Direct Cloning, Genetic Engineering, and Heterologous Expression of the Syringolin Biosynthetic Gene Cluster in E. coli through Red/ET Recombineering

重组工程 生物 基因簇 克隆(编程) 异源表达 基因 大肠杆菌 同源重组 遗传学 计算生物学 异源的 重组DNA 计算机科学 程序设计语言
作者
Xiaoying Bian,Fan Huang,Francis Stewart,Liqiu Xia,Youming Zhang,Rolf Müller
出处
期刊:ChemBioChem [Wiley]
卷期号:13 (13): 1946-1952 被引量:70
标识
DOI:10.1002/cbic.201200310
摘要

Abstract The reconstruction of a natural product biosynthetic pathway from bacteria in a vector and subsequent heterologous expression in a technically amenable microbial system represents an efficient alternative to empirical traditional methods for functional discovery, yield improvement, and genetic engineering to produce “unnatural” derivatives. However, the traditional cloning procedure based on genomic library construction and screening are complicated due to the large size (>10 kb) of most biosynthetic pathways. Here, we describe the direct cloning of a partial syringolin biosynthetic gene cluster ( sylCDE , 19 kb) from a digested genomic DNA mixture of Pseudomonas syringae into a plasmid in which sylCDE is under the control of an inducible promoter by one step linear‐plus‐linear homologous recombination (LLHR) in Escherichia coli . After expression in E. coli GB05‐MtaA, two new syringolin derivatives were discovered. The complete syringolin gene cluster was assembled by addition of sylAB and exchange of a synthetic bidirectional promoter against the native promoter to drive sylB and sylC expression by using Red/ET recombineering. The varying production distribution of syringolin derivatives showed the different efficiencies of native and synthetic promoters in E. coli . The successful reconstitution and expression of the syringolin biosynthetic pathway shows that Red/ET recombineering is an efficient tool to clone and engineer secondary metabolite biosynthetic pathways.
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