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锤头状核酶截短茎环II变体在非周转条件下低镁浓度时切割活性的体外优化

In vitro optimization of truncated stem-loop II variants of the hammerhead ribozyme for cleavage in low concentrations of magnesium under non-turnover conditions.

作者信息

Zillmann M, Limauro S E, Goodchild J

机构信息

HYBRIDON, Inc., Cambridge, Massachusetts 02139, USA.

出版信息

RNA. 1997 Jul;3(7):734-47.

Abstract

By truncating helix II to two base pairs in a hammerhead ribozyme having long flanking sequences (greater than 30 bases), the rate of cleavage in 1 mM magnesium can be increased roughly 100-fold. Replacing most of the nucleotides in a typical stem-loop II with 1-4 randomized nucleotides gave an RNA library that, even before selection, was more active in 1 mM magnesium than the parent ribozyme, but considerably less active than the truncated stem-loop II ribozyme. A novel, multiround selection for intermolecular cleavage was exploited to optimize this library for cleavage in low concentrations of magnesium. After three rounds of selection at sequentially lower concentrations of magnesium, the library cleaved substrate RNA 20-fold faster than the initial pool and was cloned. This pool was heavily enriched for one particular sequence (5'-CGUG-3') that represented 16 of 52 isolates (the next most common sequence was represented only six times). This sequence also represented the most active sequence, exceeding the activity of the short helix II variant under the conditions of the selection, thereby demonstrating the effectiveness of the selection technique. Analysis of the cleavage rates of RNAs made from eight isolates having different four-base insert sequences allowed assignment of highly preferred bases at each position in the insert. Analysis of pool clones having insert of differing lengths showed that, in general, activity decreased as the length of the insert decreased from 4 to 1. This supports the suggested role of stem-loop II in stabilizing the non-Watson-Crick interactions between the conserved bases of the catalytic core.

摘要

在具有长侧翼序列(大于30个碱基)的锤头状核酶中,将螺旋II截短至两个碱基对,在1 mM镁离子存在的情况下,切割速率可提高约100倍。用1 - 4个随机核苷酸取代典型茎环II中的大部分核苷酸,得到一个RNA文库,该文库即使在未进行筛选之前,在1 mM镁离子存在时的活性就比亲本核酶高,但比截短的茎环II核酶的活性低得多。利用一种新的、用于分子间切割的多轮筛选方法,在低浓度镁离子条件下优化该文库的切割活性。在依次降低的镁离子浓度下进行三轮筛选后,该文库切割底物RNA的速度比初始文库快20倍,并进行了克隆。该文库高度富集了一个特定序列(5'-CGUG-3'),在52个分离株中有16个含有该序列(第二常见的序列仅出现6次)。该序列也是最具活性的序列,在筛选条件下其活性超过了短螺旋II变体,从而证明了筛选技术的有效性。对由8个具有不同四碱基插入序列的分离株制备的RNA的切割速率进行分析,确定了插入序列中每个位置的高度偏好碱基。对具有不同长度插入序列的文库克隆进行分析表明,一般来说,随着插入序列长度从4个碱基减少到1个碱基,活性降低。这支持了茎环II在稳定催化核心保守碱基之间非沃森-克里克相互作用中所起的作用。

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