The effect of ethyldeshydroxy-sparsomycin and cisplatin on the intracellular glutathione level and glutathione S-transferase activity

被引:4
|
作者
Hofs, HP
Wagener, TDJ
deValkBakker, V
vanRennes, H
Doesburg, WH
Ottenheijm, HCJ
deGrip, WJ
机构
[1] UNIV NIJMEGEN HOSP,DEPT INTERNAL MED,DIV MED ONCOL,NL-6500 HB NIJMEGEN,NETHERLANDS
[2] CATHOLIC UNIV NIJMEGEN,DEPT MED STAT,NL-6500 HC NIJMEGEN,NETHERLANDS
[3] CATHOLIC UNIV NIJMEGEN,DEPT ORGAN CHEM,NL-6500 HC NIJMEGEN,NETHERLANDS
[4] CATHOLIC UNIV NIJMEGEN,DEPT BIOCHEM,NL-6500 HC NIJMEGEN,NETHERLANDS
关键词
cisplatin; drug-resistance; glutathione S-transferase; glutathione; sparsomycin;
D O I
10.1097/00001813-199704000-00007
中图分类号
R73 [肿瘤学];
学科分类号
100214 ;
摘要
Ethyldeshydroxy-sparsomycin (EdSm) is a ribosomal protein synthesis inhibitor which synergistically enhances the antitumor activity of cisplatin against L1210 leukemia in vivo. Because cellular glutathione (GSH) and glutathione S-transferases (GST) are reported to interfere with the antitumor activity of cisplatin, we analyzed the effect of EdSm and cisplatin on GSH and GST activity in selected tumor cells. For this purpose we used three murine leukemia tumors with different sensitivities towards EdSm and cisplatin: L1210-WT, sensitive to both drugs, L1210-Sm, resistant to EdSm, and L1210-CDDP, resistant to cisplatin. No significant differences were detectable between these three cell lines regarding the population doubling time, the cell size, and the cellular level of protein and glutathione. Neither of the resistant L1210 subclones showed P-glycoprotein expression. Drug exposure, however, changed the intracellular dynamics. Exposure to EdSm strongly decreased the amount of cellular protein, decreased the overall GST activity and led to GSH depletion, whereas exposure to cisplatin induced a rise in the amount of protein, in GSH, and in the total GST activity. These effects are dose-dependent and correlate well with the sensitivity of the tumor cells for EdSm or cisplatin. In addition, exposure to EdSm lowered the V-max of GST in L1210-WT and L1210-Sm; however, in L1210-CDDP both the V-max and the K-m were increased. That this was not a direct effect of EdSm on GST was shown in a cell-free system, where EdSm did not influence the GST activity nor could it act as a substrate for GST. Our results suggest that the synergistic combination of EdSm and cisplatin might be explained by EdSm switching off the cellular detoxification mechanism for cisplatin, i.e. by inhibition of de novo synthesis and subsequent depletion of GSH and GST.
引用
收藏
页码:349 / 357
页数:9
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