Department of Strategic and Integrative Research, Tianjin Institute of Industrial Biotechnology, Chinese Academy of Sciences, Tianjin, 300308, China.
National Center of Technology Innovation for Synthetic Biology, Tianjin, 300308, China.
Commun Biol. 2024 May 24;7(1):628. doi: 10.1038/s42003-024-06340-0.
Generating genetic diversity lies at the heart of directed evolution which has been widely used to engineer genetic parts and gene circuits in synthetic biology. With the ever-expanding application of directed evolution, different approaches of generating genetic diversity are required to enrich the traditional toolbox. Here we show in vitro generation of genetic diversity for directed evolution by error-prone artificial DNA synthesis (epADS). This approach comprises a three-step process which incorporates base errors randomly generated during chemical synthesis of oligonucleotides under specific conditions into the target DNA. Through this method, 200 ~ 4000 folds of diversification in fluorescent strength have been achieved in genes encoding fluorescent proteins. EpADS has also been successfully used to diversify regulatory genetic parts, synthetic gene circuits and even increase microbial tolerance to carbenicillin in a short time period. EpADS would be an alternative tool for directed evolution which may have useful applications in synthetic biology.
产生遗传多样性是定向进化的核心,定向进化已被广泛用于合成生物学中工程遗传元件和基因回路。随着定向进化的应用不断扩展,需要不同的产生遗传多样性的方法来丰富传统工具集。在这里,我们通过易错人工 DNA 合成(epADS)展示了用于定向进化的体外遗传多样性的产生。该方法包括三个步骤,即在特定条件下化学合成寡核苷酸的过程中随机产生碱基错误,然后将这些错误整合到目标 DNA 中。通过这种方法,成功地在编码荧光蛋白的基因中实现了荧光强度 200~4000 倍的多样化。epADS 还成功地用于多样化调控遗传元件、合成基因回路,甚至在短时间内提高微生物对卡那霉素的耐受性。epADS 将成为定向进化的另一种工具,在合成生物学中可能具有有用的应用。
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