Fig. 3.
Fig. 3. Intracellular cytokine accumulation in CD161+ NK cells from cultures of Lin− cells with IL-2 to determine the proportion of cells capable of cytokine production, and cytokine production by distinct subsets. / Umbilical cord blood 10-day NK cells (top), and CD3−/CD161+ cells from 30-day primary cultures of Lin− cells with IL-2 and Sl/Sl4hSCF220 feeder cells (bottom) were stimulated (6 hours, 37°C) with PMA and Ca++ ionophore (see “Materials and methods”). Surface phenotype and expression of the indicated cytokines were detected simultaneously (3-color immunofluorescence) on gated CD161+ cells as described in “Materials and methods,” and analyzed as in Figure 2. Percent positive cells is indicated in each quadrant. Experiment representative of at least 4 performed with similar results with each Ab combination.

Intracellular cytokine accumulation in CD161+ NK cells from cultures of Lin cells with IL-2 to determine the proportion of cells capable of cytokine production, and cytokine production by distinct subsets.

Umbilical cord blood 10-day NK cells (top), and CD3/CD161+ cells from 30-day primary cultures of Lin cells with IL-2 and Sl/Sl4hSCF220 feeder cells (bottom) were stimulated (6 hours, 37°C) with PMA and Ca++ ionophore (see “Materials and methods”). Surface phenotype and expression of the indicated cytokines were detected simultaneously (3-color immunofluorescence) on gated CD161+ cells as described in “Materials and methods,” and analyzed as in Figure 2. Percent positive cells is indicated in each quadrant. Experiment representative of at least 4 performed with similar results with each Ab combination.

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