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通过高通量筛选组成型启动子突变文库优化大肠杆菌头孢菌素 C 酰化酶的表达。

Optimization of Cephalosporin C Acylase Expression in Escherichia coli by High-Throughput Screening a Constitutive Promoter Mutant library.

机构信息

Department of Biological Science and Engineering, University of Science and Technology Beijing, Beijing, 100083, China.

Department of Environmental Engineering, University of Science and Technology Beijing, Beijing, 100083, China.

出版信息

Appl Biochem Biotechnol. 2021 Apr;193(4):1056-1071. doi: 10.1007/s12010-020-03482-9. Epub 2021 Jan 6.

Abstract

Cephalosporin C acylase (CCA) is capable of catalyzing cephalosporin C (CPC) to produce 7-aminocephalosporanic acid (7-ACA), an intermediate of semi-synthetic cephalosporins. Inducible expression is usually used for CCA. To improve the efficiency of CCA expression without gene induction, three recombinant strains regulated by constitutive promoters BBa_J23105, PLtetO1, and tac were constructed, respectively. Among them, BBa_J23105 was the best promoter and its mutant libraries were established using saturation mutagenesis. In order to obtain the mutants with enhanced activity, a high-throughput screening method based on flow cytometric sorting techniques was developed by using green fluorescent protein (GFP) as the reporter gene. A series of mutants were screened at 28 °C, 200 rpm, and 24-h culture condition. The study of mutants showed that the enzyme activity, fluorescence intensity, and promoter transcriptional strength were positively correlated. The enzyme activity of the optimal mutant obtained by screening reached 12772 U/L, 3.47 times that of the original strain.

摘要

头孢菌素 C 酰化酶(CCA)能够催化头孢菌素 C(CPC)生成 7-氨基头孢烷酸(7-ACA),这是半合成头孢菌素的一种中间体。通常使用诱导型表达来生产 CCA。为了在不进行基因诱导的情况下提高 CCA 的表达效率,分别构建了受组成型启动子 BBa_J23105、PLtetO1 和 tac 调控的三个重组菌株。其中,BBa_J23105 是最佳启动子,并使用饱和突变对其进行了突变文库的构建。为了获得活性增强的突变体,开发了一种基于流式细胞术分选技术的高通量筛选方法,该方法使用绿色荧光蛋白(GFP)作为报告基因。在 28°C、200rpm 和 24 小时培养条件下对一系列突变体进行了筛选。对突变体的研究表明,酶活性、荧光强度和启动子转录强度呈正相关。通过筛选获得的最佳突变体的酶活达到 12772 U/L,是原始菌株的 3.47 倍。

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