Figure 1.
Energetic substrate use in NKDim vs NKBr cells at steady state and upon activation. (A) In vitro model of NKBr and NKDim cell priming and activation. (B-D) Freshly fluorescence-activated cell-sorted NKDim and NKBr cells, IL-15 primed or activated with IL-15/12/18 (18 h) were monitored for cell-surface expression of the GLUT-1 and ASCT2 transporters and percentage of positive cells (B) (data from 3 independent experiments with 1 HD each) and FL-BODIPY-C16 uptake (C) (data from 3 independent experiments with 1 or 2 HDs each). (D) Expression of IFN-γ and percentage of IFN-γ–producing cells were monitored in NKBr and NKDim cells incubated with IL-15 or IL-15/12/18 for 18 hours in the presence of different inhibitors: 1 mM of 2-DG, 4 μM of BPTES, or 20 μM of ETO (data are mean ± standard error of the mean [SEM]; data summarized from 3 independent experiments with at least 2 HDs each). P > .05 was considered not significant (ns). *P < .05, **P < .01, ***P < .001, ****P < .0001 using 2-way analysis of variance with Tukey’s correction. MFI, mean fluorescence intensity.

Energetic substrate use in NKDim vs NKBr cells at steady state and upon activation. (A) In vitro model of NKBr and NKDim cell priming and activation. (B-D) Freshly fluorescence-activated cell-sorted NKDim and NKBr cells, IL-15 primed or activated with IL-15/12/18 (18 h) were monitored for cell-surface expression of the GLUT-1 and ASCT2 transporters and percentage of positive cells (B) (data from 3 independent experiments with 1 HD each) and FL-BODIPY-C16 uptake (C) (data from 3 independent experiments with 1 or 2 HDs each). (D) Expression of IFN-γ and percentage of IFN-γ–producing cells were monitored in NKBr and NKDim cells incubated with IL-15 or IL-15/12/18 for 18 hours in the presence of different inhibitors: 1 mM of 2-DG, 4 μM of BPTES, or 20 μM of ETO (data are mean ± standard error of the mean [SEM]; data summarized from 3 independent experiments with at least 2 HDs each). P > .05 was considered not significant (ns). *P < .05, **P < .01, ***P < .001, ****P < .0001 using 2-way analysis of variance with Tukey’s correction. MFI, mean fluorescence intensity.

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