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通过将寡脱氧核糖核苷酸连接到模板链含有脱氧尿苷的缺口异源双链DNA中进行简单且高效的位点特异性诱变。

Simple and highly efficient site-specific mutagenesis, by ligation of an oligodeoxyribonucleotide into gapped heteroduplex DNA in which the template strand contains deoxyuridine.

作者信息

Terwilliger T C

机构信息

Department of Biochemistry and Molecular Biology, University of Chicago, IL 60637.

出版信息

Gene. 1988 Sep 30;69(2):317-24. doi: 10.1016/0378-1119(88)90441-6.

Abstract

A simple and highly efficient procedure for oligodeoxynucleotide (oligo)-directed mutagenesis has been developed. In this procedure, a gapped heteroduplex DNA is first constructed and purified. The gapped heteroduplex consists of a circular 'template' strand of DNA, which contains some misincorporated deoxyuridine nucleotides, and a complementary strand which does not contain deoxyuridine, and which lacks a defined segment. Making a specific change in the sequence of the DNA within the gapped region then only requires ligation and transformation. An oligo, exactly the same length as the gap, and with the desired sequence, is synthesized, purified, and ligated directly into the gap in the heteroduplex. When this DNA is used to transform wt (ung+) Escherichia coli, about 80% of the resulting plasmids contain the sequence determined by the synthetic oligo. One gapped heteroduplex preparation can be used for many mutagenesis experiments, so that this procedure is well-suited for producing a series of defined mutations within a defined target region flanked by sites for restriction enzyme cleavage. As the method does not require a polymerase, the effects of primer displacement and polymerase infidelity are avoided.

摘要

已开发出一种用于寡脱氧核苷酸(oligo)定向诱变的简单且高效的方法。在此方法中,首先构建并纯化带缺口的异源双链DNA。该带缺口的异源双链由一条环状“模板”DNA链组成,其含有一些错配掺入的脱氧尿苷核苷酸,以及一条互补链,该互补链不含脱氧尿苷且缺少一个确定的片段。然后,仅需连接和转化即可在缺口区域内的DNA序列中进行特定改变。合成一条与缺口长度完全相同且具有所需序列的寡核苷酸,将其纯化后直接连接到异源双链的缺口中。当使用这种DNA转化野生型(ung+)大肠杆菌时,约80%的所得质粒包含由合成寡核苷酸确定的序列。一份带缺口的异源双链制剂可用于多次诱变实验,因此该方法非常适合在由限制性内切酶切割位点侧翼的特定靶区域内产生一系列确定的突变。由于该方法不需要聚合酶,避免了引物置换和聚合酶错配的影响。

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