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致癌性非氨基偶氮染料1-苯基偶氮-2-羟基萘与转移核糖核酸的过氧化物酶介导反应。

Peroxidase-mediated reaction of the carcinogenic non-aminoazo dye 1-phenylazo-2-hydroxynaphthalene with transfer ribonucleic acid.

作者信息

Stiborová M, Frei E, Klokow K, Wiessler M, Safarík L, Anzenbacher P, Hradec J

机构信息

Department of Biochemistry, Faculty of Natural Sciences, Charles University, Prague, Czechoslovakia.

出版信息

Carcinogenesis. 1990 Oct;11(10):1789-94. doi: 10.1093/carcin/11.10.1789.

Abstract

Horseradish peroxidase in the presence of hydrogen peroxide has the ability to mediate the activation of carcinogenic 1-phenylazo-2-hydroxynaphthalene (Sudan I) to DNA- and transfer RNA (tRNA)-bound products in vitro. tRNA is more accessible for modification by the activated carcinogen studied. tRNA modified by activated Sudan I becomes colored and has an absorption maximum of approximately 480 nm. Binding of metabolite(s) to tRNA is inhibited by ascorbate, glutathione, Mg2+ ions and nitrosobenzene. The mechanism of these protections was shown to be different for the different agents. tRNA modified by activated Sudan I exhibits a significantly increased acceptance for L-methionine. Enzymatic hydrolysis of modified tRNA with subsequent separation of nucleosides by HPLC suggests that the covalent modification of tRNA originating from the formation of more than one adduct with the nucleosides in tRNA is the predominant interaction of the activated Sudan I with tRNA.

摘要

在过氧化氢存在的情况下,辣根过氧化物酶能够在体外介导致癌物质1-苯基偶氮-2-羟基萘(苏丹红I)活化为与DNA和转运RNA(tRNA)结合的产物。所研究的活化致癌物更容易对tRNA进行修饰。经活化的苏丹红I修饰的tRNA会变色,其最大吸收波长约为480nm。抗坏血酸、谷胱甘肽、Mg2+离子和亚硝基苯会抑制代谢物与tRNA的结合。结果表明,这些保护作用的机制因不同试剂而异。经活化的苏丹红I修饰的tRNA对L-甲硫氨酸的接受能力显著增强。用HPLC对修饰的tRNA进行酶促水解并随后分离核苷,结果表明,tRNA的共价修饰源于与tRNA中的核苷形成多个加合物,这是活化的苏丹红I与tRNA的主要相互作用。

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