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在暴露于亚致死浓度叔丁基过氧化氢的U937细胞中,钙依赖性线粒体形成介导DNA单链断裂的物质。

Calcium-dependent mitochondrial formation of species mediating DNA single strand breakage in U937 cells exposed to sublethal concentrations of tert-butylhydroperoxide.

作者信息

Guidarelli A, Clementi E, Sciorati C, Cattabeni F, Cantoni O

机构信息

Istituto di Farmacologia e Farmacognosia, Università di Urbino, Italy.

出版信息

J Pharmacol Exp Ther. 1997 Oct;283(1):66-74.

PMID:9336309
Abstract

Treatment of U937 cells with a sublethal albeit DNA-damaging concentration of tert-butylhydroperoxide (tB-OOH) enhanced mitochondrial Ca++ uptake and ruthenium red (RR), a polycation that inhibits the calcium uniporter of mitochondria, significantly reduced the extent of DNA cleavage generated by the hydroperoxide. Release of Ca++ from the ryanodine(Ry)/caffeine(Cf)-sensitive stores further increased mitochondrial Ca++ uptake and elicited a parallel enhancement in DNA strand scission induced by tB-OOH that was prevented by both Ry and RR. DNA damage caused by tB-OOH alone or associated with either Cf or RR was prevented by iron chelators, insensitive to antioxidants and repaired with kinetics superimposable with those observed after treatment with H2O2. Cf enhanced the DNA-damaging effects of tB-OOH in permeabilized cells as well, and similar effects were observed upon addition of CaCl2. Cf did not further increase the formation of DNA lesions elicited by tB-OOH in the presence of CaCl2. The enhancing effects of Cf were prevented by RR and ryanodine, whereas those mediated by exogenous calcium were prevented only by RR. DNA strand scission caused by tB-OOH alone or associated with Cf in the permeabilized cell system was severely inhibited by ethylene glycol-bis(beta-aminoethyl ether)-N, N,N',N'-tetraacetic acid. The mechanism(s) whereby Ca++ promotes the mitochondrial formation of species that will ultimately result in the formation of DNA lesions was subsequently analyzed using intact as well as permeabilized cells. Hydrogen peroxide was identified to be one of these species.

摘要

用亚致死剂量但具有DNA损伤作用的叔丁基过氧化氢(tB - OOH)处理U937细胞,可增强线粒体对钙离子的摄取,而钌红(RR)是一种抑制线粒体钙单向转运体的聚阳离子,它能显著降低过氧化氢引起的DNA切割程度。从ryanodine(Ry)/咖啡因(Cf)敏感储存库释放的钙离子进一步增加了线粒体对钙离子的摄取,并引发了由tB - OOH诱导的DNA链断裂的平行增强,而Ry和RR均可阻止这种增强。单独的tB - OOH或与Cf或RR相关联引起的DNA损伤可被铁螯合剂阻止,铁螯合剂对抗氧化剂不敏感,其修复动力学与用H2O2处理后观察到的动力学叠加。Cf也增强了tB - OOH对通透细胞的DNA损伤作用,添加氯化钙时也观察到类似的效果。在存在氯化钙的情况下,Cf不会进一步增加tB - OOH引起的DNA损伤的形成。RR和ryanodine可阻止Cf的增强作用,而外源性钙介导的增强作用仅被RR阻止。在通透细胞系统中,单独的tB - OOH或与Cf相关联引起的DNA链断裂被乙二醇双(β - 氨基乙基醚)- N,N,N',N'-四乙酸严重抑制。随后使用完整细胞和通透细胞分析了钙离子促进最终导致DNA损伤形成的线粒体物种形成的机制。过氧化氢被确定为这些物种之一。

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