Figure 5
Figure 5. Distribution of myeloid progenitor populations of transplanted BM cells at the early stage. BM cells were isolated from mice preinjected with 5-FU 5 days before, and infected with retroviral vectors containing control GFP (MigR1), COP1, and Trib1. Six to 8 weeks after BMT, mice were killed, and BM cells were analyzed by fluorescence-activated cell sorter. (A) The level of GFP signals in BM cells is shown in the upper panels (the percentage of GFP-positive cells). GFP-negative (GFP−, middle panels) and -positive (GFP+, lower panels) BM cells were stained with anti-Mac1 and anti–Gr-1 antibodies. The percentages of immature (Mac-1+Gr-1lo) and differentiated (Mac-1+Gr-1hi) granulocytes are shown. (B) GFP-positive BM cells were stained with a lineage cocktail without anti–Mac-1 and anti–Gr-1 (Lin*, upper panels), and the Lin*negSca-1− population was stained with anti–c-Kit and anti–Mac-1 (lower panels). The percentages of fractions containing CMP/GMP/MEP (Lin*negSca-1−Mac1−c-Kit+), committed myeloid progenitors (Lin*negSca-1−Mac1+c-Kit+), and differentiated myeloid cells (Lin*negSca-1−Mac1+c-Kitlo/−) are shown. Results are representative of 4 independent experiments.

Distribution of myeloid progenitor populations of transplanted BM cells at the early stage. BM cells were isolated from mice preinjected with 5-FU 5 days before, and infected with retroviral vectors containing control GFP (MigR1), COP1, and Trib1. Six to 8 weeks after BMT, mice were killed, and BM cells were analyzed by fluorescence-activated cell sorter. (A) The level of GFP signals in BM cells is shown in the upper panels (the percentage of GFP-positive cells). GFP-negative (GFP, middle panels) and -positive (GFP+, lower panels) BM cells were stained with anti-Mac1 and anti–Gr-1 antibodies. The percentages of immature (Mac-1+Gr-1lo) and differentiated (Mac-1+Gr-1hi) granulocytes are shown. (B) GFP-positive BM cells were stained with a lineage cocktail without anti–Mac-1 and anti–Gr-1 (Lin*, upper panels), and the Lin*negSca-1 population was stained with anti–c-Kit and anti–Mac-1 (lower panels). The percentages of fractions containing CMP/GMP/MEP (Lin*negSca-1Mac1c-Kit+), committed myeloid progenitors (Lin*negSca-1Mac1+c-Kit+), and differentiated myeloid cells (Lin*negSca-1Mac1+c-Kitlo/−) are shown. Results are representative of 4 independent experiments.

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