![Glutamine supports both mitochondrial function and glutathione production following FLT3 TK inhibition. (A) Total and isotopologue levels of TCA cycle intermediates, glutamate and reduced glutathione (GSH), measured by LC-MS analysis in MV411 cells treated with AC220 1 nM or vehicle control and grown in media containing U-13C5 and 15nitrogen [15N2] glutamine (GLN) (mean ± SEM, n = 5; ***P = .0005, **P = .0017, *P = .0195 for citrate, P = .0228 for malate, P = .0216 for glutamate; ns, not significant; 2-tailed, paired Student t test). A schematic representation of glutamine metabolism and labeling pattern of metabolites is also provided. (B) Percentage of total levels of TCA cycle metabolites labeled by U-13C5,15N2-GLN through its oxidative metabolism measured by LC-MS analysis in MV411 cells treated with AC220 1 nM or vehicle control (mean ± SEM, n = 5; ****P < .0001, ***P = .0008, **P = .0067; 2-way ANOVA with Bonferroni’s multiple comparisons). (C) Relative mitochondrial membrane potential of MV411 cells treated with AC220 1 nM or vehicle control (left) with representative flow cytometry histogram (right) (mean ± SEM, n = 3; * P = .0145; 2-tailed, paired Student t test). (D) Relative mitochondrial mass of MV411 cells treated with AC220 1 nM or vehicle control (left) with representative flow cytometry histogram (right panel) (mean ± SEM, n = 3; ns, not significant; P = .13; 2-tailed paired t test). (E) Relative GSH/GSSG ratio, GSH, and GSSG of MV411 cells treated with AC220 1 nM or vehicle control (mean ± SEM, n = 6; * P = .0173; ns, not significant; 2-tailed, paired Student t test). (F) Percentage of total levels of glutamine, glutamate, GSH, and GSSG labeled by U-13C5,15N2-GLN measured by LC-MS analysis in MV411 cells treated as in panel A (mean ± SEM, n = 5; **** P < .0001; ns, not significant; 2-way ANOVA with Bonferroni’s multiple comparisons. (G) Relative GSH levels of MV411 cells treated with AC220 1 nM or vehicle control in the presence or absence of glutamine (mean ± SEM, n = 5; **P = .0017, *P = .0471, q = 4.248; ANOVA with Tukey’s multiple comparisons). (H) Relative cytoplasmic ROS levels of MV411 cells treated with AC220 1 nM or vehicle control in the presence or absence of glutamine (mean ± SEM, n = 14; ****P < .0001; ANOVA with Tukey’s multiple comparisons).](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/131/15/10.1182_blood-2017-12-820035/4/blood820035f3-2.jpeg?Expires=1721698958&Signature=j1dPZZ2goLLZDGhMxptVBMu6FDfQYLEhiXXwDSsl9~2pYWzwnCaooLH518q4xa2EaLWdh~D5vCDWmomSwHQvPgAz7J3ViYFxa~3QWXVGzFcxErxw3W2sbF9cqtlubNIWaU1FhiPue8NYIL1eDZ0ggbVgFh5f9Mu3ddhqiO~R1Bz8goijbbaSI3Egjq9dSzEbUWwONBvGHIgaB5513M0KBG2r-qpNThtIO0JJrb0bkbCAFCYHLu9Esn0AK6PX2X5yGVy2MH~Pmndh5Wc07TRP6LRCzgWLzypATHVBHToEP7wy98VtuKzlqjbYJJAFJ8u0D2yLr8rVDSRLBTwH7doeww__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Glutamine supports both mitochondrial function and glutathione production following FLT3 TK inhibition. (A) Total and isotopologue levels of TCA cycle intermediates, glutamate and reduced glutathione (GSH), measured by LC-MS analysis in MV411 cells treated with AC220 1 nM or vehicle control and grown in media containing U-13C5 and 15nitrogen [15N2] glutamine (GLN) (mean ± SEM, n = 5; ***P = .0005, **P = .0017, *P = .0195 for citrate, P = .0228 for malate, P = .0216 for glutamate; ns, not significant; 2-tailed, paired Student t test). A schematic representation of glutamine metabolism and labeling pattern of metabolites is also provided. (B) Percentage of total levels of TCA cycle metabolites labeled by U-13C5,15N2-GLN through its oxidative metabolism measured by LC-MS analysis in MV411 cells treated with AC220 1 nM or vehicle control (mean ± SEM, n = 5; ****P < .0001, ***P = .0008, **P = .0067; 2-way ANOVA with Bonferroni’s multiple comparisons). (C) Relative mitochondrial membrane potential of MV411 cells treated with AC220 1 nM or vehicle control (left) with representative flow cytometry histogram (right) (mean ± SEM, n = 3; * P = .0145; 2-tailed, paired Student t test). (D) Relative mitochondrial mass of MV411 cells treated with AC220 1 nM or vehicle control (left) with representative flow cytometry histogram (right panel) (mean ± SEM, n = 3; ns, not significant; P = .13; 2-tailed paired t test). (E) Relative GSH/GSSG ratio, GSH, and GSSG of MV411 cells treated with AC220 1 nM or vehicle control (mean ± SEM, n = 6; * P = .0173; ns, not significant; 2-tailed, paired Student t test). (F) Percentage of total levels of glutamine, glutamate, GSH, and GSSG labeled by U-13C5,15N2-GLN measured by LC-MS analysis in MV411 cells treated as in panel A (mean ± SEM, n = 5; **** P < .0001; ns, not significant; 2-way ANOVA with Bonferroni’s multiple comparisons. (G) Relative GSH levels of MV411 cells treated with AC220 1 nM or vehicle control in the presence or absence of glutamine (mean ± SEM, n = 5; **P = .0017, *P = .0471, q = 4.248; ANOVA with Tukey’s multiple comparisons). (H) Relative cytoplasmic ROS levels of MV411 cells treated with AC220 1 nM or vehicle control in the presence or absence of glutamine (mean ± SEM, n = 14; ****P < .0001; ANOVA with Tukey’s multiple comparisons).
