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核糖核苷酸还原酶表达的改变以及M2基因扩增在羟基脲抗性仓鼠、小鼠、大鼠和人类细胞系中的作用。

Altered expression of ribonucleotide reductase and role of M2 gene amplification in hydroxyurea-resistant hamster, mouse, rat, and human cell lines.

作者信息

Wright J A, Alam T G, McClarty G A, Tagger A Y, Thelander L

出版信息

Somat Cell Mol Genet. 1987 Mar;13(2):155-65. doi: 10.1007/BF01534695.

Abstract

Five hamster, mouse, and rat cell lines resistant to the cytotoxic effects of hydroxyurea have been characterized. All cell lines contained increased ribonucleotide reductase activity, elevated levels of the M2 component of ribonucleotide reductase as judged by electron paramagnetic resonance spectroscopy, and increased copies of M2 mRNA as determined by Northern blot analysis. Two species of M2 mRNA were detected in rodent cell lines, a high-molecular-weight species of approximately 3.4 kb in hamster and rat cells and about 2.1 kb in mouse cells. The low molecular-weight M2 mRNA was about 1.6 kb in all rodent lines. Northern blot analysis showed that the mRNA for the other component of ribonucleotide reductase, M1, was not markedly elevated in the drug-resistant cells and existed as a single 3.1-kb species. Four of the five resistant lines contained an M2 gene amplification as determined by Southern blot analysis, providing direct evidence to support earlier suggestions that hydroxyurea resistance is often accompanied by amplification of a ribonucleotide reductase gene. An increase in gene dosage was detected even in cells exhibiting only modest drug-resistance properties. No evidence for amplification of the M1 gene of ribonucleotide reductase was found. In keeping with these observations with drug-resistant rodent lines, a human (HeLa) cell line resistant to hydroxyurea was also found to contain increased levels of two M2 mRNA species (about 3.4 and 1.6 kb) and exhibited M2 gene amplification. One hamster cell line resembled the other resistant rodent lines in cellular characteristics but did not show amplification of either the M1 or M2 gene, providing an example of a drug-resistant mechanism in which an elevation of M2 mRNA has occurred without a concomitant increase in M2 gene copy number.

摘要

已对五种对羟基脲细胞毒性作用具有抗性的仓鼠、小鼠和大鼠细胞系进行了特性分析。所有细胞系均具有增强的核糖核苷酸还原酶活性,通过电子顺磁共振光谱判断,核糖核苷酸还原酶的M2组分水平升高,通过Northern印迹分析确定,M2 mRNA的拷贝数增加。在啮齿动物细胞系中检测到两种M2 mRNA,在仓鼠和大鼠细胞中为高分子量的约3.4 kb,在小鼠细胞中约为2.1 kb。在所有啮齿动物细胞系中,低分子量的M2 mRNA约为1.6 kb。Northern印迹分析表明,核糖核苷酸还原酶另一组分M1的mRNA在耐药细胞中未明显升高,且以单一的3.1 kb形式存在。通过Southern印迹分析确定,五个耐药细胞系中有四个含有M2基因扩增,为早期关于羟基脲耐药性常伴有核糖核苷酸还原酶基因扩增的观点提供了直接证据。即使在仅表现出适度耐药特性的细胞中也检测到基因剂量增加。未发现核糖核苷酸还原酶M1基因扩增的证据。与这些耐药啮齿动物细胞系的观察结果一致,还发现一种对羟基脲耐药的人(HeLa)细胞系含有两种M2 mRNA(约3.4和1.6 kb)水平升高,并表现出M2基因扩增。一个仓鼠细胞系在细胞特征上与其他耐药啮齿动物细胞系相似,但未显示M1或M2基因扩增,提供了一种耐药机制的例子,其中M2 mRNA升高但M2基因拷贝数未随之增加。

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