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用于细菌素收获的乳链菌肽生物合成途径的克隆与优化。

Cloning and optimization of a nisin biosynthesis pathway for bacteriocin harvest.

作者信息

Kong Wentao, Lu Ting

机构信息

Department of Bioengineering and Institute for Genomic Biology, University of Illinois at Urbana-Champaign , Urbana, Illinois 61801, United States.

出版信息

ACS Synth Biol. 2014 Jul 18;3(7):439-45. doi: 10.1021/sb500225r. Epub 2014 May 21.

Abstract

Nisin is an important antimicrobial peptide that has enormous applications in biotechnology. Despite many encouraging efforts, its overproduction has been a long-standing challenge due to the complexity of the underlying pathway and the difficulty in genetic modification of lactic acid bacteria. Here, we cloned an entire nisin biosynthesis pathway from a nisin-producing strain (Lactococcus lactis K29) into a plasmid and transplanted the plasmid into a nisin deficient strain Lactococcus lactis MG1363, resulting in successful heterologous expression of bioactive recombinant nisin. To increase nisin harvest, we also overexpressed nisA, a gene responsible for nisin precursor production, with a set of constitutive promoters. To further optimize nisin yield, we minimized the metabolic cost of the engineered strains by integrating nisA overexpression cassettes and the recombinant pathway into a single circuit. With our rational construction and optimization, our engineered optimized strain is able to produce bioactive nisin with a yield of 1098 IU/mL, which is more than six times higher than that of the original strain.

摘要

乳酸链球菌素是一种重要的抗菌肽,在生物技术领域有广泛应用。尽管已经做出了许多令人鼓舞的努力,但由于其合成途径的复杂性以及对乳酸菌进行基因改造的困难,其过量生产一直是一个长期存在的挑战。在此,我们将来自乳酸链球菌素产生菌株(乳酸乳球菌K29)的完整乳酸链球菌素生物合成途径克隆到一个质粒中,并将该质粒转入乳酸链球菌素缺陷菌株乳酸乳球菌MG1363,从而成功实现了具有生物活性的重组乳酸链球菌素的异源表达。为了提高乳酸链球菌素的产量,我们还使用一组组成型启动子过表达了负责乳酸链球菌素前体产生的基因nisA。为了进一步优化乳酸链球菌素的产量,我们通过将nisA过表达盒和重组途径整合到一个单一回路中,最小化了工程菌株的代谢成本。通过我们合理的构建和优化,我们的工程优化菌株能够以1098 IU/mL的产量生产具有生物活性的乳酸链球菌素,这比原始菌株的产量高出六倍多。

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