首页> 外文期刊>Applied biochemistry and biotechnology, Part A. enzyme engineering and biotechnology >The 'bringer' strategy: a very fast and highly efficient method for construction of mutant libraries by error-prone polymerase chain reaction of ring-closed plasmids.
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The 'bringer' strategy: a very fast and highly efficient method for construction of mutant libraries by error-prone polymerase chain reaction of ring-closed plasmids.

机译:“ bringer”策略:通过闭环质粒的易错聚合酶链反应,构建突变体文库的非常快速和高效的方法。

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摘要

Random mutagenesis constitutes a keystone in many strategies of directed evolution of biocatalysts and is often done by error-prone polymerase chain reaction (epPCR). Traditionally, the epPCR-generated DNA fragments are then subcloned into an expression vector to obtain a mutant library, which in turn is transformed into a suited host and screened for mutants that display the desired property. However, the vast majority of epPCR-generated fragments generally are lost during the subcloning step, making it the bottleneck in the mutant library construction procedure. Here we report a rapid and convenient strategy based on the epPCR amplification of a ring-closed expression plasmid that contains the gene of interest; after a DpnI digest the product of the epPCR reaction constitutes the mutant library and can be used directly for screening procedures. Primers binding to the beta-lactamase gene were chosen to allow application of the strategy to as broad a range of target plasmids as possible. The functionality of this approach was demonstrated by mutating the alpha-peptide coding region of the lacZ gene.
机译:随机诱变是生物催化剂定向进化的许多策略的基石,通常是通过容易出错的聚合酶链反应(epPCR)完成的。传统上,然后将epPCR生成的DNA片段亚克隆到表达载体中,以获得突变体文库,然后将其转化为合适的宿主,并筛选出具有所需特性的突变体。但是,大多数epPCR产生的片段通常在亚克隆步骤中丢失,这使其成为突变体文库构建过程的瓶颈。在这里,我们报告了一种快速且方便的策略,该策略基于包含目的基因的闭环表达质粒的epPCR扩增;经过DpnI消化后,epPCR反应的产物构成了突变文库,可直接用于筛选程序。选择与β-内酰胺酶基因结合的引物以允许将该策略应用于尽可能广泛的靶质粒。该方法的功能通过突变lacZ基因的α-肽编码区来证明。

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