STI PCR: An efficient method for amplification and de novo synthesis of long DNA sequences

生物 多重位移放大 DNA 基因组DNA 聚合酶链反应 DNA测序 计算生物学 克隆(编程) 分子生物学 PCR的应用 滚动圆复制 基因组 遗传学 基因 聚合酶 数字聚合酶链反应 DNA提取 计算机科学 程序设计语言
作者
Zhe Zhao,Xianrong Xie,Weizhi Liu,Jingjing Huang,Jiantao Tan,Haixin Yu,Wubei Zong,Jintao Tang,Yanchang Zhao,Yang Xue,Zhizhan Chu,Letian Chen,Yao‐Guang Liu
出处
期刊:Molecular Plant [Elsevier]
卷期号:15 (4): 620-629 被引量:21
标识
DOI:10.1016/j.molp.2021.12.018
摘要

Despite continuous improvements, it is difficult to efficiently amplify large sequences from complex templates using current PCR methods. Here, we developed a suppression thermo-interlaced (STI) PCR method for the efficient and specific amplification of long DNA sequences from genomes and synthetic DNA pools. This method uses site-specific primers containing a common 5' tag to generate a stem-loop structure, thereby repressing the amplification of smaller non-specific products through PCR suppression (PS). However, large target products are less affected by PS and show enhanced amplification when the competitive amplification of non-specific products is suppressed. Furthermore, this method uses nested thermo-interlaced cycling with varied temperatures to optimize strand extension of long sequences with an uneven GC distribution. The combination of these two factors in STI PCR produces a multiplier effect, markedly increasing specificity and amplification capacity. We also developed a webtool, calGC, for analyzing the GC distribution of target DNA sequences and selecting suitable thermo-cycling programs for STI PCR. Using this method, we stably amplified very long genomic fragments (up to 38 kb) from plants and human and greatly increased the length of de novo DNA synthesis, which has many applications such as cloning, expression, and targeted genomic sequencing. Our method greatly extends PCR capacity and has great potential for use in biological fields.
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