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A lanthipeptide library used to identify a protein–protein interaction inhibitor

机译:用来鉴定蛋白质与蛋白质相互作用抑制剂的多肽肽库

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摘要

We describe the production and screening of a genetically encoded library of 106 lanthipeptides in Escherichia coli using the substrate-tolerant lanthipeptide synthetase ProcM. This plasmidencoded library was combined with a bacterial reverse two-hybrid system for the interaction of the HIV p6 protein with the UEV domain of the human TSG101 protein, a critical protein–protein interaction for HIV budding from infected cells. Using this approach, we identified an inhibitor of this interaction from the lanthipeptide library, whose activity was verified in vitro and in cell-based virus-like particle budding assays. Given the variety of lanthipeptide backbone scaffolds that may be produced with ProcM, this method may be used for the generation of genetically encoded libraries of natural product-like lanthipeptides containing substantial structural diversity. Such libraries may be combined with any cell-based assay for the identification of lanthipeptides with new biological activities.
机译:我们描述了使用底物耐受性多肽肽合成酶ProcM在大肠杆菌中生产和筛选10 6 多肽肽的遗传编码文库。该质粒编码的文库与细菌反向双杂交系统结合使用,可将HIV p6蛋白与人TSG101蛋白的UEV域相互作用,这是从感染细胞中萌发的HIV的关键蛋白-蛋白相互作用。使用这种方法,我们从lanthipeptide库中鉴定了这种相互作用的抑制剂,该抑制剂的活性已在体外和基于细胞的病毒样颗粒出芽测定中得到验证。鉴于可以用ProcM产生的多种多肽肽骨架支架,该方法可用于生成包含大量结构多样性的天然产物样多肽的遗传编码文库。此类文库可与任何基于细胞的测定法结合使用,以鉴定具有新的生物活性的瘦肽。

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