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Exploring the potential of megaprimer PCR in conjunction with orthogonal array design for mutagenesis library construction

机译:探索兆引物PCR与正交阵列设计相结合的诱变文库构建潜力

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Although megaprimer PCR mutagenesis has been used routinely in protein directed evolution, users sometimes encounter technical hurdles, particularly inefficiency during amplification when large fragments are used or the template is difficult to be amplified. Instead of methodology development, here we simply overcome the limitation by optimizing megaprimer PCR conditions via orthogonal array design of the four PCR components in three levels of each: template, primer, Mg~(2+), and dNTPs. For this, only nine PCRs need to be performed. The strategy (termed as OptiMega) was not only successfully applied for the construction of one multiple-site saturation mutagenesis library of halohydrin dehalogenase HheC, which failed to be constructed previously using the standard QuikChange? protocol, but also expanded the construction of two high-quality random mutagenesis libraries of HheA and HheC. Most importantly, OptiMega offers a quick and simple way of constructing random mutagenesis libraries by eliminating the ligation step. Our results demonstrated that the OptiMega strategy could greatly strengthen the potential of megaprimer PCR mutagenesis for library construction.
机译:尽管兆引物PCR诱变已常规用于蛋白质定向进化,但用户有时会遇到技术障碍,特别是在使用大片段或难以扩增模板的扩增过程中效率低下。代替方法学的发展,在这里,我们通过正交PCR设计四个引物,分别以模板,引物,Mg〜(2+)和dNTPs三个水平对四个引物进行正交阵列设计,克服了局限性。为此,仅需要执行9个PCR。该策略(称为OptiMega)不仅成功地用于构建卤代醇脱卤酶HheC的一个多位点饱和诱变文库,而该文库以前无法使用标准QuikChange构建。协议,但也扩展了HheA和HheC的两个高质量随机诱变文库的构建。最重要的是,OptiMega通过消除连接步骤,提供了一种构建随机诱变文库的快速简便的方法。我们的结果表明,OptiMega策略可以极大地增强巨引物PCR诱变的文库构建潜力。

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