Fig. 7.
Fig. 7. Induction of the DC-associated differentiation/activation antigens CMRF-44, CMRF-56, and CD83 on cultured Lin− cells. / Sort-purified CD11c+ and CD11c− populations were cultured for 18 hours in the presence of GM-CSF and IL-3 with or without allogeneic T lymphocytes. Following culture, cells were harvested and stained with biotinylated CMRF-44 or CMRF-56, or purified CD83 mAb followed by biotinylated anti–mouse IgG. Biotinylated antibody was detected with PE- or PE-Cy5–conjugated streptavidin, in conjunction with PE-Cy5– or PE-conjugated CD16 or CD34 for the (A) CD11c+ and (B) CD11c− populations, respectively. CD11c+CD16−, CD11c+CD16+, CD11c−CD34+, and CD11c−CD34− populations were gated and examined for their expression of activation antigens (solid lines). Dashed lines represent negative control antibody staining.

Induction of the DC-associated differentiation/activation antigens CMRF-44, CMRF-56, and CD83 on cultured Lin cells.

Sort-purified CD11c+ and CD11c populations were cultured for 18 hours in the presence of GM-CSF and IL-3 with or without allogeneic T lymphocytes. Following culture, cells were harvested and stained with biotinylated CMRF-44 or CMRF-56, or purified CD83 mAb followed by biotinylated anti–mouse IgG. Biotinylated antibody was detected with PE- or PE-Cy5–conjugated streptavidin, in conjunction with PE-Cy5– or PE-conjugated CD16 or CD34 for the (A) CD11c+ and (B) CD11c populations, respectively. CD11c+CD16, CD11c+CD16+, CD11cCD34+, and CD11cCD34 populations were gated and examined for their expression of activation antigens (solid lines). Dashed lines represent negative control antibody staining.

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