Figure 3
Figure 3. Slug-deficient BM shows enhanced long-term repopulating ability in vivo. (A) Relative repopulating ability of Slug−/− and Slug+/− HSCs in recipients. Equal number (2 × 105) of Slug−/− and Slug+/− BM cells (test cells, CD45.2+) were cotransplanted with wild-type competitor BM cells (CD45.1+/ CD45.2+) into lethally irradiated recipient mice (CD45.1+, n = 8 for each group). The relative repopulating ability of test cells was determined by the percentage of CD45.2+ with total donor-derived cells (CD45.2+ and CD45.1+/ CD45.2+ cells) in blood at 8 weeks and 16 weeks after BM transplantation. There is a significant difference between the 2 groups of reconstituted mice (**P < .01 for Slug−/− vs Slug+/−). (B) Multilineage distribution (4 months after BM transplantation) in Slug+/− BM (test, CD45.2+)–derived and wild-type competitor cell (CD45.1+/ CD45.2+) population-derived hematopoietic cells of recipients (n = 8) transplanted with Slug+/− BM donors. There is no significant difference in the percentage of T, B, and myeloid cells derived from transplanted donor cells from Slug+/− mice and competitive cells. (C) Multilineage distribution (4 months after BM transplantation) in Slug−/− BM (test, CD45.2+) donor-derived and wild-type competitor cell (CD45.1+/CD45.2+) population-derived hematopoietic cells of recipients (n = 8) reconstituted with Slug−/− BM. There is no significant difference in the percentage of T, B, and myeloid cells derived from transplanted donor cells from Slug−/− mice and competitive cells. (D) Diagram of BM homing assay for primitive hematopoietic cells. Test BM cells (CD45.2+) from mice were equally mixed with wild-type competitor BM cells (CD45.1+/CD45.2+), and the ratio of Lin−Sca-1+ cells in test vs competitor cells (the number of Lin−Sca-1+ cells in test BM cells to the number of Lin−Sca-1+ cells in competitor BM cells) was determined by flow cytometry before being injected into lethally irradiated recipients (CD45.1+). Sixteen hours after BM injection, the ratio of Lin−Sca-1+ cells in test vs competitor cells (the percentage of CD45.2+ Lin−Sca-1+ cells to the percentage of CD45.1+/CD45.2+ Lin−Sca-1+ cells) was determined and compared with the ratio of these cells before BM injection. (E) Relative homing ability of Lin−Sca-1+ primitive hematopoietic cells from Slug−/− or Slug+/− mice. The graph indicates that the ratio of Lin−Sca-1+ cells in test (Slug−/− or Slug+/−) BM cells vs competitor cells was comparable in recipients (n = 4). (F) Chimerism in recipients transplanted with BM cells of Slug−/− or Slug+/− mice. Limiting numbers (5 × 104 and 2 × 105) of BM cells from Slug−/− or Slug+/− mice were cotransplanted with 2 × 105 competitor cells (CD45.1+/CD45.2+) into 2 groups of recipients (n = 8 for each group). Chimerism was analyzed by flow cytometric analysis of peripheral blood cells 4 months after BM transplantation. In each animal, 1% or higher of donor-derived (CD45.2+) cells containing T, B, and myeloid cell was defined as positive engraftment. **P < .01 for Slug−/− vs Slug+/−.

Slug-deficient BM shows enhanced long-term repopulating ability in vivo. (A) Relative repopulating ability of Slug−/− and Slug+/− HSCs in recipients. Equal number (2 × 105) of Slug−/− and Slug+/− BM cells (test cells, CD45.2+) were cotransplanted with wild-type competitor BM cells (CD45.1+/ CD45.2+) into lethally irradiated recipient mice (CD45.1+, n = 8 for each group). The relative repopulating ability of test cells was determined by the percentage of CD45.2+ with total donor-derived cells (CD45.2+ and CD45.1+/ CD45.2+ cells) in blood at 8 weeks and 16 weeks after BM transplantation. There is a significant difference between the 2 groups of reconstituted mice (**P < .01 for Slug−/− vs Slug+/−). (B) Multilineage distribution (4 months after BM transplantation) in Slug+/− BM (test, CD45.2+)–derived and wild-type competitor cell (CD45.1+/ CD45.2+) population-derived hematopoietic cells of recipients (n = 8) transplanted with Slug+/− BM donors. There is no significant difference in the percentage of T, B, and myeloid cells derived from transplanted donor cells from Slug+/− mice and competitive cells. (C) Multilineage distribution (4 months after BM transplantation) in Slug−/− BM (test, CD45.2+) donor-derived and wild-type competitor cell (CD45.1+/CD45.2+) population-derived hematopoietic cells of recipients (n = 8) reconstituted with Slug−/− BM. There is no significant difference in the percentage of T, B, and myeloid cells derived from transplanted donor cells from Slug−/− mice and competitive cells. (D) Diagram of BM homing assay for primitive hematopoietic cells. Test BM cells (CD45.2+) from mice were equally mixed with wild-type competitor BM cells (CD45.1+/CD45.2+), and the ratio of LinSca-1+ cells in test vs competitor cells (the number of LinSca-1+ cells in test BM cells to the number of LinSca-1+ cells in competitor BM cells) was determined by flow cytometry before being injected into lethally irradiated recipients (CD45.1+). Sixteen hours after BM injection, the ratio of LinSca-1+ cells in test vs competitor cells (the percentage of CD45.2+ LinSca-1+ cells to the percentage of CD45.1+/CD45.2+ LinSca-1+ cells) was determined and compared with the ratio of these cells before BM injection. (E) Relative homing ability of LinSca-1+ primitive hematopoietic cells from Slug−/− or Slug+/− mice. The graph indicates that the ratio of LinSca-1+ cells in test (Slug−/− or Slug+/−) BM cells vs competitor cells was comparable in recipients (n = 4). (F) Chimerism in recipients transplanted with BM cells of Slug−/− or Slug+/− mice. Limiting numbers (5 × 104 and 2 × 105) of BM cells from Slug−/− or Slug+/− mice were cotransplanted with 2 × 105 competitor cells (CD45.1+/CD45.2+) into 2 groups of recipients (n = 8 for each group). Chimerism was analyzed by flow cytometric analysis of peripheral blood cells 4 months after BM transplantation. In each animal, 1% or higher of donor-derived (CD45.2+) cells containing T, B, and myeloid cell was defined as positive engraftment. **P < .01 for Slug−/− vs Slug+/−.

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