was performed in duplicate or triplicate within each experiment. (B) In vivo cross-presentation of soluble OVA (top panels). OVA-coated irradiated bm-1 splenocytes or soluble OVA was injected into recipient wild-type or Batf3−/− mice containing 1.5 × 106 CTV-labeled Ly5.1+ OT-I cells. After 3 days, the spleen was isolated and analyzed for proliferation by loss of CTV from Ly5.1+Vα2+CD8+ T cells. (C) Cross-presentation of cell-associated OVA in GVHD. Bm1.ActmOVA mice were irradiated and transplanted with 5 × 106 BM from either Id2-GFP or Id2 × Batf3−/− bone marrow, and 2 × 103 CD3+ T cells from Ly5.1 congenic mice. CSFE-labeled Ly5.1+ OT-I cells were adoptively transferred into mice on day 10 after transplantation and proliferation in the OVA-specific Vα2+ CD8+ T-cell population analyzed after 3 days. Data show representative proliferation profiles (left panels) and the mean number ± SD of Kb-OVA Vα2+ CD8+ T cells recovered per spleen (n = 8). NS, not significant. (D) Responses to HSV-1 virus infection. 1.5 × 106 CTV labeled Ly5.1+ HSV-1–specific (glycoprotein B, gB) CD8α+ T cells were adoptively transferred into wild-type or Batf3−/− mice 1 day before subcutaneous foot pad inoculation with HSV-1. After 3 days, the spleen was isolated and analyzed for proliferation by loss of CTV from Ly5.1+Vα2+CD8+ T cells. Data are representative of 3 experiments with 2 to 4 mice in each group for each experiment.

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