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吸水链霉菌JCM4427中参与格尔德霉素聚酮化合物修饰的剪裁基因的表征

Characterization of tailoring genes involved in the modification of geldanamycin polyketide in Streptomyces hygroscopicus JCM4427.

作者信息

Shin Jin-Chul, Na Zhu, Lee Dong-Ho, Kim Won-Cheol, Lee Kyeong, Shen Yue-Mao, Paik Sang-Gi, Hong Young-Soo, Lee Jung-Joon

机构信息

Korea Research Institute of Bioscience and Biotechnology, Daejeon, Korea.

出版信息

J Microbiol Biotechnol. 2008 Jun;18(6):1101-8.

Abstract

Geldanamycin and its analogs are important anticancer agents that inhibit the newly targeted, heat-shock protein (Hsp) 90, which is a chaperone protein in eukaryotic cells. To resolve which geldanamycin biosynthetic genes are responsible for particular post-polyketide synthase (PKS) processing steps and in which order the reactions occur, we individually inactivated candidate genes in Streptomyces hygroscopicus subsp. duamyceticus JCM4427, and isolated and elucidated the structures of intermediates from each mutant. The results indicated that gel7 governs at least one of the benzoquinone ring oxidation steps. In addition, gel16 was found to be involved in double-bond formation between C-4 and C-5 of 4,5-dihydrogeldanamycin, which confirmed our previous findings that this double bond reduced during the post-PKS modification of the polyketide assembly. In addition, pro-geldanamycin, which does not possess a double bond at C-4/5, was purified from the gel7 and 8 double-gene-inactivated mutant.

摘要

格尔德霉素及其类似物是重要的抗癌药物,它们能抑制新的靶点——热休克蛋白(Hsp)90,Hsp90是真核细胞中的一种伴侣蛋白。为了确定哪些格尔德霉素生物合成基因负责特定的聚酮合酶(PKS)后加工步骤以及反应按何种顺序发生,我们分别使吸水链霉菌亚种杜瓦霉素链霉菌JCM4427中的候选基因失活,并从每个突变体中分离和阐明中间体的结构。结果表明,gel7至少控制着苯醌环氧化步骤中的一个。此外,发现gel16参与4,5-二氢格尔德霉素C-4和C-5之间的双键形成,这证实了我们之前的发现,即该双键在聚酮组装的PKS后修饰过程中会减少。此外,从gel7和8双基因失活突变体中纯化出了在C-4/5处不具有双键的前体格尔德霉素。

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