Figure 2
Figure 2. Effect of frataxin deficiency on mitochondrial redox potential, ROS generation, and MMP. (A) T-rex cells were transfected with a construct encoding for the redox potential reporting ratiometric roGFP2 protein, which was fused to a mitochondrial targeting sequence. After 6 days with (Tet+) or without tetracycline induction, the cells were analyzed by confocal microscopy (left panel), using ratiometric fluorescence at 405/488 excitation ratios (see lookup table in pseudo-image color in the “Tet+” image) and 520 nm emission. Scale bar represents 10 μm. (Right panel) Redox potentials calculated from the roGFP2 405/488 excitation ratios normalized to the range between maximal (10 mM H2O2) and minimal (10 mM DTT) oxidation, in combination with the nonlinear regression fit to an in situ calibration curve, f = 0.0509 + 0.8305/(1 + exp(−(x = 249.5422)/6.6161)). Mitochondrial redox potential in Tet+ cells was significantly higher than in untreated cells (n = 3 experiments, P < .05, one-way ANOVA with Dunnett post-hoc test). (B,C) T-rex cells, treated (Tet+) or not with tetracycline for 6 days (left panels) or for the durations indicated (right panels), were labeled with (B) the ROS-sensitive agent CDCF-DA-AM (10 μM) or (C) the MMP potentiometric probe TMRE (0.2 μM). Cells were examined by confocal microscopy using (B) the 405 excitation/488 emission filter set for CDCF (green) or (C) the 543 excitation/633 emission filter set for TMRE (red). (Right panels) Data are from similar fluorescence microscopy analyses of cells treated with Tet for 0 to 9 days. CDCF fluorescence was higher and TMRE fluorescence was lower in Tet+ cells compared with noninduced cells (n = 3 experiments, P < .05, one-way ANOVA with Dunnett post-hoc test). The average number of mitochondria punctae per cell in Tet+ cells was 235 plus or minus 90, significantly higher (P < .05, unpaired, 2-tailed t test) than in noninduced cells, where it was 66 plus or minus 54. Scale bars represent 10 μm.

Effect of frataxin deficiency on mitochondrial redox potential, ROS generation, and MMP. (A) T-rex cells were transfected with a construct encoding for the redox potential reporting ratiometric roGFP2 protein, which was fused to a mitochondrial targeting sequence. After 6 days with (Tet+) or without tetracycline induction, the cells were analyzed by confocal microscopy (left panel), using ratiometric fluorescence at 405/488 excitation ratios (see lookup table in pseudo-image color in the “Tet+” image) and 520 nm emission. Scale bar represents 10 μm. (Right panel) Redox potentials calculated from the roGFP2 405/488 excitation ratios normalized to the range between maximal (10 mM H2O2) and minimal (10 mM DTT) oxidation, in combination with the nonlinear regression fit to an in situ calibration curve, f = 0.0509 + 0.8305/(1 + exp(−(x = 249.5422)/6.6161)). Mitochondrial redox potential in Tet+ cells was significantly higher than in untreated cells (n = 3 experiments, P < .05, one-way ANOVA with Dunnett post-hoc test). (B,C) T-rex cells, treated (Tet+) or not with tetracycline for 6 days (left panels) or for the durations indicated (right panels), were labeled with (B) the ROS-sensitive agent CDCF-DA-AM (10 μM) or (C) the MMP potentiometric probe TMRE (0.2 μM). Cells were examined by confocal microscopy using (B) the 405 excitation/488 emission filter set for CDCF (green) or (C) the 543 excitation/633 emission filter set for TMRE (red). (Right panels) Data are from similar fluorescence microscopy analyses of cells treated with Tet for 0 to 9 days. CDCF fluorescence was higher and TMRE fluorescence was lower in Tet+ cells compared with noninduced cells (n = 3 experiments, P < .05, one-way ANOVA with Dunnett post-hoc test). The average number of mitochondria punctae per cell in Tet+ cells was 235 plus or minus 90, significantly higher (P < .05, unpaired, 2-tailed t test) than in noninduced cells, where it was 66 plus or minus 54. Scale bars represent 10 μm.

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