利用 Golden Gate 克隆技术生成定点饱和突变文库并将其转移到广谱宿主范围质粒上。

Generating Site Saturation Mutagenesis Libraries and Transferring Them to Broad Host-Range Plasmids Using Golden Gate Cloning.

机构信息

Max Planck Institute for Terrestrial Microbiology, Marburg, Germany.

Center for Synthetic Microbiology (SYNMIKRO), Philipps-University Marburg, Marburg, Germany.

出版信息

Methods Mol Biol. 2025;2850:251-264. doi: 10.1007/978-1-0716-4220-7_14.

DOI:10.1007/978-1-0716-4220-7_14

PMID:39363076

Abstract

Protein engineering is an established method for tailoring enzymatic reactivity. A commonly used method is directed evolution, where the mutagenesis and natural selection process is mimicked and accelerated in the laboratory. Here, we describe a reliable method for generating saturation mutagenesis libraries by Golden Gate cloning in a broad host range plasmid containing the pBBR1 replicon. The applicability is demonstrated by generating a mutant library of the iron nitrogenase gene cluster (anfHDGK) of Rhodobacter capsulatus, which is subsequently screened for the improved formation of molecular hydrogen.

摘要

蛋白质工程是一种用于调整酶反应性的成熟方法。一种常用的方法是定向进化，在该方法中，突变和自然选择过程在实验室中被模拟和加速。在这里，我们描述了一种通过 Golden Gate 克隆在含有 pBBR1 复制子的广泛宿主范围质粒中生成饱和突变文库的可靠方法。该方法的适用性通过生成荚膜红细菌的铁氮酶基因簇（anfHDGK）的突变文库来证明，随后对其进行筛选以提高分子氢的形成。

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利用 Golden Gate 克隆技术生成定点饱和突变文库并将其转移到广谱宿主范围质粒上。

Generating Site Saturation Mutagenesis Libraries and Transferring Them to Broad Host-Range Plasmids Using Golden Gate Cloning.

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