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使用混合底物法研究tRNA甲基化酶的特异性。

Use of the method of mixed substrates to study the specificity of tRNA methylases.

作者信息

Gambaryan A S, Venkstern T V, Baev A A

出版信息

Mol Biol (Mosk). 1976 Jul-Aug;10(4):697-705.

PMID:799257
Abstract

The absence of summation of the rate of methylation of positionally analogous cytidine residues in tRNA1Val, tRNAPhe, and tRNAMet in the case of simultaneous presence of two substrates in the incubation mixture was demonstrated by the method of mixed substrates. The same result was also obtained in the methylation of A19 (counting from the 3' end of the molecule) in tRNA1Val, tRNAPhe, tRNAfMet, tRNASer, and tRNAGlu individually and in the case of their mixing in pairs. These data are evidence that positionally analogous nucleotides in different RNAs are attacked by the same enzyme. Yeast tRNASer, already possessing a methyl group at the cytidine residue studied, proved to be an effective inhibitor of methylase, forming m5C with valine and phenylalanine tRNAs. The results obtained are evidence that differences in the primary and secondary structures at the site of methylation are not the deciding factors in the interaction of tRNA with methylases.

摘要

通过混合底物法证明,在孵育混合物中同时存在两种底物的情况下,tRNA1Val、tRNAPhe和tRNAMet中位置类似的胞苷残基的甲基化速率不存在加和现象。在单独对tRNA1Val、tRNAPhe、tRNAfMet、tRNASer和tRNAGlu中A19(从分子3'端计数)进行甲基化以及将它们成对混合的情况下,也得到了相同的结果。这些数据证明,不同RNA中位置类似的核苷酸受到相同酶的作用。酵母tRNASer在所研究的胞苷残基处已含有一个甲基,事实证明它是甲基化酶的有效抑制剂,能与缬氨酸和苯丙氨酸tRNA形成m5C。所得结果证明,甲基化位点处一级和二级结构的差异不是tRNA与甲基化酶相互作用的决定性因素。

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