Figure 3.
Bahcc1 depletion suppressed myeloid immortalization of LT-HSCs by conditional expression of MLL-ENL. (A-B) Western blot analyses of Bahcc1 in 293 cells (293Bahcc1) that stably expressed 3XFLAG-tagged Bahcc1 (A), and in shRNA-transduced 293Bahcc1 cells (B). 293 cells transduced with pcDNA3.1 vector alone were used as a negative control in panel A. shRNAs against luciferase (shLuc, a negative control) and Bahcc1 (shB-2 and shB-8) were transduced into 293Bahcc1 cells in panel B. Immunoprecipitants with anti-FLAG antibody were blotted with anti-DDDDK-tag antibody to detect expression of Bahcc1 (upper panels). α-Tubulin was analyzed in total lysates as an internal control (bottom panels). (C-D) Relative-relative expression levels of Bahcc1 (C) in immortalized LT-HSCs with shRNA transduction and clonogenicity (D) of the cells. (E-F) Representative FACS plots and quantification of CD11b+/Gr-1+, Gr-1−/c-kit+, and apoptotic (annexin V+/7AAD−) subpopulations by FACS (E), and RT-qPCR of Hoxa9, Meis1, and Evi1 (F) in colony-forming cells derived from immortalized LT-HSCs with depletion of Bahcc1. Bar graphs show the mean with SD of at least 3 independent experiments. ∗P < .05; ∗∗P < .01; ∗∗∗P < .001; ∗∗∗∗P < .0001; ns, not significant (ANOVA followed by Dunnett multiple comparisons for panels D-F).

Bahcc1 depletion suppressed myeloid immortalization of LT-HSCs by conditional expression of MLL-ENL. (A-B) Western blot analyses of Bahcc1 in 293 cells (293Bahcc1) that stably expressed 3XFLAG-tagged Bahcc1 (A), and in shRNA-transduced 293Bahcc1 cells (B). 293 cells transduced with pcDNA3.1 vector alone were used as a negative control in panel A. shRNAs against luciferase (shLuc, a negative control) and Bahcc1 (shB-2 and shB-8) were transduced into 293Bahcc1 cells in panel B. Immunoprecipitants with anti-FLAG antibody were blotted with anti-DDDDK-tag antibody to detect expression of Bahcc1 (upper panels). α-Tubulin was analyzed in total lysates as an internal control (bottom panels). (C-D) Relative-relative expression levels of Bahcc1 (C) in immortalized LT-HSCs with shRNA transduction and clonogenicity (D) of the cells. (E-F) Representative FACS plots and quantification of CD11b+/Gr-1+, Gr-1/c-kit+, and apoptotic (annexin V+/7AAD) subpopulations by FACS (E), and RT-qPCR of Hoxa9, Meis1, and Evi1 (F) in colony-forming cells derived from immortalized LT-HSCs with depletion of Bahcc1. Bar graphs show the mean with SD of at least 3 independent experiments. P < .05; ∗∗P < .01; ∗∗∗P < .001; ∗∗∗∗P < .0001; ns, not significant (ANOVA followed by Dunnett multiple comparisons for panels D-F).

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