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Golden Mutagenesis: An efficient multi-site-saturation mutagenesis approach by Golden Gate cloning with automated primer design

机译:黄金诱变:通过金门克隆和自动引物设计进行的高效多位点饱和诱变方法

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摘要

Site-directed methods for the generation of genetic diversity are essential tools in the field of directed enzyme evolution. The Golden Gate cloning technique has been proven to be an efficient tool for a variety of cloning setups. The utilization of restriction enzymes which cut outside of their recognition domain allows the assembly of multiple gene fragments obtained by PCR amplification without altering the open reading frame of the reconstituted gene. We have developed a protocol, termed Golden Mutagenesis that allows the rapid, straightforward, reliable and inexpensive construction of mutagenesis libraries. One to five amino acid positions within a coding sequence could be altered simultaneously using a protocol which can be performed within one day. To facilitate the implementation of this technique, a software library and web application for automated primer design and for the graphical evaluation of the randomization success based on the sequencing results was developed. This allows facile primer design and application of Golden Mutagenesis also for laboratories, which are not specialized in molecular biology.
机译:定点的遗传多样性产生方法是定向酶进化领域必不可少的工具。金门克隆技术已被证明是用于各种克隆设置的有效工具。利用在其识别结构域之外切割的限制酶,可以组装通过PCR扩增获得的多个基因片段,而无需改变重构基因的开放阅读框。我们已经开发了一种称为Golden Mutagenesis的协议,该协议可以快速,直接,可靠和廉价地构建诱变库。使用可以在一天之内执行的方案,可以同时更改编码序列中1至5个氨基酸的位置。为了促进该技术的实施,开发了用于自动引物设计和基于测序结果对随机化成功进行图形评估的软件库和Web应用程序。这使得还可以在不专门从事分子生物学的实验室中简便地设计引物,以及将Golden Mutagenesis用于实验室。

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