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Reconstitution of the Myxothiazol Biosynthetic Gene Cluster by Red/ET Recombination and Heterologous Expression in Myxococcus xanthus

机译:红色/ ET重组和异源表达在黄色粘球菌中重构的噻噻唑生物合成基因簇。

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Although many secondary metabolites exhibiting important pharmaceutical and agrochemical activities have been isolated from myxobacteria, most of these microorganisms remain difficult to handle genetically. To utilize their metabolic potential, heterologous expression methodologies are currently being developed. Here, the Red/ET recombination technology was used to perform all required gene cluster engineering steps in Escherichia coli prior to the transfer into the chromosome of the heterologous host. We describe the integration of the complete 57-kbp myxothiazol biosynthetic gene cluster reconstituted from two cosmids from a cosmid library of the myxobacterium Stigmatella aurantiaca DW4-3/1 into the chromosome of the thus far best-characterized myxobacterium, Myxococcus xanthus, in one step. The successful integration and expression of the myxothiazol biosynthetic genes in M. xanthus results in the production of myxothiazol in yields comparable to the natural producer strain.
机译:尽管已从粘菌中分离出许多具有重要药物和农用化学活性的次生代谢产物,但这些微生物大多数仍难以通过基因处理。为了利用它们的代谢潜能,目前正在开发异源表达方法。在这里,在转移到异源宿主的染色体中之前,使用Red / ET重组技术在大肠杆菌中执行了所有必需的基因簇工程步骤。我们描述了一个完整的57 kbp的噻虫唑生物合成基因簇的整合,一步一步是将两个粘粒从粘胶条杆菌Astantitella aurantiaca DW4-3 / 1的粘粒文库中重组到迄今最具特征的粘杆菌属,即黄粘球菌的染色体中。木霉中的噻噻唑生物合成基因的成功整合和表达导致生产出与天然生产菌株相当的霉菌唑。

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