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枯草芽孢杆菌 LytR-CpsA-Psr 酶在体外将真正的脂连接底物上的壁磷壁酸转移到成熟肽聚糖上。

B. subtilis LytR-CpsA-Psr Enzymes Transfer Wall Teichoic Acids from Authentic Lipid-Linked Substrates to Mature Peptidoglycan In Vitro.

机构信息

Department of Biochemistry and Biomedical Sciences, Michael G. DeGroote Institute for Infectious Disease Research, McMaster University, Hamilton, ON L8N 3Z5, Canada.

Department of Biochemistry and Center for Blood Research, University of British Columbia, Vancouver, BC V6T 1Z3, Canada.

出版信息

Cell Chem Biol. 2017 Dec 21;24(12):1537-1546.e4. doi: 10.1016/j.chembiol.2017.09.006. Epub 2017 Oct 26.

Abstract

Gram-positive bacteria endow their peptidoglycan with glycopolymers that are crucial for viability and pathogenesis. However, the cellular machinery that executes this function is not well understood. While decades of genetic and phenotypic work have highlighted the LytR-CpsA-Psr (LCP) family of enzymes as cell-wall glycopolymer transferases, their in vitro characterization has been elusive, largely due to a paucity of tools for functional assays. In this report, we synthesized authentic undecaprenyl diphosphate-linked wall teichoic acid (WTA) intermediates and built an assay system capable of monitoring LCP-mediated glycopolymer transfer. We report that all Bacillus subtilis LCP enzymes anchor WTAs to peptidoglycan in vitro. Furthermore, we probed the catalytic requirements and substrate preferences for these LCP enzymes and elaborated in vitro conditions for facile tests of enzyme function. This work sheds light on the molecular features of glycopolymer transfer and aims to aid drug discovery and development programs exploiting this promising antibacterial target.

摘要

革兰氏阳性菌赋予其肽聚糖带有糖聚合物,这对于其生存力和致病性至关重要。然而,执行此功能的细胞机制还不是很清楚。虽然几十年来的遗传和表型研究已经强调了 LytR-CpsA-Psr(LCP)家族的酶作为细胞壁糖聚合物转移酶,但它们的体外特性一直难以捉摸,主要是因为缺乏用于功能测定的工具。在本报告中,我们合成了真实的十一烯基二磷酸连接的细胞壁磷壁酸(WTA)中间体,并建立了一个能够监测 LCP 介导的糖聚合物转移的测定系统。我们报告说,所有枯草芽孢杆菌 LCP 酶都在体外将 WTAs 锚定在肽聚糖上。此外,我们探究了这些 LCP 酶的催化要求和底物偏好,并详细阐述了易于测试酶功能的体外条件。这项工作阐明了糖聚合物转移的分子特征,并旨在为利用这一有前途的抗菌靶标进行药物发现和开发计划提供帮助。

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