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一种用于分析和操纵地中海拟无枝酸菌中利福霉素聚酮生物合成的宿主-载体系统。

A host-vector system for analysis and manipulation of rifamycin polyketide biosynthesis in Amycolatopsis mediterranei.

作者信息

Hu Zhihao, Hunziker Daniel, Hutchinson C Richard, Khosla Chaitan

机构信息

Departments of Chemical Engineering1, Chemistry and Biochemistry2, Stanford University, Stanford, CA 94305-5025, USA.

出版信息

Microbiology (Reading). 1999 Sep;145 ( Pt 9):2335-2341. doi: 10.1099/00221287-145-9-2335.

DOI:10.1099/00221287-145-9-2335
PMID:10517586
Abstract

Modular polyketide synthases (PKSs) are a large family of multifunctional enzymes responsible for the biosynthesis of numerous bacterial natural products such as erythromycin and rifamycin. Advanced genetic analysis of these remarkable systems is often seriously hampered by the large size (>40 kb) of PKS gene clusters, and, notwithstanding their considerable fundamental and biotechnological significance, by the lack of suitable methods for engineering non-selectable modifications in chromosomally encoded PKS genes. The development of a facile host-vector strategy for genetic engineering of the rifamycin PKS in the producing organism, Amycolatopsis mediterranei S699, is described here. The genes encoding all 10 modules of the rifamycin PKS were replaced with a hygromycin-resistance marker gene. In a similar construction, only the first six modules of the PKS were replaced. The deletion hosts retained the ability to synthesize the primer unit 3-amino-5-hydroxybenzoic acid (AHBA), as judged by co-synthesis experiments with a mutant strain lacking AHBA synthase activity. Suicide plasmids carrying a short fragment from the 5' flanking end of the engineered deletion, an apramycin-resistance marker gene, and suitably engineered PKS genes could be introduced via electroporation into the deletion hosts, resulting in the integration of PKS genes and biosynthesis of a reporter polyketide in quantities comparable to those produced by the wild-type organism. Since this strategy for engineering recombinant PKSs in A. mediterranei requires only a selectable single crossover and eliminates the need for tedious non-selectable double-crossover experiments, it makes rifamycin PKS an attractive target for extensive genetic manipulation.

摘要

模块化聚酮合酶(PKSs)是一类多功能酶的大家族,负责多种细菌天然产物的生物合成,如红霉素和利福霉素。这些卓越系统的深入遗传分析常常因PKS基因簇的大尺寸(>40 kb)而受到严重阻碍,而且,尽管它们具有相当重要的基础和生物技术意义,但由于缺乏对染色体编码的PKS基因进行非选择性修饰的合适方法,也受到阻碍。本文描述了一种用于在生产菌株地中海拟无枝酸菌S699中对利福霉素PKS进行基因工程的简便宿主-载体策略的开发。编码利福霉素PKS所有10个模块的基因被潮霉素抗性标记基因取代。在类似的构建中,仅PKS的前六个模块被取代。通过与缺乏AHBA合酶活性的突变菌株的共合成实验判断,缺失宿主保留了合成引物单元3-氨基-5-羟基苯甲酸(AHBA)的能力。携带来自工程缺失5'侧翼末端的短片段、阿泊拉霉素抗性标记基因和经过适当工程改造的PKS基因的自杀质粒可通过电穿孔导入缺失宿主,导致PKS基因整合并合成与野生型生物体产生的量相当的报告聚酮化合物。由于在地中海拟无枝酸菌中构建重组PKS的这种策略仅需要可选择的单交换,并且无需繁琐的不可选择的双交换实验,因此它使利福霉素PKS成为广泛遗传操作的有吸引力的目标。

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Stereochemical assignment of intermediates in the rifamycin biosynthetic pathway by precursor-directed biosynthesis.通过前体定向生物合成对利福霉素生物合成途径中的中间体进行立体化学归属。
J Am Chem Soc. 2005 Aug 17;127(32):11202-3. doi: 10.1021/ja051430y.
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Development of cloning vectors and transformation methods for Amycolatopsis.拟无枝酸菌克隆载体及转化方法的开发
J Ind Microbiol Biotechnol. 2003 Apr;30(4):195-204. doi: 10.1007/s10295-003-0040-6. Epub 2003 Apr 8.