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使用靶向NUH三联体的间隙嵌合体鉴定核酶可及位点。

Identifying ribozyme-accessible sites using NUH triplet-targeting gapmers.

作者信息

Mir A A, Lockett T J, Hendry P

机构信息

CSIRO Division of Molecular Science, PO Box 184, North Ryde, NSW 1670, Australia.

出版信息

Nucleic Acids Res. 2001 May 1;29(9):1906-14. doi: 10.1093/nar/29.9.1906.

Abstract

Accurately identifying accessible sites in RNA is a critical prerequisite for optimising the cleavage efficiency of hammerhead ribozymes and other small nucleozymes. Here we describe a simple RNase H-based procedure to rapidly identify hammerhead ribozyme-accessible sites in gene length RNAS: Twelve semi-randomised RNA-DNA-RNA chimeric oligonucleotide probes, known as 'gapmers', were used to direct RNase H cleavage of transcripts with the specificity expected for hammerhead ribozymes, i.e. after NUH sites (where H is A, C or U). Cleavage sites were identified simply by the mobility of RNase H cleavage products relative to RNA markers in denaturing polyacrylamide gels. Sites were identified in transcripts encoding human interleukin-2 and platelet-derived growth factor. Thirteen minimised hammerhead ribozymes, miniribozymes (Mrz), were synthesised and in vitro cleavage efficiency (37 degrees C, pH 7.6 and 1 mM MgCl2) at each site was analysed. Of the 13 Mrz, five were highly effective, demonstrating good initial rate constants and extents of cleavage. The speed and accuracy of this method commends its use in screening for hammerhead-accessible sites.

摘要

准确识别RNA中的可及位点是优化锤头状核酶和其他小核酶切割效率的关键前提条件。在此,我们描述了一种基于核糖核酸酶H的简单方法,用于快速识别基因长度RNA中锤头状核酶的可及位点:使用12种半随机RNA-DNA-RNA嵌合寡核苷酸探针(即“缺口嵌合体”),按照锤头状核酶预期的特异性,即NUH位点(其中H为A、C或U)之后,引导核糖核酸酶H切割转录本。通过变性聚丙烯酰胺凝胶中核糖核酸酶H切割产物相对于RNA标记物的迁移率,简单地确定切割位点。在编码人白细胞介素-2和血小板衍生生长因子的转录本中确定了这些位点。合成了13种最小化的锤头状核酶,即微型核酶(Mrz),并分析了每个位点的体外切割效率(37℃、pH 7.6和1 mM MgCl2)。在这13种Mrz中,有5种非常有效,显示出良好的初始速率常数和切割程度。该方法的速度和准确性使其适用于筛选锤头状可及位点。

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