Figure 4
Figure 4. Progressive loss of competitive repopulating activity is accompanied by an increase in SA-β-gal expression in hematopoietic stem progenitor cells. (A) BM cells derived from Ews−/− and WT littermates were stained as described in Methods for Lin−, LSK, and CD150+CD48− LSK populations and subsequently analyzed for apoptotic cell death. The percentages of Annexin V-positive cells are indicated. (B) Top panel: BM cells from Ews−/− mice (KO, CD45.2; right panel) and their Ews+/+ littermates (WT, CD45.2; left panel) were mixed with an equal number of competitor cells (CD45.1) and transplanted into lethally irradiated recipient (CD45.1.2) mice. Peripheral blood from the transplanted recipients was analyzed for CD45.1/CD45.2 expression by flow cytometry every 4 weeks after transplantation. Bottom panel: representative FACS profile showing donor (Ews−/−, CD45.2) and competitor (CD45.1) contributions at 20 weeks after transplantation in the peripheral blood of recipients. (C) Top panel: recipient mice were killed 20 weeks after transplant. Ews+/+- and Ews−/−-derived LSK cells were stained for SA-β-gal activity. At least 30 cells from 3 random fields were counted in each experiment and the percentage of SA-β-gal–positive cells is shown on the y-axis. *Statistically significant difference (2-tailed Student t test, n = 2, P = .01). Bottom panel: flow cytometric analysis of Ews−/− and WT littermate-derived LSK cells for the expression of SA-β-gal before and after transplantation. The cells were stained with a fluorescent β-galactosidase substrate (C12FDG) and analyzed by flow cytometry.

Progressive loss of competitive repopulating activity is accompanied by an increase in SA-β-gal expression in hematopoietic stem progenitor cells. (A) BM cells derived from Ews−/− and WT littermates were stained as described in Methods for Lin, LSK, and CD150+CD48 LSK populations and subsequently analyzed for apoptotic cell death. The percentages of Annexin V-positive cells are indicated. (B) Top panel: BM cells from Ews−/− mice (KO, CD45.2; right panel) and their Ews+/+ littermates (WT, CD45.2; left panel) were mixed with an equal number of competitor cells (CD45.1) and transplanted into lethally irradiated recipient (CD45.1.2) mice. Peripheral blood from the transplanted recipients was analyzed for CD45.1/CD45.2 expression by flow cytometry every 4 weeks after transplantation. Bottom panel: representative FACS profile showing donor (Ews−/−, CD45.2) and competitor (CD45.1) contributions at 20 weeks after transplantation in the peripheral blood of recipients. (C) Top panel: recipient mice were killed 20 weeks after transplant. Ews+/+- and Ews−/−-derived LSK cells were stained for SA-β-gal activity. At least 30 cells from 3 random fields were counted in each experiment and the percentage of SA-β-gal–positive cells is shown on the y-axis. *Statistically significant difference (2-tailed Student t test, n = 2, P = .01). Bottom panel: flow cytometric analysis of Ews−/− and WT littermate-derived LSK cells for the expression of SA-β-gal before and after transplantation. The cells were stained with a fluorescent β-galactosidase substrate (C12FDG) and analyzed by flow cytometry.

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