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棘孢小单孢菌中部分刺糖菌素生物合成基因簇的复制增强了刺糖菌素的生产。

Duplication of partial spinosyn biosynthetic gene cluster in Saccharopolyspora spinosa enhances spinosyn production.

机构信息

College of Life Science, Hunan Normal University, Hunan Provincial Key Laboratory of Microbial Molecular Biology, Changsha, China.

出版信息

FEMS Microbiol Lett. 2011 Dec;325(1):22-9. doi: 10.1111/j.1574-6968.2011.02405.x. Epub 2011 Oct 10.

DOI:10.1111/j.1574-6968.2011.02405.x
PMID:22092858
Abstract

Spinosyns, the secondary metabolites produced by Saccharopolyspora spinosa, are the active ingredients in a family of insect control agents. Most of the S. spinosa genes involved in spinosyn biosynthesis are found in a contiguous c. 74-kb cluster. To increase the spinosyn production through overexpression of their biosynthetic genes, part of its gene cluster (c. 18 kb) participating in the conversion of the cyclized polyketide to spinosyn was obtained by direct cloning via Red/ET recombination rather than by constructing and screening the genomic library. The resultant plasmid pUCAmT-spn was introduced into S. spinosa CCTCC M206084 from Escherichia coli S17-1 by conjugal transfer. The subsequent single-crossover homologous recombination caused a duplication of the partial gene cluster. Integration of this plasmid enhanced production of spinosyns with a total of 388 (± 25.0) mg L(-1) for spinosyns A and D in the exconjugant S. spinosa trans1 compared with 100 (± 7.7) mg L(-1) in the parental strain. Quantitative real time polymerase chain reaction analysis of three selected genes (spnH, spnI, and spnK) confirmed the positive effect of the overexpression of these genes on the spinosyn production. This study provides a simple avenue for enhancing spinosyn production. The strategies could also be used to improve the yield of other secondary metabolites.

摘要

斯氏多孢菌产生的斯彭诺菌素是一类昆虫控制剂的活性成分。大多数与斯彭诺菌素生物合成有关的斯氏多孢菌基因都存在于一个连续的大约 74kb 的簇中。为了通过过度表达其生物合成基因来提高斯彭诺菌素的产量,通过 Red/ET 重组直接克隆而不是构建和筛选基因组文库,获得了参与环化聚酮转化为斯彭诺菌素的部分基因簇(约 18kb)。所得质粒 pUCAmT-spn 通过接合转移从大肠杆菌 S17-1 引入到斯氏多孢菌 CCTCC M206084 中。随后的单交换同源重组导致部分基因簇的重复。该质粒的整合增强了斯彭诺菌素的产生,与亲本菌株相比,转 1 号斯氏多孢菌 exconjugant 中的斯彭诺菌素 A 和 D 的总产量达到 388(±25.0)mg/L,而亲本菌株中的产量为 100(±7.7)mg/L。对三个选定基因(spnH、spnI 和 spnK)的实时定量聚合酶链反应分析证实了这些基因的过度表达对斯彭诺菌素产生的积极影响。本研究为提高斯彭诺菌素的产量提供了一种简单的途径。这些策略也可用于提高其他次生代谢产物的产量。

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