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细胞脱氧尿苷酸增加导致的DNA片段化和细胞毒性。

DNA fragmentation and cytotoxicity from increased cellular deoxyuridylate.

作者信息

Ingraham H A, Dickey L, Goulian M

出版信息

Biochemistry. 1986 Jun 3;25(11):3225-30. doi: 10.1021/bi00359a022.

DOI:10.1021/bi00359a022
PMID:3524674
Abstract

Previous results from this laboratory have shown that thymidylate deprivation results in dramatic elevation of intracellular dUTP and incorporation of dUMP into DNA. The goal of the present studies was to determine whether the latter changes may play a part in the associated cytotoxicity ("thymineless death"), which is ordinarily assumed to be a direct result of reduced intracellular dTTP. The approach used here was to increase intracellular dUTP without allowing dTTP to diminish and observe the effects on cell viability. dUMP pools were expanded by exposure of cells to deoxyuridine [in cell growth medium containing hypoxanthine, methotrexate, and thymidine (HAT medium)], resulting in accumulation of dUTP to levels that approached those of dTTP, which were at, or higher than, the levels in untreated cells. In conjunction with this the cells became nonviable, and newly synthesized DNA was fragmented, both of which occur with thymidylate depletion and, we assume, result from the active process of excision repair at the many uracil-containing sites in DNA. The results indicate that, although the relative importance of low dTTP remains unknown, elevated dUTP can account for the cytotoxicity caused by thymidine starvation. Most of the "dTTP" measured by the DNA polymerase assay in cells treated with methotrexate (MTX) (plus purine supplement) was, in fact, dUTP, which may explain some previous observations of only modest depression of dTTP in cells treated with MTX or similarly acting drugs.

摘要

该实验室先前的研究结果表明,胸苷酸剥夺会导致细胞内dUTP急剧升高以及dUMP掺入DNA。本研究的目的是确定后者的变化是否可能在相关的细胞毒性(“无胸腺死亡”)中起作用,通常认为这种细胞毒性是细胞内dTTP减少的直接结果。这里采用的方法是在不使dTTP减少的情况下增加细胞内dUTP,并观察对细胞活力的影响。通过将细胞暴露于脱氧尿苷(在含有次黄嘌呤、甲氨蝶呤和胸腺嘧啶核苷的细胞生长培养基中)来扩大dUMP池,导致dUTP积累至接近dTTP的水平,该水平与未处理细胞中的水平相当或更高。与此同时,细胞变得无活力,新合成的DNA被片段化,这两种情况都发生在胸苷酸耗竭时,并且我们认为这是由DNA中许多含尿嘧啶位点的主动切除修复过程导致的。结果表明,尽管低dTTP的相对重要性尚不清楚,但升高的dUTP可以解释胸苷饥饿引起的细胞毒性。在用甲氨蝶呤(MTX)(加嘌呤补充剂)处理的细胞中,通过DNA聚合酶测定法测得的大部分“dTTP”实际上是dUTP,这可能解释了先前一些关于用MTX或类似作用药物处理的细胞中dTTP仅适度降低的观察结果。

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