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肽基寡核苷酸缀合物能以序列特异性方式高效切割RNA。

Peptidyl-oligonucleotide conjugates demonstrate efficient cleavage of RNA in a sequence-specific manner.

作者信息

Williams Aled, Staroseletz Yaroslav, Zenkova Marina A, Jeannin Laurent, Aojula Harmesh, Bichenkova Elena V

机构信息

†Manchester Pharmacy School, University of Manchester, Oxford Road, Manchester, United Kingdom, M13 9PT.

‡Institute of Chemical Biology and Fundamental Medicine SB RAS, 8 Laurentiev Avenue, 630090, Novosibirsk, Russia.

出版信息

Bioconjug Chem. 2015 Jun 17;26(6):1129-43. doi: 10.1021/acs.bioconjchem.5b00193. Epub 2015 May 21.

DOI:10.1021/acs.bioconjchem.5b00193
PMID:25955796
Abstract

Described here is a new class of peptidyl-oligonucleotide conjugates (POCs) which show efficient cleavage of a target RNA in a sequence-specific manner. Through phosphoramidate attachment of a 17-mer TΨC-targeting oligonucleotide to amphiphilic peptide sequences containing leucine, arginine, and glycine, zero-linker conjugates are created which exhibit targeted phosphodiester cleavage under physiological conditions. tRNA(Phe) from brewer's yeast was used as a model target sequence in order to probe different structural variants of POCs in terms of selective TΨC-arm directed cleavage. Almost quantitative (97-100%) sequence-specific tRNA cleavage is observed for several POCs over a 24 h period with a reaction half-life of less than 1 h. Nontargeted cleavage of tRNA(Phe) or HIV-1 RNA is absent. Structure-activity relationships reveal that removal of the peptide's central glycine residue significantly decreases tRNA cleavage activity; however, this can be entirely restored through replacement of the peptide's C-terminal carboxylic acid group with the carboxamide functionality. Truncation of the catalytic peptide also has a detrimental effect on POC activity. Based on the encouraging results presented, POCs could be further developed with the aim of creating useful tools for molecular biology or novel therapeutics targeting specific messenger, miRNA, and genomic viral RNA sequences.

摘要

本文描述了一类新型的肽基寡核苷酸缀合物(POC),它们能以序列特异性方式高效切割靶RNA。通过将一个17聚体靶向TΨC的寡核苷酸以氨基磷酸酯的方式连接到含有亮氨酸、精氨酸和甘氨酸的两亲性肽序列上,制备出了零连接体缀合物,这些缀合物在生理条件下能实现靶向磷酸二酯键切割。以酿酒酵母的tRNA(Phe)作为模型靶序列,以探究POC在选择性TΨC臂定向切割方面的不同结构变体。在24小时内,几种POC能实现几乎定量(97 - 100%)的序列特异性tRNA切割,反应半衰期小于1小时。未观察到对tRNA(Phe)或HIV - 1 RNA的非靶向切割。构效关系表明,去除肽的中心甘氨酸残基会显著降低tRNA切割活性;然而,通过用羧酰胺官能团取代肽的C末端羧酸基团,这一活性可完全恢复。催化肽的截短也对POC活性有不利影响。基于所呈现的令人鼓舞的结果,POC有望进一步开发,旨在为分子生物学创造有用工具,或开发针对特定信使RNA、微小RNA和基因组病毒RNA序列的新型疗法。

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