Figure 1
Figure 1. CDK6 is required for reconstitution of the hematopoietic system. (A) Schematic representation of experimental design. Cdk6+/+/Ly5.1+ and Cdk6−/−/Ly5.2+ BM cells were transplanted in ratios of 1:9, 1:1, and 9:1 into lethally irradiated (9 Gy) wild-type recipient mice. Long-term BM reconstitution was analyzed 16 weeks after transplantation (n = 5 per genotype; Cdk6+/+ and Cdk6−/− groups were compared using Student t test). (B) Ly5.1+/Ly5.2+ compositions were analyzed in total BM leukocytes (n = 5 per genotype; ****P < .0001). The leukocytic population included lymphocytes and myeloid cells, but excluded debris and erythrocytes, as determined by forward scatter/side scatter blots. (C) LSK cells were analyzed for Ly5.1+/Ly5.2+ composition in each transplantation setting (n = 5 per genotype; ****P < .0001). (D) Contributions of Ly5.1+ and Ly5.2+ cells in long-term HSCs (LT-HSCs), short-term HSCs (ST-HSCs), and MPP (n = 5 per genotype; ****P < .0001, *P < .05). (E) Cdk6+/+ and Cdk6−/− BM were infected with empty dsRed+ or GFP+ retrovirus. Equal numbers of Cdk6+/+ dsRed+ LSKs and Cdk6−/− GFP+ LSKs (100 000/mouse) were injected in a 1:1 ratio into lethally irradiated recipient animals in a competitive setting (LSK-depleted carrier BM was added and a total of 3 × 106 cells/mouse were injected). After 18 hours, mice BM was analyzed for dsRed+ and GFP+ LSKs (left panel, n = 6). In a noncompetitive setting, equal numbers of either Cdk6+/+/Ly5.2+ or Cdk6−/−/Ly5.2+ BM cells were injected into lethally irradiated Ly5.1+ mice (1 × 106 cells/mouse). After 18 hours, BM was analyzed for the presence of donor-derived Ly5.2+ LSKs (right panel, n = 4 per genotype).

CDK6 is required for reconstitution of the hematopoietic system. (A) Schematic representation of experimental design. Cdk6+/+/Ly5.1+ and Cdk6−/−/Ly5.2+ BM cells were transplanted in ratios of 1:9, 1:1, and 9:1 into lethally irradiated (9 Gy) wild-type recipient mice. Long-term BM reconstitution was analyzed 16 weeks after transplantation (n = 5 per genotype; Cdk6+/+ and Cdk6−/− groups were compared using Student t test). (B) Ly5.1+/Ly5.2+ compositions were analyzed in total BM leukocytes (n = 5 per genotype; ****P < .0001). The leukocytic population included lymphocytes and myeloid cells, but excluded debris and erythrocytes, as determined by forward scatter/side scatter blots. (C) LSK cells were analyzed for Ly5.1+/Ly5.2+ composition in each transplantation setting (n = 5 per genotype; ****P < .0001). (D) Contributions of Ly5.1+ and Ly5.2+ cells in long-term HSCs (LT-HSCs), short-term HSCs (ST-HSCs), and MPP (n = 5 per genotype; ****P < .0001, *P < .05). (E) Cdk6+/+ and Cdk6−/− BM were infected with empty dsRed+ or GFP+ retrovirus. Equal numbers of Cdk6+/+ dsRed+ LSKs and Cdk6−/− GFP+ LSKs (100 000/mouse) were injected in a 1:1 ratio into lethally irradiated recipient animals in a competitive setting (LSK-depleted carrier BM was added and a total of 3 × 106 cells/mouse were injected). After 18 hours, mice BM was analyzed for dsRed+ and GFP+ LSKs (left panel, n = 6). In a noncompetitive setting, equal numbers of either Cdk6+/+/Ly5.2+ or Cdk6−/−/Ly5.2+ BM cells were injected into lethally irradiated Ly5.1+ mice (1 × 106 cells/mouse). After 18 hours, BM was analyzed for the presence of donor-derived Ly5.2+ LSKs (right panel, n = 4 per genotype).

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