Figure 6
Figure 6. Impaired in vitro and in vivo functionality of Pyroninlow/Hoechstlow GMPs from GATA-2+/− marrow. GMPs from GATA-2+/+ and GATA-2+/− bone marrow were isolated by cell sorting and were subsequently stained with the RNA dye Pyronin Y (PY) and DNA dye Hoechst 33342 (Hst). Flow cytometry was performed to distinguish the PYlo or PYhigh in the G0/G1 fraction (Hstlow). Cells residing in PYlow/Hstlow or PYhigh/Hstlow were sorted and plated into colony-forming medium containing myeloid, megakaryocyte, and erythroid growth factors. Three replicates were used per genotype in each experiment. Colony formation was scored on day 10 (A) (B) GMPs from GATA-2+/+ and GATA-2+/− bone marrow were isolated by sorting and were subsequently stained with the DNA dye Hoechst 33342 (Hst) to enable discrimination of G0/G1 and S/G2/M populations The S/G2/M population was sorted and plated into colony-forming medium containing myeloid, megakaryocyte, and erythroid growth factors. Three replicates were used per genotype in each experiment. Colony formation was scored on day 10 (C). Data from multiple experiments are displayed (A-C) (PYlow/Hstlow, n = 5; G, P = .92; M, P = .06; GM, P = .002; PYhigh/Hstlow, n = 5; G, P = .47; M, P = .85; GM, P = .83; S/G2/M, n = 6; G, P = .71; M, P = .97; GM, P = .99). In vivo functionality was assessed by competitive transplantation of PYlow/Hstlow or PYhigh/Hstlow GMPs from each genotype (B6SJL-CD45.1) with C57BL/6-CD45.2 Lin-Sca-1+CD117+CD34− competitor stem cells into C57BL/6-CD45.2–irradiated recipients. Eight days after transplantation, the peripheral blood of the recipient mice were analyzed for the contribution of donor CD45.1 within the Gr-1+Mac-1+ compartment by flow cytometry. Data from multiple experiments are displayed for PYlow/Hstlow (D) (n = 3; P = .042) and PYhigh/Hstlow (E) (n = 3; P = .31). ** indicates statistical significance. Error bars indicate SEM. Statistical analysis was performed using the paired Student t test.

Impaired in vitro and in vivo functionality of Pyroninlow/Hoechstlow GMPs from GATA-2+/− marrow. GMPs from GATA-2+/+ and GATA-2+/− bone marrow were isolated by cell sorting and were subsequently stained with the RNA dye Pyronin Y (PY) and DNA dye Hoechst 33342 (Hst). Flow cytometry was performed to distinguish the PYlo or PYhigh in the G0/G1 fraction (Hstlow). Cells residing in PYlow/Hstlow or PYhigh/Hstlow were sorted and plated into colony-forming medium containing myeloid, megakaryocyte, and erythroid growth factors. Three replicates were used per genotype in each experiment. Colony formation was scored on day 10 (A) (B) GMPs from GATA-2+/+ and GATA-2+/− bone marrow were isolated by sorting and were subsequently stained with the DNA dye Hoechst 33342 (Hst) to enable discrimination of G0/G1 and S/G2/M populations The S/G2/M population was sorted and plated into colony-forming medium containing myeloid, megakaryocyte, and erythroid growth factors. Three replicates were used per genotype in each experiment. Colony formation was scored on day 10 (C). Data from multiple experiments are displayed (A-C) (PYlow/Hstlow, n = 5; G, P = .92; M, P = .06; GM, P = .002; PYhigh/Hstlow, n = 5; G, P = .47; M, P = .85; GM, P = .83; S/G2/M, n = 6; G, P = .71; M, P = .97; GM, P = .99). In vivo functionality was assessed by competitive transplantation of PYlow/Hstlow or PYhigh/Hstlow GMPs from each genotype (B6SJL-CD45.1) with C57BL/6-CD45.2 Lin-Sca-1+CD117+CD34 competitor stem cells into C57BL/6-CD45.2–irradiated recipients. Eight days after transplantation, the peripheral blood of the recipient mice were analyzed for the contribution of donor CD45.1 within the Gr-1+Mac-1+ compartment by flow cytometry. Data from multiple experiments are displayed for PYlow/Hstlow (D) (n = 3; P = .042) and PYhigh/Hstlow (E) (n = 3; P = .31). ** indicates statistical significance. Error bars indicate SEM. Statistical analysis was performed using the paired Student t test.

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