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一种用于体外筛选和选择系统的组装线性DNA模板的有效方法。

An efficient method to assemble linear DNA templates for in vitro screening and selection systems.

作者信息

Stein Viktor, Hollfelder Florian

机构信息

Department of Biochemistry, University of Cambridge, CB2 1GA, Cambridge, UK.

出版信息

Nucleic Acids Res. 2009 Oct;37(18):e122. doi: 10.1093/nar/gkp589. Epub 2009 Jul 17.

Abstract

A method is presented to assemble a gene of interest into a linear DNA template with all the components necessary for in vitro transcription and translation in approximately 90 min. Assembly is achieved using a coupled uracil excision-ligation strategy based on USER Enzyme and T4 DNA ligase, which allows the simultaneous and seamless assembly of three different PCR products. The method is suitable for screening and selection systems of very high throughput as up to 10(11) molecules can be efficiently assembled and purified in reaction volumes of 100 microl. The method is exemplified with the gene coding for a mutant version of O(6)-alkylguanine alkyltransferase, which is efficiently assembled with an N-terminal peptide tag and its 5'- and 3'-untranslated regions that include a T7 promoter, ribosome binding site and T7 terminator. The utility of the method is further corroborated by assembling error-prone PCR libraries and regenerating templates following model affinity selections. This fast and robust method should find widespread application in directed evolution for the assembly of gene libraries and the regeneration of linear DNA templates between successive screening and selection cycles.

摘要

本文介绍了一种方法,可在约90分钟内将目的基因组装到线性DNA模板中,该模板包含体外转录和翻译所需的所有组件。使用基于USER酶和T4 DNA连接酶的尿嘧啶切除-连接偶联策略实现组装,该策略允许同时无缝组装三种不同的PCR产物。该方法适用于非常高通量的筛选和选择系统,因为在100微升的反应体积中可高效组装和纯化多达10¹¹个分子。以编码O(6)-烷基鸟嘌呤烷基转移酶突变体版本的基因为例,该基因与N端肽标签及其5'和3'非翻译区(包括T7启动子、核糖体结合位点和T7终止子)高效组装。通过组装易错PCR文库并在模型亲和选择后再生模板,进一步证实了该方法的实用性。这种快速且稳健的方法应在定向进化中广泛应用于基因文库的组装以及连续筛选和选择循环之间线性DNA模板的再生。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/af2a/2764453/209990c990dd/gkp589f1.jpg

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