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南昌链霉菌是杀虫聚醚抗生素南昌霉素和抗寄生虫大环内酯类梅岭霉素的产生菌,它含有多个聚酮化合物基因簇。

'Streptomyces nanchangensis', a producer of the insecticidal polyether antibiotic nanchangmycin and the antiparasitic macrolide meilingmycin, contains multiple polyketide gene clusters.

作者信息

Sun Yuhui, Zhou Xiufen, Liu Jun, Bao Kai, Zhang Guiming, Tu Guoquan, Kieser Tobias, Deng Zixin

机构信息

Jiangxi Agricultural University, Nanchang 330045, China3.

Huazhong Agricultural University, Wuhan 430070, China2.

出版信息

Microbiology (Reading). 2002 Feb;148(Pt 2):361-371. doi: 10.1099/00221287-148-2-361.

DOI:10.1099/00221287-148-2-361
PMID:11832500
Abstract

Several independent gene clusters containing varying lengths of type I polyketide synthase genes were isolated from 'Streptomyces nanchangensis' NS3226, a producer of nanchangmycin and meilingmycin. The former is a polyether compound similar to dianemycin and the latter is a macrolide compound similar to milbemycin, which shares the same macrolide ring as avermectin but has different side groups. Clusters A-H spanned about 133, 132, 104, 174, 122, 54, 37 and 59 kb, respectively. Two systems were developed for functional analysis of the gene clusters by gene disruption or replacement. (1) Streptomyces phage phiC31 and its derived vectors can infect and lysogenize this strain. (2) pSET152, an Escherichia coli plasmid with phiC31 attP site, and pHZ1358, a Streptomyces-Escherichia coli shuttle cosmid vector, both carrying oriT from RP4, can be mobilized from E. coli into NS3226 by conjugation. pHZ1358 was shown to be generally useful for generating mutant strains by gene disruption and replacement in NS3226 as well as in several other Streptomyces strains. A region in cluster A (approximately 133 kb) seemed to be involved in nanchangmycin production because replacement of several DNA fragments in this region by an apramycin resistance gene [aac3(IV)] gave rise to nanchangmycin non-producing mutants.

摘要

从南昌霉素和梅岭霉素的产生菌南昌链霉菌NS3226中分离出了几个独立的基因簇,这些基因簇包含不同长度的I型聚酮合酶基因。前者是一种类似于地那霉素的聚醚化合物,后者是一种类似于米尔倍霉素的大环内酯化合物,它与阿维菌素具有相同的大环内酯环,但侧链不同。A-H基因簇分别跨越约133、132、104、174、122、54、37和59 kb。通过基因破坏或替换开发了两个系统用于基因簇的功能分析。(1)链霉菌噬菌体phiC31及其衍生载体可以感染该菌株并使其溶源化。(2)带有phiC31 attP位点的大肠杆菌质粒pSET152和带有来自RP4的oriT的链霉菌-大肠杆菌穿梭粘粒载体pHZ1358,可以通过接合从大肠杆菌转移到NS3226中。结果表明,pHZ1358通常可用于通过基因破坏和替换在NS3226以及其他几种链霉菌菌株中产生突变菌株。A基因簇中的一个区域(约133 kb)似乎与南昌霉素的产生有关,因为用安普霉素抗性基因[aac3(IV)]替换该区域中的几个DNA片段会产生不产生南昌霉素的突变体。

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