Figure 3
Figure 3. Ews deletion drives cell-cycle progression in hematopoietic stem and progenitor cell populations and modulates progenitor cell activity. (A) Flow cytometric analysis of PY (Pyronin-Y) and HO (Hoechst 33342) staining of Lin−Sca1+c-Kit+ and Lin−Sca1−c-Kit+ cells from Ews KO and WT littermate controls. The percentage of cells in each phase of the cell cycle is summarized in the accompanying table. Data shown are representative of 2 independent experiments. (B) CFU-S assay. At day 12, spleens were removed and fixed in Bouin fixative and CFU-S colonies were counted. The CFU-S activity of Ews−/− (KO) and Ews+/+ littermate control (WT) BM cells was assessed before transplantation and after 2 rounds of transplantation (after transplantation). Of note, when Ews−/− BM cells were subjected to transplantation, their CFU-S activity was markedly decreased and showed a lower CFU-S activity compared with that of WT. Data are presented as mean values ± SD. (C) CAFC assay. The CAFC activity of Ews−/− (KO; white bar) and Ews+/+ littermate control (WT; black bar) BM cells was assessed before transplantation and after 2 rounds of transplantation (after transplantation). Of note, Ews−/− BM cells did not have measurable week-4 CAFC activity after BM transplantation, which is indicative of progenitor cell exhaustion. A total of 48 replicate wells were prepared per dilution and evaluated. Any well that had a colony of more than 6 cobblestone cells growing underneath the stromal cell layer was scored as positive. The y-axis denotes the percentage (%) of positive wells. Data are presented as mean ± SD. *Statistically significant difference (2-tailed Student t test, n > 4).

Ews deletion drivescell-cycleprogression in hematopoieticstemandprogenitor cellpopulations and modulates progenitor cell activity. (A) Flow cytometric analysis of PY (Pyronin-Y) and HO (Hoechst 33342) staining of LinSca1+c-Kit+ and LinSca1c-Kit+ cells from Ews KO and WT littermate controls. The percentage of cells in each phase of the cell cycle is summarized in the accompanying table. Data shown are representative of 2 independent experiments. (B) CFU-S assay. At day 12, spleens were removed and fixed in Bouin fixative and CFU-S colonies were counted. The CFU-S activity of Ews−/− (KO) and Ews+/+ littermate control (WT) BM cells was assessed before transplantation and after 2 rounds of transplantation (after transplantation). Of note, when Ews−/− BM cells were subjected to transplantation, their CFU-S activity was markedly decreased and showed a lower CFU-S activity compared with that of WT. Data are presented as mean values ± SD. (C) CAFC assay. The CAFC activity of Ews−/− (KO; white bar) and Ews+/+ littermate control (WT; black bar) BM cells was assessed before transplantation and after 2 rounds of transplantation (after transplantation). Of note, Ews−/− BM cells did not have measurable week-4 CAFC activity after BM transplantation, which is indicative of progenitor cell exhaustion. A total of 48 replicate wells were prepared per dilution and evaluated. Any well that had a colony of more than 6 cobblestone cells growing underneath the stromal cell layer was scored as positive. The y-axis denotes the percentage (%) of positive wells. Data are presented as mean ± SD. *Statistically significant difference (2-tailed Student t test, n > 4).

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