Reduced SHP-1 phosphatase activity is responsible for MDS/MPN development in lyn−/−;PLC-β3−/− mice. (A) CD34−KSL cells were cultured in the presence of IL-3 and SCF for 4 weeks and were analyzed for SHP-1 phosphatase activity. Data are mean ± SD, *P < .05 versus vector control. Similar expression levels of SHP-1 among the cells can be seen in Figure 5D. (B) CD34−KSL cells from lyn−/−;PLC-β3−/− mice were retrovirally transduced with empty vector or various SHP-1 mutants. Sorted GFP+ cells were cultured in the presence of IL-3 and SCF for 4 weeks and then measured for SHP-1 phosphatase activity. (C) Stat5 phosphorylation in the cells from panel B was measured by flow cytometry. Expression of SHP-1 (C) and Stat5 (D) was assessed by immunoblotting. (D) CD34−KSL cells from lyn−/−;PLC-β3−/− mice were transduced with a bicistronic retroviral vector encoding wt SHP-1, DYE SHP-1, or empty vector, together with GFP. Transduced GFP+ cells were sorted and cultured in the presence of IL-3 and SCF. (E) Transduced lyn−/−;PLC-β3−/−CD34−KSL cells were adoptively transferred (without sorting) to lethally irradiated C57BL/6-Ly5.1 mice. Donor-derived (Ly5.2+) CD11b+ cells in peripheral blood were analyzed by flow cytometry. **P < .01.