Figure 2
Figure 2. Lmo2 impedes thymocyte maturation at the DN2 stage. (A) Bone marrow cells from Arf+/+ and Arf−/− animals were transduced with Lmo2-mCherry and transplanted into lethally irradiated recipient animals. At 91 days after transplantation, mice were killed and thymocytes were analyzed by fluorescence-activated flow cytometry for mature (CD4 and CD8) and immature (CD44 and CD25) T-cell markers. The control was a normal age-matched thymus stained for the same markers. (B) Antibody-dependent microbead-mediated depletion was used to remove the double-positive (CD4+CD8+) and single-positive (CD4+ and CD8+) cells from the thymus of 3 Arf+/+ and 3 Arf−/− animals. The remaining double-negative thymocytes were transduced with either MSCV-IRES-mCherry or MSCV-Lmo2-IRES-mCherry. Transduced thymocytes were cultured in vitro on OP9-DL1 stromal cells together with IL-7 and FLT-3 ligand. After 14 days, transduced thymocytes expressing mCherry were immunostained as in panel A, sorted to obtain the DN2 population (CD44+CD25+), and replated at the same density on OP9-DL1 stromal cells. Seven days later, cells were reanalyzed by flow cytometry for the same markers. (C) The absolute number of cells in Lmo2, Arf+/+ and Lmo2, Arf−/− populations at day 4, 8, and 11 after the sort were counted. Consistent results were obtained in 2 replicate experiments.

Lmo2 impedes thymocyte maturation at the DN2 stage. (A) Bone marrow cells from Arf+/+ and Arf−/− animals were transduced with Lmo2-mCherry and transplanted into lethally irradiated recipient animals. At 91 days after transplantation, mice were killed and thymocytes were analyzed by fluorescence-activated flow cytometry for mature (CD4 and CD8) and immature (CD44 and CD25) T-cell markers. The control was a normal age-matched thymus stained for the same markers. (B) Antibody-dependent microbead-mediated depletion was used to remove the double-positive (CD4+CD8+) and single-positive (CD4+ and CD8+) cells from the thymus of 3 Arf+/+ and 3 Arf−/− animals. The remaining double-negative thymocytes were transduced with either MSCV-IRES-mCherry or MSCV-Lmo2-IRES-mCherry. Transduced thymocytes were cultured in vitro on OP9-DL1 stromal cells together with IL-7 and FLT-3 ligand. After 14 days, transduced thymocytes expressing mCherry were immunostained as in panel A, sorted to obtain the DN2 population (CD44+CD25+), and replated at the same density on OP9-DL1 stromal cells. Seven days later, cells were reanalyzed by flow cytometry for the same markers. (C) The absolute number of cells in Lmo2, Arf+/+ and Lmo2, Arf−/− populations at day 4, 8, and 11 after the sort were counted. Consistent results were obtained in 2 replicate experiments.

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