Figure 5.
Modulation of GSH level and its relationship with apoptosis. (A-B) Relative GSH levels, as determined by monochlorobimane derivatization, in U-937 cell cultures treated for 24 hours with LY294002 and the indicated concentrations of As2O3, alone and in combination (A); and in U-937 and NB4 cell cultures treated for the indicated time periods with 4 μM (U-937) and 2 μM (NB4) As2O3 alone, with LY294002 alone, and with As2O3 plus either LY294002, wortmannin, or Akti5 (B). All results are expressed in relation to untreated U-937 cell cultures (approximate GSH content, 9 nmol/106 cells), which received the arbitrary value of one. (C) Frequency of apoptotic cells in U-937 cell cultures treated for 24 hours with BSO alone, and with As2O3, camptothecin, cisplatin, and lonidamine, either alone (-) or in combination with BSO. (D) Relative GSH levels in U-937 cells treated for 24 hours with LY294002, with BSO, and with the combination of As2O3 plus either LY294002, TPA, or ascorbic acid (AA), in the absence (-) or the presence of NAC (+NAC). (E) Frequency of apoptotic cells in U-937 cell cultures treated for 24 hours with As2O3 alone, TPA alone, AA alone, and NAC alone, and with the combinations of As2O3 plus either LY294002, TPA, or AA, in the absence (-) or the presence of NAC. BSO, TPA, AA, and NAC were used at 1 mM, 20 nM, 150 μM, and 10 mM, respectively. All drugs were applied simultaneously. The data represent the means ± standard deviation of at least 3 determinations. All other conditions were as in Figure 1.