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一种改进的利用化学修饰的RNA测序快速酶促方法。

An improved rapid enzymatic method of RNA sequencing using chemical modification.

作者信息

Mazo A M, Mashkova T D, Avdonina T A, Ambartsumyan N S, Kisselev L L

出版信息

Nucleic Acids Res. 1979 Dec 20;7(8):2469-82. doi: 10.1093/nar/7.8.2469.

Abstract

A version of rapid gel sequencing procedure based on the analysis of partial endonuclease hydrolizates of chemically modified 5'-32P-labelled RNA is suggested. Complete and selective modification of cytidilic residues by a methoxyamine-bisulfite mixture leads to the unfolding of the RNA secondary structure and, due to this effect, to the generation of a more uniform set of fragments after partial RNAase hydrolysis. The position of cytidines in an RNA sequence can be determined by restricting the hydrolysis of phosphodiester bonds between the modified CMP residues and their 3'-neighbours with T2 and A RNAases. The method was verified with tRNATrp (yeast) and 5S RNA (rat liver and yeast).

摘要

提出了一种基于对化学修饰的5'-32P标记RNA的部分核酸内切酶水解产物进行分析的快速凝胶测序程序版本。用甲氧基胺-亚硫酸氢盐混合物对胞嘧啶残基进行完全和选择性修饰会导致RNA二级结构展开,并且由于这种效应,在部分核糖核酸酶水解后会产生更均匀的片段集。RNA序列中胞嘧啶的位置可以通过用T2和A核糖核酸酶限制修饰的CMP残基与其3'-邻位之间的磷酸二酯键的水解来确定。该方法已用酵母的tRNATrp和大鼠肝脏及酵母的5S RNA进行了验证。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1e85/342397/6ed425f7b5c3/nar00461-0394-a.jpg

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