Figure 5
Figure 5. Analysis of myeloid lineage properties and in vitro differentiation potential. (A) Sorted B220+Mac1−/Gr-1− cells were evaluated for the ability to generate myeloid colonies in M3434 methylcellulose. (B) MPO expression in the B220+Mac-1−/Gr-1−, compared with WT controls. (C) MPO expression in the B220+Mac-1+/Gr-1+ population compared with WT controls. (D) B220+Mac-1−/Gr-1− cells from FLT3/ITD-NHD13 mice were grown in liquid culture with myeloid cytokines and evaluated for differentiation ability and (E) functional activity. Images were acquired at room temperature using a Nikon TE 2000-E microscope system (Nikon) with a Nikon Plan APO VC 100×/1.40 oil objective and Nikon EZ-C1 Version 3.5 software. (F) Cells differentiated in liquid culture were stained for markers of macrophage differentiation.

Analysis of myeloid lineage properties and in vitro differentiation potential. (A) Sorted B220+Mac1/Gr-1 cells were evaluated for the ability to generate myeloid colonies in M3434 methylcellulose. (B) MPO expression in the B220+Mac-1/Gr-1, compared with WT controls. (C) MPO expression in the B220+Mac-1+/Gr-1+ population compared with WT controls. (D) B220+Mac-1/Gr-1 cells from FLT3/ITD-NHD13 mice were grown in liquid culture with myeloid cytokines and evaluated for differentiation ability and (E) functional activity. Images were acquired at room temperature using a Nikon TE 2000-E microscope system (Nikon) with a Nikon Plan APO VC 100×/1.40 oil objective and Nikon EZ-C1 Version 3.5 software. (F) Cells differentiated in liquid culture were stained for markers of macrophage differentiation.

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