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通过基于PCR的质粒多聚化在枯草芽孢杆菌中生成大型随机突变体文库。

Generation of large libraries of random mutants in Bacillus subtilis by PCR-based plasmid multimerization.

作者信息

Shafikhani S, Siegel R A, Ferrari E, Schellenberger V

机构信息

Genencor International, Palo Alto, CA, USA.

出版信息

Biotechniques. 1997 Aug;23(2):304-10. doi: 10.2144/97232rr01.

Abstract

We describe a PCR-based method for the generation of plasmid multimers that can be directly transformed into Bacillus subtilis with very high efficiency. This technique is particularly useful for the generation of large libraries of randomly mutagenized genes, which are required for the optimization of enzymes by directed evolution. We subjected the gene coding for the protease subtilisin to six consecutive rounds of PCR at three different levels of mutagenicity. The resulting 18 populations were cloned using our PCR multimerization protocol, and the mutation frequencies were determined by DNA sequencing. The resulting data demonstrate that the mutation frequency during PCR can be controlled by adding varying concentrations of manganese chloride to the reaction mixture. We observed a bias in the type of base pair changes with A and T being mutated much more frequently than C and G. We determined the fraction of active clones in all populations and found that its natural logarithm is proportional to the average mutation frequency of the populations. These data reveal that a fraction of about 0.27 of all possible mutations leads to the inactivation of the subtilisin gene, which provides a measure for its structural plasticity.

摘要

我们描述了一种基于聚合酶链式反应(PCR)的方法,用于生成质粒多聚体,该多聚体能够以非常高的效率直接转化到枯草芽孢杆菌中。这项技术对于生成大量随机诱变基因文库尤为有用,而这些文库是通过定向进化优化酶所必需的。我们将编码枯草杆菌蛋白酶的基因在三种不同诱变水平下进行了连续六轮PCR。使用我们的PCR多聚化方案克隆了所得的18个群体,并通过DNA测序确定了突变频率。所得数据表明,通过向反应混合物中添加不同浓度的氯化锰,可以控制PCR过程中的突变频率。我们观察到碱基对变化类型存在偏差,A和T的突变频率比C和G高得多。我们确定了所有群体中活性克隆的比例,发现其自然对数与群体的平均突变频率成正比。这些数据表明,所有可能突变中约0.27的比例会导致枯草杆菌蛋白酶基因失活,这为其结构可塑性提供了一种衡量方法。

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