Figure 2.
Figure 2. MIST is dispensable for development of NK and NKT cells. (A) Cells isolated from liver (left) and spleen (right) of 4- to 6-week-old MIST-deficient mice (-/-) and their littermates (+/+) were stained with the indicated antibodies and analyzed by flow cytometry. The percentages of gated cells are shown. Data are representative of 4 independent experiments. (B) Expression of inhibitory receptors as well as activating receptors on NK1.1+TCRab- NK cells from MIST-deficient mice. Histograms indicate expression of various inhibitory receptors (Ly receptors and CD94) and other activating receptors (NK1.1 and CD16) on NK cells in MIST-deficient (-/-) and wild-type NK cells (+/+). The gate used to calculate the percentage of cells expressing each receptor is shown by a horizontal line above each histogram. All histograms are representative of analyses from at least 3 mice of each genotype. (C) Flow cytometric analysis of knock-in EGFP fluorescence in spleen cells left unstimulated (arrows) or stimulated with α-GalCer (arrowheads) for 12 hours. FACS plot is shown for each set of markers, because there were no significant differences in phenotype between wild-type and MIST+/Δneo mice. For each of the gated populations indicated, histograms for EGFP fluorescence were generated. Wild-type histograms (dotted lines) were overlaid with mutant histograms (solid lines).

MIST is dispensable for development of NK and NKT cells. (A) Cells isolated from liver (left) and spleen (right) of 4- to 6-week-old MIST-deficient mice (-/-) and their littermates (+/+) were stained with the indicated antibodies and analyzed by flow cytometry. The percentages of gated cells are shown. Data are representative of 4 independent experiments. (B) Expression of inhibitory receptors as well as activating receptors on NK1.1+TCRab- NK cells from MIST-deficient mice. Histograms indicate expression of various inhibitory receptors (Ly receptors and CD94) and other activating receptors (NK1.1 and CD16) on NK cells in MIST-deficient (-/-) and wild-type NK cells (+/+). The gate used to calculate the percentage of cells expressing each receptor is shown by a horizontal line above each histogram. All histograms are representative of analyses from at least 3 mice of each genotype. (C) Flow cytometric analysis of knock-in EGFP fluorescence in spleen cells left unstimulated (arrows) or stimulated with α-GalCer (arrowheads) for 12 hours. FACS plot is shown for each set of markers, because there were no significant differences in phenotype between wild-type and MIST+/Δneo mice. For each of the gated populations indicated, histograms for EGFP fluorescence were generated. Wild-type histograms (dotted lines) were overlaid with mutant histograms (solid lines).

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