Fig. 2.
Fig. 2. TGF-β1 enhanced differentiation of CD11b+hiCD11c− cells from murine Lin−c-kit+ HPCs in the presence of GM-CSF + SCF with or without TNF at day 6. (A) Dose-dependent induction of CD11b+hiCD11c− cells by TGF-β1 in the cultures stimulated with GM-CSF + SCF + TNF. The data represent the mean value ± SD of the percentage of CD11b+hiCD11c− cells observed in more than five experiments. *P < .05 significance as compared with the cultures in the absence of TGF-β1. (B) Induction of CD11b−/dullCD11c+, CD11b+hiCD11c+, and CD11b+hiCD11c− cells by TGF-β1 in Lin−c-kit+ HPC cultures stimulated by various combination of cytokines as indicated. Quads were set up on the isotype-matched control dot plot, and the results are representative of more than five experiments.

TGF-β1 enhanced differentiation of CD11b+hiCD11c cells from murine Linc-kit+ HPCs in the presence of GM-CSF + SCF with or without TNF at day 6. (A) Dose-dependent induction of CD11b+hiCD11c cells by TGF-β1 in the cultures stimulated with GM-CSF + SCF + TNF. The data represent the mean value ± SD of the percentage of CD11b+hiCD11c cells observed in more than five experiments. *P < .05 significance as compared with the cultures in the absence of TGF-β1. (B) Induction of CD11b−/dullCD11c+, CD11b+hiCD11c+, and CD11b+hiCD11c cells by TGF-β1 in Linc-kit+ HPC cultures stimulated by various combination of cytokines as indicated. Quads were set up on the isotype-matched control dot plot, and the results are representative of more than five experiments.

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