Figure 4
Figure 4. NKp80+ CD8 T cells are potent effectors. (A,B) Enhanced expression of cytotoxic effector proteins perforin and granzyme B by NKp80+ CD8 T cells. Flow cytometric analysis of freshly isolated PBMCs gated on CD3+CD8+ cells for coexpression of NKp80 and intracellular perforin or granzyme B, respectively. (A) Representative dot plot analysis of 1 donor and (B) compiled MFI data for 8 healthy donors are shown. Lines indicate MFI values derived from same donors. (C,D) High responsiveness of NKp80+ CD8 T cells. Freshly purified CD8+ cells were stimulated with PMA/ionomycin for 6 hours and stained for CD107a or intracellular IFNγ in conjunction with NKp80. CD3+CD8+ T cells were gated for flow cytometric analysis. Dot plots (C) and means and standard deviations (D) of triplicates for one representative donor. Similar results were obtained with 2 other donors (not shown). (E) Multiple cytokine expression by NKp80+ CD8 T cells. Freshly isolated PBMCs were stimulated with PMA/ionomycin for 6 hours and simultaneously stained for intracellular IFN-γ, TNF, and IL-2. CD3+CD8+CCR7− T cells were gated for flow cytometric analysis of cytokine expression by NKp80+ and NKp80− cells, respectively. Means and standard deviations of frequencies of T-cell subsets expressing different combinations of cytokines are shown for 1 representative donor. Similar data were obtained with 3 other donors. (F) Fresh PBMCs were stained with CFSE and cultured for 8 days in the presence of IL-2, IL-7, and IL-15. On day 8, NKp80+CD3+ and NKp80−CD3+ cells were gated (left) and analyzed for CFSE levels (right). Data are representative of 5 experiments.

NKp80+ CD8 T cells are potent effectors. (A,B) Enhanced expression of cytotoxic effector proteins perforin and granzyme B by NKp80+ CD8 T cells. Flow cytometric analysis of freshly isolated PBMCs gated on CD3+CD8+ cells for coexpression of NKp80 and intracellular perforin or granzyme B, respectively. (A) Representative dot plot analysis of 1 donor and (B) compiled MFI data for 8 healthy donors are shown. Lines indicate MFI values derived from same donors. (C,D) High responsiveness of NKp80+ CD8 T cells. Freshly purified CD8+ cells were stimulated with PMA/ionomycin for 6 hours and stained for CD107a or intracellular IFNγ in conjunction with NKp80. CD3+CD8+ T cells were gated for flow cytometric analysis. Dot plots (C) and means and standard deviations (D) of triplicates for one representative donor. Similar results were obtained with 2 other donors (not shown). (E) Multiple cytokine expression by NKp80+ CD8 T cells. Freshly isolated PBMCs were stimulated with PMA/ionomycin for 6 hours and simultaneously stained for intracellular IFN-γ, TNF, and IL-2. CD3+CD8+CCR7 T cells were gated for flow cytometric analysis of cytokine expression by NKp80+ and NKp80 cells, respectively. Means and standard deviations of frequencies of T-cell subsets expressing different combinations of cytokines are shown for 1 representative donor. Similar data were obtained with 3 other donors. (F) Fresh PBMCs were stained with CFSE and cultured for 8 days in the presence of IL-2, IL-7, and IL-15. On day 8, NKp80+CD3+ and NKp80CD3+ cells were gated (left) and analyzed for CFSE levels (right). Data are representative of 5 experiments.

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