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Fluorescent probes for investigation of isoprenoid configuration and size discrimination by bactoprenol-utilizing enzymes

机译:荧光探针用于研究利用类胡萝卜素的类异戊二烯构型和大小区分

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摘要

Undecaprenyl Pyrophosphate Synthase (UPPS) is an enzyme critical to the production of complex polysaccharides in bacteria, as it produces the crucial bactoprenol scaffold on which these materials are assembled. Methods to characterize the systems associated with polysaccharide production are non-trivial, in part due to the lack of chemical tools to investigate their assembly. In this report, we develop a new fluorescent tool using UPPS to incorporate a powerful fluorescent anthranilamide moiety into bactoprenol. The activity of this analogue in polysaccharide biosynthesis is then tested with the initiating hexose-1-phosphate transferases involved in Capsular Polysaccharide A biosynthesis in the symbiont Bacteroides fragilis and the asparagine-linked glycosylation system of the pathogenic Campylobacter jejuni. In addition, it is shown that the UPPS used to make this probe is not specific for E-configured isoprenoid substrates and that elongation by UPPS is required for activity with the downstream enzymes.
机译:十一碳烯基焦磷酸合酶(UPPS)是细菌中复杂多糖生产的关键酶,因为它会产生关键的细菌素肾上腺素支架,将这些材料组装在其上。表征与多糖生产相关的系统的方法并不简单,部分原因是缺乏研究其组装的化学工具。在本报告中,我们开发了一种新的荧光工具,使用UPPS将功能强大的荧光邻氨基苯甲酰胺部分掺入到贝托酚中。然后用参与荚膜多糖A的脆弱共生细菌和空肠弯曲杆菌空肠天冬酰胺连接的糖基化系统中涉及的荚膜多糖A的起始合成的磷酸1-己糖转移酶测试该类似物在多糖生物合成中的活性。另外,显示出用于制造该探针的UPPS对E-构型的类异戊二烯底物不是特异性的,并且与下游酶的活性需要UPPS的延伸。

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