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形成RNA凸起:通过金属离子催化切割RNA/DNA双链体中的RNA。

Creating RNA bulges: cleavage of RNA in RNA/DNA duplexes by metal ion catalysis.

作者信息

Hüsken D, Goodall G, Blommers M J, Jahnke W, Hall J, Häner R, Moser H E

机构信息

Central Research Laboratories, Ciba-Geigy Ltd., Basel, Switzerland.

出版信息

Biochemistry. 1996 Dec 24;35(51):16591-600. doi: 10.1021/bi961700c.

Abstract

The manipulation of a single-stranded RNA target by forming different RNA/antisense hybrids demonstrates the possibility of cleaving the RNA strand within duplexes. This was achieved using the sequence composition of the antisense oligonucleotide, an approach that results in various bulges [unpaired base(s)] in the RNA target, which is then cleavable at these specific bulge sites under free metal ion or metal complex catalysis. RNA cleavages promoted by metal ions were performed under mild conditions and characterized by separating the RNA fragments carrying end label. The observed products result from intramolecular transesterification causing RNA strand scission. No detectable cleavage of the RNA was observed with either a fully complementary RNA/antisense hybrid or a bulged base in the antisense strand. A molecular modeling study of the RNA backbone suggests that the local conformation of the RNA backbone at a bulge in such hybrid duplexes greatly facilitates the metal-assisted catalytic cleavage. Endonucleolytic RNA cleavage within an RNA/antisense hybrid by metal complexes attached to the antisense oligonucleotide might lead to a new approach in antisense technology with artificial ribonucleases which operate with catalytic turnover.

摘要

通过形成不同的RNA/反义杂交体来操纵单链RNA靶标,证明了在双链体中切割RNA链的可能性。这是利用反义寡核苷酸的序列组成实现的,该方法会在RNA靶标中产生各种凸起(未配对碱基),然后在游离金属离子或金属配合物催化下,这些特定凸起位点处的RNA可被切割。由金属离子促进的RNA切割在温和条件下进行,并通过分离带有末端标记的RNA片段来表征。观察到的产物是由分子内酯交换导致RNA链断裂产生的。无论是完全互补的RNA/反义杂交体还是反义链中的凸起碱基,都未观察到可检测到的RNA切割。对RNA主链的分子建模研究表明,此类杂交双链体中凸起处的RNA主链局部构象极大地促进了金属辅助催化切割。通过连接到反义寡核苷酸上的金属配合物在RNA/反义杂交体内进行核酸内切RNA切割,可能会导致反义技术中使用具有催化周转功能的人工核糖核酸酶的新方法。

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