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不同种类的乙基化剂在体外和体内对HeLa细胞DNA各个位点的特异性。

The specificity of different classes of ethylating agents toward various sites of HeLa cell DNA in vitro and in vivo.

作者信息

Sun L, Singer B

出版信息

Biochemistry. 1975 Apr 22;14(8):1795-802. doi: 10.1021/bi00679a036.

Abstract

The sites and extent of ethyl products of neutral ethylation of HeLa cell DNA by [14-C]diethyl sulfate, [14-C]ethyl methanesulfonate, and [14-C]ethylnitrosourea have been determined in vitro and in vivo, and found to differ significantly depending on the ethylating agents. Diethyl sulfate and ethyl methanesulfonate ethylate the bases of HeLa cell DNA in the following order: 7-ethylguanine greater than 3-ethyladenine greater than 1-ethyladenine, 7-ethyladenine greater than 3-ethylguanine, 3-ethylcytosine, O-6-ethylguanine. Ethyl bases accounted for 84-87% of the total ethyl groups associated with HeLa cell DNA. Ethylnitrosourea, in contrast, has particular affinity for the O-6 position of guanine. It ethylates the bases of HeLa cell DNA in the following order: O-6-ethylguanine, 7-ethylguanine greater than 3-ethyladenine greater than 3-ethylguanine, 3-ethylthymine greater than 1-ethyladenine, 7-ethyladenine, 3-ethylcytosine. Ethylation of the bases only accounts for 30% of the total ethylation in the case of ethylnitrosourea. The remaining 70% of the [14-C]ethyl groups, introduced in vivo and in vitro, are in the form of phosphotriesters which after perchloric acid hydrolysis are found as [14-CA1ethanol and [14-C]ethyl phosphate. In contrast, phosphotriesters amounted to only 8-20% of total ethylation in in vivo or in vitro diethyl sulfate and ethyl methanesulfonate treated HeLa cell DNA, and 25% of the total methylation in in vitro methylnitrosourea treated HeLa cell DNA. Alkylation at the N-7 and N-3 positions of purines in DNA destabilizes the glycosidic linkages. Part of 7-ethylguanine and 3-ethyladenine are found to be spontaneously released during the ethylation reaction. Incorporation of the 14-C of the alkylating agents into normal DNA bases of HeLa cells can be eliminated by performing the alkylations, in the presence of cytosine arabinoside, for 1 hr.

摘要

通过[¹⁴C]硫酸二乙酯、[¹⁴C]甲磺酸乙酯和[¹⁴C]乙基亚硝基脲对HeLa细胞DNA进行中性乙基化反应的位点和程度已在体外和体内确定,并发现其因乙基化剂的不同而有显著差异。硫酸二乙酯和甲磺酸乙酯对HeLa细胞DNA碱基的乙基化顺序如下:7-乙基鸟嘌呤>3-乙基腺嘌呤>1-乙基腺嘌呤,7-乙基腺嘌呤>3-乙基鸟嘌呤,3-乙基胞嘧啶,O-6-乙基鸟嘌呤。乙基化碱基占与HeLa细胞DNA相关的总乙基基团的84 - 87%。相比之下,乙基亚硝基脲对鸟嘌呤的O-6位具有特殊亲和力。它对HeLa细胞DNA碱基的乙基化顺序如下:O-6-乙基鸟嘌呤,7-乙基鸟嘌呤>3-乙基腺嘌呤>3-乙基鸟嘌呤,3-乙基胸腺嘧啶>1-乙基腺嘌呤,7-乙基腺嘌呤,3-乙基胞嘧啶。在乙基亚硝基脲的情况下,碱基的乙基化仅占总乙基化的30%。在体内和体外引入的其余70%的[¹⁴C]乙基基团以磷酸三酯的形式存在,在高氯酸水解后以[¹⁴C]乙醇和[¹⁴C]磷酸乙酯的形式被发现。相比之下,在体内或体外经硫酸二乙酯和甲磺酸乙酯处理的HeLa细胞DNA中,磷酸三酯仅占总乙基化的8 - 20%,在体外经甲基亚硝基脲处理的HeLa细胞DNA中,磷酸三酯占总甲基化的25%。DNA中嘌呤的N-7和N-3位的烷基化会破坏糖苷键。部分7-乙基鸟嘌呤和3-乙基腺嘌呤在乙基化反应过程中会自发释放。在阿糖胞苷存在的情况下进行烷基化反应1小时,可以消除烷基化剂的¹⁴C掺入HeLa细胞的正常DNA碱基中。

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