Deletion of Moz results in a substantial reduction in populations with a cell surface phenotype characteristic of HSCs and of cells in G0. (A) Experimental design. Mice were treated with poly(I:C) and then left undisturbed for 4 months to allow recovery from acute inflammation induced by poly(I:C). (B) Examples of PCR genotyping of progenitor colonies from Mozfl/fl and Mozfl/fl;Mx1-cre cultures after stimulation with SCF, EPO, and IL3. Note that myeloid colony-forming progenitors (supplemental Figure 3) are derived from Moz-deleted cells that have existed for 4 months. (C) Flow cytometry plots showing analyses of the LSK-CD34–FLT3– and LSK-CD48–CD150+ populations in Mozfl/fl and Mozfl/fl;Mx1-cre bone marrow cells. (D-E) Quantification of stem cell surface markers by flow cytometry of recipients of Mozfl/fl and Mozfl/fl;Mx1-cre cells. Note the absence of typical LSK-CD34–FLT3– and LSK-CD48–CD150+ populations. (F) Cell cycle analysis of stem/progenitor populations. Note the reduction in the number of cells in G0. Data are presented as the mean ± SEM.