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Nonactin Biosynthesis: the Product of nonS Catalyzes the Formation of the Furan Ring of Nonactic Acid

机译:非肌动蛋白的生物合成:nonS的产物催化非乳酸呋喃环的形成

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摘要

Nonactin is the parent compound of a group of ionophore antibiotics, known as the macrotetrolides, produced by Streptomyces griseus subsp. griseus ETH A7796. Nonactin is a significant compound because of its inhibitory effects on the P170 glycoprotein-mediated efflux of chemotherapeutic agents in multiple-drug-resistant cancer cells. Nonactin is also significant in that it is a highly atypical polyketide. Very little is presently known about the genes of the nonactin biosynthesis cluster. In this paper we describe our efforts to establish a connection between the product of a gene from the nonactin biosynthesis cluster and a known biochemical transformation in nonactin biosynthesis. Nonactate synthase is the enzyme which catalyzes the formation of nonactic acid from an acyclic precursor in nonactin biosynthesis. We have synthesized the substrate for this enzyme and have detected the in vitro cyclization activity of the substrate in cell-free preparations of S. griseus subsp. griseus ETH A7796. Previous studies by R. Plater and J. A. Robinson (Gene 112:117–122, 1992) had suggested, based on sequence homology, that the product of a partial open reading frame found close to the tetranactin resistance gene of S. griseus could be the nonactate synthase. We have therefore cloned, sequenced, and heterologously expressed this full gene (nonS), and we have shown that the gene product, NonS, does indeed catalyze the formation of the furan ring of nonactic acid as hypothesized.
机译:Nonactin是由灰链霉菌亚种生产的一组离子载体抗生素(称为大环内酯)的母体化合物。 griseus ETH A7796。非肌动蛋白是重要的化合物,因为它对多重耐药性癌细胞中P170糖蛋白介导的化学治疗药物的流出具有抑制作用。非肌动蛋白也很重要,因为它是高度非典型的聚酮化合物。目前对非肌动蛋白生物合成簇的基因知之甚少。在本文中,我们描述了我们在非肌动蛋白生物合成簇中的基因产物与非肌动蛋白生物合成中已知的生化转化之间建立联系的努力。非actate合酶是催化非actin生物合成中非环状前体形成nonactic acid的酶。我们已经合成了这种酶的底物,并在无糖链球菌亚种的无细胞制剂中检测了底物的体外环化活性。 griseus ETH A7796。 R. Plater和JA Robinson先前的研究(基因112:117–122,1992)基于序列同源性建议,发现接近灰霉菌四联素抗性基因的部分开放阅读框的产物可能是非乳酸合成酶。因此,我们已经克隆,测序并异源表达了这个完整的基因(nonS),并且我们已经证明,基因产物NonS确实确实催化了假设的非乳酸呋喃环的形成。

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