Figure 3
Figure 3. SCL level determines the output of hematopoietic progenitors. (A) WT bone marrow cells expressing either SCL, ΔbSCL, or control empty vector were plated in suspension culture with SF and IL-11 in selective media (G418). Samples were taken at the indicated times and plated in methylcellulose, and colonies were scored 9 days later. Represented are the cumulative growth curves of multipotent progenitors (CFU-GEMM) (upper panel) or MEPs (BFU-E/Meg) in culture. (B) Bone marrow cells expressing the indicated genes were plated in methylcellulose, and multipotent colonies were aspirated 9 days later, dispersed into single-cell suspensions and counted to determine colony size. Data shown (A-B) are typical of at least 2 independent experiments. (C) Western blot of total protein extracts from unfractionated bone marrow was used to assess SCL protein levels in WT and SCLtg mice. α-Protein tyrosine phosphatase 1D was used as a loading control. (D-E) Bone marrow cells from heterozygous SCLtg mice and WT littermates were cultured in methylcellulose in the presence of increasing concentrations of SF (D) or IL-3 (E). Multipotent colonies (CFU-GEMM) were scored 9 days later. Data represent the mean ± SD of 3 independent experiments performed in duplicate or quadruplicate. Data were analyzed using a nonlinear regression curve fitting routine (ALLFIT). Estimates of the half-effective concentrations of the different ligands on progenitors from SCLtg mice or WT littermates were as follows: 0.7 ± 0.4 (SCLtg) and 6 ± 3 (WT) ng/mL of SF for CFU-GEMMs or BFU-Es, and 0.2 ± 0.2 (SCLtg) and 0.2 ± 0.1 (WT) ng/mL of IL-3. *P < .05; **P < .01.

SCL level determines the output of hematopoietic progenitors. (A) WT bone marrow cells expressing either SCL, ΔbSCL, or control empty vector were plated in suspension culture with SF and IL-11 in selective media (G418). Samples were taken at the indicated times and plated in methylcellulose, and colonies were scored 9 days later. Represented are the cumulative growth curves of multipotent progenitors (CFU-GEMM) (upper panel) or MEPs (BFU-E/Meg) in culture. (B) Bone marrow cells expressing the indicated genes were plated in methylcellulose, and multipotent colonies were aspirated 9 days later, dispersed into single-cell suspensions and counted to determine colony size. Data shown (A-B) are typical of at least 2 independent experiments. (C) Western blot of total protein extracts from unfractionated bone marrow was used to assess SCL protein levels in WT and SCLtg mice. α-Protein tyrosine phosphatase 1D was used as a loading control. (D-E) Bone marrow cells from heterozygous SCLtg mice and WT littermates were cultured in methylcellulose in the presence of increasing concentrations of SF (D) or IL-3 (E). Multipotent colonies (CFU-GEMM) were scored 9 days later. Data represent the mean ± SD of 3 independent experiments performed in duplicate or quadruplicate. Data were analyzed using a nonlinear regression curve fitting routine (ALLFIT). Estimates of the half-effective concentrations of the different ligands on progenitors from SCLtg mice or WT littermates were as follows: 0.7 ± 0.4 (SCLtg) and 6 ± 3 (WT) ng/mL of SF for CFU-GEMMs or BFU-Es, and 0.2 ± 0.2 (SCLtg) and 0.2 ± 0.1 (WT) ng/mL of IL-3. *P < .05; **P < .01.

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