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橄榄色链霉菌S-140中编码抗肿瘤大环内酯类抗生素连氮霉素生物合成的基因簇的鉴定与定位。

Identification and localization of the gene cluster encoding biosynthesis of the antitumor macrolactam leinamycin in Streptomyces atroolivaceus S-140.

作者信息

Cheng Yi-Qiang, Tang Gong-Li, Shen Ben

机构信息

Division of Pharmaceutical Sciences. Department of Chemistry, University of Wisconsin, Madison 53705, USA.

出版信息

J Bacteriol. 2002 Dec;184(24):7013-24. doi: 10.1128/JB.184.24.7013-7024.2002.

Abstract

Leinamycin (LNM), produced by Streptomyces atroolivaceus, is a thiazole-containing hybrid peptide-polyketide natural product structurally characterized with an unprecedented 1,3-dioxo-1,2-dithiolane moiety that is spiro-fused to a 18-member macrolactam ring. LNM exhibits a broad spectrum of antimicrobial and antitumor activities, most significantly against tumors that are resistant to clinically important anticancer drugs, resulting from its DNA cleavage activity in the presence of a reducing agent. Using a PCR approach to clone a thiazole-forming nonribosomal peptide synthetase (NRPS) as a probe, we localized a 172-kb DNA region from S. atroolivaceus S-140 that harbors the lnm biosynthetic gene cluster. Sequence analysis of 11-kb DNA revealed three genes, lnmG, lnmH, and lnmI, and the deduced product of lnmI is characterized by domains characteristic to both NRPS and polyketide synthase (PKS). The involvement of the cloned gene cluster in LNM biosynthesis was confirmed by disrupting the lnmI gene to generate non-LNM-producing mutants and by characterizing LnmI as a hybrid NRPS-PKS megasynthetase, the NRPS module of which specifies for L-Cys and catalyzes thiazole formation. These results have now set the stage for full investigations of LNM biosynthesis and for generation of novel LNM analogs by combinatorial biosynthesis.

摘要

链黑菌素(LNM)由橄榄色链霉菌产生,是一种含噻唑的杂合肽-聚酮天然产物,其结构特征是具有一个前所未有的1,3-二氧代-1,2-二硫戊环部分,该部分与一个18元大环内酰胺环螺稠合。LNM具有广泛的抗菌和抗肿瘤活性,对临床上重要抗癌药物耐药的肿瘤活性最为显著,这源于其在还原剂存在下的DNA切割活性。我们采用PCR方法克隆形成噻唑的非核糖体肽合成酶(NRPS)作为探针,从橄榄色链霉菌S-140中定位了一个172 kb的DNA区域,该区域包含lnm生物合成基因簇。对11 kb DNA的序列分析揭示了三个基因,lnmG、lnmH和lnmI,lnmI推导的产物具有NRPS和聚酮合酶(PKS)的特征结构域。通过破坏lnmI基因产生不产生LNM的突变体,并将LnmI鉴定为一种杂合NRPS-PKS巨型合成酶,其NRPS模块指定L-半胱氨酸并催化噻唑形成,从而证实了克隆的基因簇参与LNM生物合成。这些结果为全面研究LNM生物合成以及通过组合生物合成产生新型LNM类似物奠定了基础。

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