TPEN induces mitochondrial depolarization, plasma membrane damage, and chromatin fragmentation in Jurkat cells. ((a)–(c)) Jurkat cells (1 × 10⁶ cells/mL) were incubated with TPEN (3 μM) at 37°C for 1, 3, 6, 12, and 24 h. The cells were then used for several assays. (a) Representative histograms showing SubG₁ cell population indicative of DNA fragmentation after TPEN treatment, as described in according to Material and Methods section (b) Representative density (dot) plots showing PI/DiOC₆(3) percentage of four different cell populations under TPEN treatment, as described in Material and Methods section. (c) Representative density (dot) plots showing annexin V/7-AAD percentage of four different cell populations under TPEN exposure, as described Material and Methods section. Circled number is the mean percentage of three independent experiments. S.D. values were below ±5% (also for Figures 5 and 6) of the mean values and are not shown.