A modified method for PCR-directed gene synthesis from large number of overlapping oligodeoxyribonucleotides

Journal of biochemical and biophysical methods Pub Date : 2008-04-24 DOI:10.1016/j.jprot.2007.12.009

Jessica Cherry, Bart W. Nieuwenhuijsen, Edward J. Kaftan, Jeffrey D. Kennedy, Pranab K. Chanda

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引用次数: 11

Abstract

Here we report an improved, reproducible, simple, rapid, and cost-effective PCR-based DNA synthesis method using short (25–40 bp) overlapping oligodeoxyribonucleotides (oligos). The method involves two steps; (1) assembly of multiple/overlapping oligos by PCR to generate the template DNA and (2) amplification of the template DNA sequence with the two outermost oligos as primers. We have tested this method by synthesizing approximately 35 genes ranging in size between 300 bp and 1700 bp and G + C content from moderate (30%) to high (65%). In addition, we used the method to introduce 29 mutations simultaneously into a single gene. Key to the success of this method is the use of optimized oligo concentrations and the type of DNA polymerase used. This simplified and highly reproducible method is expected to be beneficial for the synthesis of a wide variety of genes.

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从大量重叠的寡脱氧核糖核苷酸合成pcr定向基因的改进方法

在这里，我们报告了一种改进的，可重复的，简单的，快速的，成本效益高的基于pcr的DNA合成方法，使用短(25-40 bp)重叠的寡脱氧核糖核苷酸(oligos)。该方法包括两个步骤;(1)用PCR方法组装多个/重叠的寡核苷酸生成模板DNA;(2)用最外层的两个寡核苷酸作为引物扩增模板DNA序列。我们已经合成了大约35个基因，大小在300 bp到1700 bp之间，G + C含量从中等(30%)到高(65%)不等。此外，我们使用该方法将29个突变同时引入到单个基因中。该方法成功的关键是使用优化的寡聚物浓度和使用的DNA聚合酶的类型。这种简化和高重复性的方法有望有利于多种基因的合成。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Journal of biochemical and biophysical methods

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