Figure 4
Figure 4. Analysis of activation of the Arf locus at various stages of tumorigenesis. (A) Bone marrow cells from Arf+/+ mice (controls) and ArfGfp/Gfp knock-in mice (functionally Arf-null) were transduced with MSCV-Lmo2-IRES-mCherry and transplanted back into lethally irradiated wild-type recipients. Between weeks 4 and 23 after transplantation, individual animals were killed from each cohort of recipients, their thymi removed, and thymocytes analyzed for expression of GFP and mCherry by flow cytometry. Only a small fraction of mCherry+ cells expressed GFP by 13 weeks after transplantation. An example of GFP activation in a thymic tumor arising 24 weeks after transplantation is illustrated at the right. GFP-positive cells were also detected in the spleen, bone marrow, and peripheral blood of this mouse. (B) CD4−/CD8− double-negative Arf+/+ and ArfGfp/Gfp thymocytes transduced with either MSCV-IRES-mCherry or MSCV-Lmo2-IRES-mCherry were cultured in vitro on OP9-DL1 stromal cells together with IL-7 and FLT-3 ligand. After 20 days in culture, thymocytes were sorted to recover mCherry+ cells at the DN2 stage. DN2 mCherry+ thymocytes (2 × 105) were transplanted into lethally irradiated mice together with 2 × 105 bone marrow cells. The panels show the cultured thymocytes in the graft before sorting and then from thymi harvested between 6 and 12 weeks after transplantation and analyzed for the presence of mCherry and GFP.

Analysis of activation of the Arf locus at various stages of tumorigenesis. (A) Bone marrow cells from Arf+/+ mice (controls) and ArfGfp/Gfp knock-in mice (functionally Arf-null) were transduced with MSCV-Lmo2-IRES-mCherry and transplanted back into lethally irradiated wild-type recipients. Between weeks 4 and 23 after transplantation, individual animals were killed from each cohort of recipients, their thymi removed, and thymocytes analyzed for expression of GFP and mCherry by flow cytometry. Only a small fraction of mCherry+ cells expressed GFP by 13 weeks after transplantation. An example of GFP activation in a thymic tumor arising 24 weeks after transplantation is illustrated at the right. GFP-positive cells were also detected in the spleen, bone marrow, and peripheral blood of this mouse. (B) CD4/CD8 double-negative Arf+/+ and ArfGfp/Gfp thymocytes transduced with either MSCV-IRES-mCherry or MSCV-Lmo2-IRES-mCherry were cultured in vitro on OP9-DL1 stromal cells together with IL-7 and FLT-3 ligand. After 20 days in culture, thymocytes were sorted to recover mCherry+ cells at the DN2 stage. DN2 mCherry+ thymocytes (2 × 105) were transplanted into lethally irradiated mice together with 2 × 105 bone marrow cells. The panels show the cultured thymocytes in the graft before sorting and then from thymi harvested between 6 and 12 weeks after transplantation and analyzed for the presence of mCherry and GFP.

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