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在过表达p185(erbB - 2)的细胞中,细胞对顺铂诱导的DNA损伤和DNA修复的反应调节依赖于ras信号通路。

Regulation of cellular response to cisplatin-induced DNA damage and DNA repair in cells overexpressing p185(erbB-2) is dependent on the ras signaling pathway.

作者信息

Yen L, Nie Z R, You X L, Richard S, Langton-Webster B C, Alaoui-Jamali M A

机构信息

Lady Davis Institute of the Sir Mortimer B Davis Jewish General Hospital, Department of Medicine, McGill University, Montreal, Canada.

出版信息

Oncogene. 1997 Apr 17;14(15):1827-35. doi: 10.1038/sj.onc.1201019.

DOI:10.1038/sj.onc.1201019
PMID:9150389
Abstract

We have examined the role of erbB-2 expression in the modulation of cellular toxicity to cisplatin. We have demonstrated that treatment of NIH3T3-erbB-2 cells, which overexpress the p185(erbB-2) product of the human erbB-2 gene, with a monoclonal antibody directed against the extracellular domain (TAb-250), results in enhanced cisplatin cytotoxicity. A similar enhancement was obtained when cells were exposed to herbimycin A and its analogue CP127 374, both of which inhibit tyrosine kinase activity. Using the host cell reactivation (HCR) of reporter gene expression from cisplatin-damaged plasmid and unscheduled DNA synthesis (UDS) following cisplatin treatment of cells, we have found that modulation of erbB-2 by TAb-250 was associated with inhibition of DNA repair. TAb-250 alone, under conditions which modulate DNA repair, slightly reduces the S-phase of the cell cycle, while cisplatin induced arrest at S and G2 phases. Combination of TAb-250 and cisplatin only slightly prevented cisplatin-induced S and G2 blocks. Since the ras pathway is one of the major signaling components coupled to erbB-2, we have examined the role of ras in DNA repair regulation. Transient expression of a ras dominant negative mutant, Asn-17-ras(H), prevents DNA repair modulation by TAb-250, suggesting that the erbB-2 receptor regulates DNA repair mechanism(s), at least in part, through ras-coupled pathway(s).

摘要

我们研究了erbB - 2表达在调节细胞对顺铂毒性反应中的作用。我们已经证明,用一种针对细胞外结构域的单克隆抗体(TAb - 250)处理过表达人erbB - 2基因p185(erbB - 2)产物的NIH3T3 - erbB - 2细胞,会增强顺铂的细胞毒性。当细胞暴露于抑制酪氨酸激酶活性的除草霉素A及其类似物CP127 374时,也能获得类似的增强效果。利用顺铂损伤质粒的报告基因表达的宿主细胞再激活(HCR)以及顺铂处理细胞后的非定标DNA合成(UDS),我们发现TAb - 250对erbB - 2的调节与DNA修复的抑制有关。在调节DNA修复的条件下,单独的TAb - 250会轻微降低细胞周期的S期,而顺铂会诱导细胞在S期和G2期停滞。TAb - 250与顺铂联合使用仅轻微阻止了顺铂诱导的S期和G2期阻滞。由于ras途径是与erbB - 2偶联的主要信号传导成分之一,我们研究了ras在DNA修复调节中的作用。ras显性负突变体Asn - 17 - ras(H)的瞬时表达可阻止TAb - 250对DNA修复的调节,这表明erbB - 2受体至少部分地通过ras偶联途径调节DNA修复机制。

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