Figure 1.
Figure 1. NK cytolytic activity is dependent on LFA-1. (A) Fresh lymphocytes were tested for natural cytolysis of CMFDA-labeled K562 or Daudi tumor cell lines in a 4-hour flow cytometric killing assay at 1:12.5 target cell/NK cell target ratio. Samples were incubated with α-NKG2D, α-KIR, or α–LFA-1 (clone TS1/22) antibodies (10 μg/mL). (B) Lymphocytes were treated with IL-2 or IL-12 (200 ng/mL) for 12 hours and incubated with K562 targets at the indicated target/NK ratio and specific lysis was assessed by flow cytometry. (C) Lymphocytes were treated with IL-2 (200 ng/mL) or ICAM-2 (1 μg) and incubated with CMDFA-labeled K562 cells. Lymphocytes were prestained with CD56-PerCPCy5.5 for 10 minutes, mixed with K562 cells at 1:12.5 target cell/NK ratio for 10 minutes, and fixed directly in 2% PFA. Conjugates were assessed as previously described.20 (D) PBMCs depleted for adherent cells were stained for surface CD3-PerCPCy5.5, CD8-PE, CD56-APC, and intracellular perforin-FITC expression. Quadrant gating for CD3 and CD8 is color coded and displayed on CD56 and perforin parameters for gated populations. Distinction between CD56bright and CD56dim and the distinctions among perforin low, medium, and high levels are displayed. Subset frequencies for intracellular perforin levels in CD3+/–CD8+/–CD56+/– subsets are displayed in Table 1. Numbers in each quadrant correspond to population frequencies within those quadrants. (E) ICAM binding to CD56+CD8+ NK cells and CD3+CD8+ cells. The 1 × 106 cells that were cultured in the presence or absence of IL-2 (100 ng/mL, 12 hours) were labeled with ICAM-1, ICAM-2, or ICAM-3 fusion proteins (1.25 μg) at 37°C for 15 minutes in the presence of mouse IgG MOPC21 (4 μg/mL) and human sera. Cells were washed and stained with goat antihuman FC-AX488 (Fab′)2, and CD56-PE, CD8-PerCPCy5.5, and CD3-APC. Geometric means for ICAM-AX488 are displayed for CD3– CD56+CD8+ and CD3+CD8+ gated populations. Error bars in panels A, C, and E indicate standard deviation of at least 3 experiments.

NK cytolytic activity is dependent on LFA-1. (A) Fresh lymphocytes were tested for natural cytolysis of CMFDA-labeled K562 or Daudi tumor cell lines in a 4-hour flow cytometric killing assay at 1:12.5 target cell/NK cell target ratio. Samples were incubated with α-NKG2D, α-KIR, or α–LFA-1 (clone TS1/22) antibodies (10 μg/mL). (B) Lymphocytes were treated with IL-2 or IL-12 (200 ng/mL) for 12 hours and incubated with K562 targets at the indicated target/NK ratio and specific lysis was assessed by flow cytometry. (C) Lymphocytes were treated with IL-2 (200 ng/mL) or ICAM-2 (1 μg) and incubated with CMDFA-labeled K562 cells. Lymphocytes were prestained with CD56-PerCPCy5.5 for 10 minutes, mixed with K562 cells at 1:12.5 target cell/NK ratio for 10 minutes, and fixed directly in 2% PFA. Conjugates were assessed as previously described.20 (D) PBMCs depleted for adherent cells were stained for surface CD3-PerCPCy5.5, CD8-PE, CD56-APC, and intracellular perforin-FITC expression. Quadrant gating for CD3 and CD8 is color coded and displayed on CD56 and perforin parameters for gated populations. Distinction between CD56bright and CD56dim and the distinctions among perforin low, medium, and high levels are displayed. Subset frequencies for intracellular perforin levels in CD3+/–CD8+/–CD56+/– subsets are displayed in Table 1. Numbers in each quadrant correspond to population frequencies within those quadrants. (E) ICAM binding to CD56+CD8+ NK cells and CD3+CD8+ cells. The 1 × 106 cells that were cultured in the presence or absence of IL-2 (100 ng/mL, 12 hours) were labeled with ICAM-1, ICAM-2, or ICAM-3 fusion proteins (1.25 μg) at 37°C for 15 minutes in the presence of mouse IgG MOPC21 (4 μg/mL) and human sera. Cells were washed and stained with goat antihuman FC-AX488 (Fab′)2, and CD56-PE, CD8-PerCPCy5.5, and CD3-APC. Geometric means for ICAM-AX488 are displayed for CD3 CD56+CD8+ and CD3+CD8+ gated populations. Error bars in panels A, C, and E indicate standard deviation of at least 3 experiments.

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