Figure 2
Figure 2. IL-15 administration expands multiple subsets of NK and memory T cells. (A) Gating strategy used for the identification of NK-cell subsets. A first gate on time versus fluorescence was drawn to exclude artifacts and singlets were selected on the basis of FSC-A and FSC-H. Monocytes and dead cells were excluded by gating on CD14–/ViViD– cells. Within the lymphocyte gate, NK cells were defined as those negative for CD3 and CD20 and positive for either CD56 or CD16. Two major NK-cell subsets could be identified in the RM: CD56+CD16− and CD56−CD16+ NK cells. (B) Left, dynamics of NK-cell subsets after treatment with IL-15. Data from the different dose groups were indicated as in Figure 1. Right, 1 representative example of the dynamics of NKG2D, NKG2A, NKp80, and NKp46 expression in a RM receiving the 50-μg/kg/d dose. Data relative to baseline, day 8 and day 48 after treatment are shown from the 2 identified subsets of NK cells. (C) Gating strategy used for the identification of naive and memory T-cell subsets. Monocytes and dead cells were excluded as in panel A, and T cells were further selected for CD3+ positivity. Within the lymphocyte gate, CD4+ and CD8+ cells were identified (CD8+ T cells only are shown for more clarity). For both lineages, total memory cells are defined as those expressing CD95, while CD95- (almost exclusively CD45RA bright) naive (TN) cells are further restricted as CD28+ and CCR7+. Within the memory cell gate, central memory (TCM) are CCR7+CD28+, transitional memory (TTM) are CCR7–CD28+, and total effectors (TEff) are CCR7–CD28– and could be then subdivided into effector memory (TEM; not expressing CD45RA) or terminal effectors (TTE, expressing CD45RA). (B) Dynamics of TN and memory T-cell subset counts in the peripheral blood after treatment with IL-15. Data from the different dose groups are shown as in Figure 1. *P < .05 for Wilcoxon rank test in IL-15–treated versus sham.

IL-15 administration expands multiple subsets of NK and memory T cells. (A) Gating strategy used for the identification of NK-cell subsets. A first gate on time versus fluorescence was drawn to exclude artifacts and singlets were selected on the basis of FSC-A and FSC-H. Monocytes and dead cells were excluded by gating on CD14/ViViD cells. Within the lymphocyte gate, NK cells were defined as those negative for CD3 and CD20 and positive for either CD56 or CD16. Two major NK-cell subsets could be identified in the RM: CD56+CD16 and CD56CD16+ NK cells. (B) Left, dynamics of NK-cell subsets after treatment with IL-15. Data from the different dose groups were indicated as in Figure 1. Right, 1 representative example of the dynamics of NKG2D, NKG2A, NKp80, and NKp46 expression in a RM receiving the 50-μg/kg/d dose. Data relative to baseline, day 8 and day 48 after treatment are shown from the 2 identified subsets of NK cells. (C) Gating strategy used for the identification of naive and memory T-cell subsets. Monocytes and dead cells were excluded as in panel A, and T cells were further selected for CD3+ positivity. Within the lymphocyte gate, CD4+ and CD8+ cells were identified (CD8+ T cells only are shown for more clarity). For both lineages, total memory cells are defined as those expressing CD95, while CD95- (almost exclusively CD45RA bright) naive (TN) cells are further restricted as CD28+ and CCR7+. Within the memory cell gate, central memory (TCM) are CCR7+CD28+, transitional memory (TTM) are CCR7CD28+, and total effectors (TEff) are CCR7CD28 and could be then subdivided into effector memory (TEM; not expressing CD45RA) or terminal effectors (TTE, expressing CD45RA). (B) Dynamics of TN and memory T-cell subset counts in the peripheral blood after treatment with IL-15. Data from the different dose groups are shown as in Figure 1. *P < .05 for Wilcoxon rank test in IL-15–treated versus sham.

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