Figure 5
Figure 5. E47 null HSCs displayed hyperproliferation under steady state and after transplantation stress. (A) Flk2− LSKs from WT and E47 KO littermates were sorted by flow cytometry, and the expression of p21 and β-actin was examined by quantitative reverse-transcription PCR. The data are presented as KO/WT ratios for each transcript (n = 4 independent sorts). **P < .05. (B) Bone marrow cells from WT and E47 KO littermates were stained with cell surface antibodies to resolve HSC-enriched flk2− LSKs, and the number of flk2− LSKs was counted (n = 11 mice). (C) Surface-stained flk2− LSKs from E47 WT or KO mice were fixed and then stained with antibodies to the Ki67 proliferation antigen and DAPI for cell-cycle analysis. (Left panels) Representative flow cytometric profiles used to generate the bar graph on the right (n = 3 or 4 mice). **P < .05. (D) Lethally irradiated mice reconstituted with E47 KO or WT CD45.2 donor bone marrow cells were killed at 3 weeks after transplantation. A total of 100 μg BrdU was injected into recipient mice at a 12-hour interval for 24 hours before death. The donor-derived CD45.2 flk2− LSKs were fixed and stained with antibodies to BrdU, Ki67, or DAPI for proliferation and cell-cycle analysis (n = 4 mice). **P < .05. ns indicates not significant. (E) Bone marrow from E47 KO (CD45.2) and WT (CD45.1/2) mice was cotransferred into lethally irradiated CD45.1 hosts, and cell-cycle status was examined as in panel D at 2 weeks after transplantation. (n = 6 mice). P < .05.

E47 null HSCs displayed hyperproliferation under steady state and after transplantation stress. (A) Flk2 LSKs from WT and E47 KO littermates were sorted by flow cytometry, and the expression of p21 and β-actin was examined by quantitative reverse-transcription PCR. The data are presented as KO/WT ratios for each transcript (n = 4 independent sorts). **P < .05. (B) Bone marrow cells from WT and E47 KO littermates were stained with cell surface antibodies to resolve HSC-enriched flk2 LSKs, and the number of flk2 LSKs was counted (n = 11 mice). (C) Surface-stained flk2 LSKs from E47 WT or KO mice were fixed and then stained with antibodies to the Ki67 proliferation antigen and DAPI for cell-cycle analysis. (Left panels) Representative flow cytometric profiles used to generate the bar graph on the right (n = 3 or 4 mice). **P < .05. (D) Lethally irradiated mice reconstituted with E47 KO or WT CD45.2 donor bone marrow cells were killed at 3 weeks after transplantation. A total of 100 μg BrdU was injected into recipient mice at a 12-hour interval for 24 hours before death. The donor-derived CD45.2 flk2 LSKs were fixed and stained with antibodies to BrdU, Ki67, or DAPI for proliferation and cell-cycle analysis (n = 4 mice). **P < .05. ns indicates not significant. (E) Bone marrow from E47 KO (CD45.2) and WT (CD45.1/2) mice was cotransferred into lethally irradiated CD45.1 hosts, and cell-cycle status was examined as in panel D at 2 weeks after transplantation. (n = 6 mice). P < .05.

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