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用户友好型 DNA 重组(USERec):一种简单灵活的近同源非依赖基因文库构建方法。

USER friendly DNA recombination (USERec): a simple and flexible near homology-independent method for gene library construction.

机构信息

Department of Biochemistry, University of Cambridge, 80 Tennis Court Road, Cambridge CB2 1GA, UK.

出版信息

Protein Eng Des Sel. 2010 Jan;23(1):1-8. doi: 10.1093/protein/gzp063.

Abstract

USER friendly DNA recombination (USERec) is introduced as a near homology-independent method that allows the simultaneous recombination of an unprecedented number of 10 DNA fragments (approximately 40-400 bp) within a day. The large number of fragments and their ease of preparation enables the creation of libraries of much larger genetic diversity (potentially approximately 10(10)-10(11) sequences) than current alternative methods based on DNA truncation (ITCHY, SCRATCHY and SHIPREC) or type IIb restriction enzymes (SISDC). At the same time, the frequency of frameshifts in the recombined library is low (90% of the recombined sequences are in frame). Compared to overlap extension PCR, USERec also requires much reduced crossover sequence constraints (only a 5'-AN(4-8)T-3' motif) and fewer experimental steps. Based on its simplicity and flexibility, and the accessibility of large and high quality recombined DNA libraries, USERec is established as a convenient alternative for the combinatorial assembly of gene fragments (e.g. exon or domain shuffling) and for a number of applications in gene library construction, such as loop grafting and multi-site-directed or random mutagenesis.

摘要

用户友好型 DNA 重组(USERec)是一种近乎无需同源性的方法,可在一天内同时重组数量空前的 10 个 DNA 片段(约 40-400bp)。大量的片段及其易于制备的特点,使得创建的遗传多样性文库更大(潜在地大约为 10(10)-10(11)个序列),而不是当前基于 DNA 截断的替代方法(ITCHY、SCRATCHY 和 SHIPREC)或 IIb 型限制酶(SISDC)。同时,重组文库中的移码频率较低(90%的重组序列是框架内的)。与重叠延伸 PCR 相比,USERec 还需要大大减少交叉序列限制(仅需要 5'-AN(4-8)T-3' 基序)和更少的实验步骤。基于其简单性和灵活性,以及易于获得大量高质量的重组 DNA 文库,USERec 成为了组合组装基因片段(例如外显子或结构域改组)的便捷替代方法,并且在基因文库构建的许多应用中,例如环嫁接和多位点定向或随机诱变中也很有用。

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