Figure 2
Figure 2. Reduction in the number of immunophenotypically defined GMPs from GATA-2+/− marrow. Bone marrow–nucleated cells from each genotype were lineage depleted using magnetic bead separation and lineage-negative–enriched cells were stained with various cell-surface antibodies to enable isolation of immunophenotypically defined progenitor subsets by flow cytometry. Representative flow cytometry plots for (Lin/CD127−CD117+Sca-1−CD34+CD16/32high) GMP, (Lin/CD127−CD117+Sca-1−CD34+CD16/32lo) CMP, and (Lin/CD127−CD117+Sca-1−CD34−CD16/32−) MEP isolation are shown (A) and for (Lin−CD117+Sca-1+Flt-3+CD34+) LMPP (B). The percentages for each gate are shown. The absolute number of LMPP, CMP, GMP, and MEP progenitors produced per harvest from multiple experiments is depicted (C) (LMPP, n = 4, P = .38; CMP, n = 9, P = .15; GMP, n = 9, P < .001<; and MEP, n = 9, P = .1). ** indicates statistical significance. Error bars indicate SEM. Statistical analysis was performed by using the paired Student t test.

Reduction in the number of immunophenotypically defined GMPs from GATA-2+/− marrow. Bone marrow–nucleated cells from each genotype were lineage depleted using magnetic bead separation and lineage-negative–enriched cells were stained with various cell-surface antibodies to enable isolation of immunophenotypically defined progenitor subsets by flow cytometry. Representative flow cytometry plots for (Lin/CD127CD117+Sca-1CD34+CD16/32high) GMP, (Lin/CD127CD117+Sca-1CD34+CD16/32lo) CMP, and (Lin/CD127CD117+Sca-1CD34CD16/32) MEP isolation are shown (A) and for (LinCD117+Sca-1+Flt-3+CD34+) LMPP (B). The percentages for each gate are shown. The absolute number of LMPP, CMP, GMP, and MEP progenitors produced per harvest from multiple experiments is depicted (C) (LMPP, n = 4, P = .38; CMP, n = 9, P = .15; GMP, n = 9, P < .001<; and MEP, n = 9, P = .1). ** indicates statistical significance. Error bars indicate SEM. Statistical analysis was performed by using the paired Student t test.

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