Figure 2.
Figure 2. PUM1 and PUM2 contribute to murine HSPC expansion. (A) RT-qPCR analysis of mPum1 and mPum2 transcripts in mouse stem/progenitor subpopulations: LT-HSC (long-term HSC, Lin−Sca+cKit+CD34−CD150+), ST-HSC (short-term HSC, Lin−Sca+cKit+CD34+CD150+), MPP (Lin−Sca+cKit+CD34+CD150−), CMP (Lin−Sca−cKit+CD34+CD16−), MEP (Lin−Sca−cKit+CD34−CD16−), and GMP (Lin−Sca−cKit+CD34+CD16+). Results are normalized to Gapdh expression and expressed relative to Pum expression in LT-HSCs. (B-F) LSK cells were transduced with lentiviral vectors encoding the indicated shRNA targeting mPum1 (shmPum1) or mPum2 (shmPum2) or both (shmPum1a+2a) or luciferase as control (shCtrl) (sequences detailed in supplemental Table 8). shRNA/GFP+ LSK cells were sorted 2 days after transduction and maintained in liquid culture. (B) Immunoblot analysis of the indicated proteins at day 7 posttransduction. p85-PI3kinase was used as loading control. (C) Cell expansion analysis along time of culture posttransduction (n = 3). (D) Cell cycle analysis upon propidium iodide labeling at day 5 posttransduction (n = 4). (E) Apoptosis analysis at day 7 posttransduction through AnnexinV-PE/7AAD labeling (n = 4). (F) At day 7 posttransduction, shRNA/GFP+ output LSK-derived cells were seeded in methylcellulose medium and numbering of CFC was assessed after 7 days (n = 5); representative micrographs of colonies are presented on the right side (×20). (G-I) Murine LSKCD150+ cells were transduced with lentiviral vectors encoding shRNA targeting mPum1 (shmPum1-a) or mPum2 (shmPum2-a) or luciferase as control (shCtrl). shRNA/GFP+ cells were sorted 2 days after transduction and maintained in liquid culture. (G) Immunoblot analysis of the indicated proteins at day 7 posttransduction. β-Tubulin was used as loading control. (H) Cell expansion analysis along time of culture posttransduction (n = 3). (I) Three days posttransduction, lethally irradiated C57BL/6-Ly5.2 mice received 15 000 sorted shRNA/GFP+ LSKCD150+ cells from C57Bl/6 (Ly5.1) donors, in competition with the same amount of GFP− LSKCD150+ cells from Ly5.1 mice, together with 1.5 × 105 Ly5.2 BM cells. Presence of GFP+ cells in CD45.1+ BM cells of engrafted mice was assessed 4 months later by flow cytometry (at least 105 events). Each symbol represents data from a single chimeric mouse. (Figure representative of 1 experiment out of 2). Data are expressed as mean ± SEM. *P < .05; **P < .01; ***P < .001 (Student t test).

PUM1 and PUM2 contribute to murine HSPC expansion. (A) RT-qPCR analysis of mPum1 and mPum2 transcripts in mouse stem/progenitor subpopulations: LT-HSC (long-term HSC, LinSca+cKit+CD34CD150+), ST-HSC (short-term HSC, LinSca+cKit+CD34+CD150+), MPP (LinSca+cKit+CD34+CD150), CMP (LinScacKit+CD34+CD16), MEP (LinScacKit+CD34CD16), and GMP (LinScacKit+CD34+CD16+). Results are normalized to Gapdh expression and expressed relative to Pum expression in LT-HSCs. (B-F) LSK cells were transduced with lentiviral vectors encoding the indicated shRNA targeting mPum1 (shmPum1) or mPum2 (shmPum2) or both (shmPum1a+2a) or luciferase as control (shCtrl) (sequences detailed in supplemental Table 8). shRNA/GFP+ LSK cells were sorted 2 days after transduction and maintained in liquid culture. (B) Immunoblot analysis of the indicated proteins at day 7 posttransduction. p85-PI3kinase was used as loading control. (C) Cell expansion analysis along time of culture posttransduction (n = 3). (D) Cell cycle analysis upon propidium iodide labeling at day 5 posttransduction (n = 4). (E) Apoptosis analysis at day 7 posttransduction through AnnexinV-PE/7AAD labeling (n = 4). (F) At day 7 posttransduction, shRNA/GFP+ output LSK-derived cells were seeded in methylcellulose medium and numbering of CFC was assessed after 7 days (n = 5); representative micrographs of colonies are presented on the right side (×20). (G-I) Murine LSKCD150+ cells were transduced with lentiviral vectors encoding shRNA targeting mPum1 (shmPum1-a) or mPum2 (shmPum2-a) or luciferase as control (shCtrl). shRNA/GFP+ cells were sorted 2 days after transduction and maintained in liquid culture. (G) Immunoblot analysis of the indicated proteins at day 7 posttransduction. β-Tubulin was used as loading control. (H) Cell expansion analysis along time of culture posttransduction (n = 3). (I) Three days posttransduction, lethally irradiated C57BL/6-Ly5.2 mice received 15 000 sorted shRNA/GFP+ LSKCD150+ cells from C57Bl/6 (Ly5.1) donors, in competition with the same amount of GFP LSKCD150+ cells from Ly5.1 mice, together with 1.5 × 105 Ly5.2 BM cells. Presence of GFP+ cells in CD45.1+ BM cells of engrafted mice was assessed 4 months later by flow cytometry (at least 105 events). Each symbol represents data from a single chimeric mouse. (Figure representative of 1 experiment out of 2). Data are expressed as mean ± SEM. *P < .05; **P < .01; ***P < .001 (Student t test).

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