Figure 3
Figure 3. In vivo Ho uptake by BM HSCs and multipotent progenitor cells according to their CD34 and FLT3 expression profiles. 129SvJ mice were perfused with Ho dye intravenously 10 and 5 minutes before tissue sampling, and BM was processed exactly as described in Figure 1. BM cells were stained for lineage, CD41, Sca-1, KIT, CD34, and FLT3 surface antigens. (A) Dot plot of CD34 versus FLT3 expression on viable 7-amino-actinomycin D− LSK CD41−Sca-1+KIT+ cells. (B-D) Representative dot plots of Ho blue fluorescence versus Ho red fluorescence of gated viable LSK CD41−CD34−FLT3− long-term reconstituting HSCs, LSK CD41−CD34+FLT3− short-term reconstituting myeloid progenitors, and LSK CD41−FLT3+ short-term reconstituting lymphoid progenitors, respectively. (E) Distribution of Hoechst bright, medium, and negative cells among LSK CD41−CD34−FLT3− (CD34- FLT3-), LSK CD41−CD34+FLT3− (CD34+ FLT3-), and LSK CD41−FLT3+ (FLT3+) populations. Data are average ± SD from 3 mice.

In vivo Ho uptake by BM HSCs and multipotent progenitor cells according to their CD34 and FLT3 expression profiles. 129SvJ mice were perfused with Ho dye intravenously 10 and 5 minutes before tissue sampling, and BM was processed exactly as described in Figure 1. BM cells were stained for lineage, CD41, Sca-1, KIT, CD34, and FLT3 surface antigens. (A) Dot plot of CD34 versus FLT3 expression on viable 7-amino-actinomycin D LSK CD41Sca-1+KIT+ cells. (B-D) Representative dot plots of Ho blue fluorescence versus Ho red fluorescence of gated viable LSK CD41CD34FLT3 long-term reconstituting HSCs, LSK CD41CD34+FLT3 short-term reconstituting myeloid progenitors, and LSK CD41FLT3+ short-term reconstituting lymphoid progenitors, respectively. (E) Distribution of Hoechst bright, medium, and negative cells among LSK CD41CD34FLT3 (CD34- FLT3-), LSK CD41CD34+FLT3 (CD34+ FLT3-), and LSK CD41FLT3+ (FLT3+) populations. Data are average ± SD from 3 mice.

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