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通过非典型应答调节因子的表达鉴定金蒽醌生物合成基因簇。

Identification of the kinanthraquinone biosynthetic gene cluster by expression of an atypical response regulator.

作者信息

Takao Risa, Sakai Katsuyuki, Koshino Hiroyuki, Osada Hiroyuki, Takahashi Shunji

机构信息

Graduate School of Science and Engineering, Saitama University, Sakura-ku, Saitama-shi, Saitama, Japan.

Natural Product Biosynthesis Research Unit, RIKEN Centre for Sustainable Resource Science, Wako, Saitama, Japan.

出版信息

Biosci Biotechnol Biochem. 2021 Feb 24;85(3):714-721. doi: 10.1093/bbb/zbaa082.

Abstract

Recent advances in genome sequencing have revealed a variety of secondary metabolite biosynthetic gene clusters in actinomycetes. Understanding the biosynthetic mechanism controlling secondary metabolite production is important for utilizing these gene clusters. In this study, we focused on the kinanthraquinone biosynthetic gene cluster, which has not been identified yet in Streptomyces sp. SN-593. Based on chemical structure, 5 type II polyketide synthase gene clusters were listed from the genome sequence of Streptomyces sp. SN-593. Among them, a candidate gene cluster was selected by comparing the gene organization with grincamycin, which is synthesized through an intermediate similar to kinanthraquinone. We initially utilized a BAC library for subcloning the kiq gene cluster, performed heterologous expression in Streptomyces lividans TK23, and identified the production of kinanthraquinone and kinanthraquinone B. We also found that heterologous expression of kiqA, which belongs to the DNA-binding response regulator OmpR family, dramatically enhanced the production of kinanthraquinones.

摘要

基因组测序的最新进展揭示了放线菌中多种次生代谢物生物合成基因簇。了解控制次生代谢物产生的生物合成机制对于利用这些基因簇至关重要。在本研究中,我们聚焦于链霉菌属SN-593中尚未鉴定的kinanthraquinone生物合成基因簇。基于化学结构,从链霉菌属SN-593的基因组序列中列出了5个II型聚酮合酶基因簇。其中,通过将基因组织与通过类似于kinanthraquinone的中间体合成的grincamycin进行比较筛选出一个候选基因簇。我们最初利用BAC文库对kiq基因簇进行亚克隆,在变铅青链霉菌TK23中进行异源表达,并鉴定出kinanthraquinone和kinanthraquinone B的产生。我们还发现,属于DNA结合反应调节因子OmpR家族的kiqA的异源表达显著提高了kinanthraquinones的产量。

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