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光活化糖脂探针用于鉴定活分枝杆菌中类脂-蛋白相互作用。

Photoactivatable Glycolipid Probes for Identifying Mycolate-Protein Interactions in Live Mycobacteria.

机构信息

Department of Chemistry and Biochemistry, Central Michigan University, Mount Pleasant, Michigan 48859, United States.

Department of Microbiology, University of Massachusetts, Amherst, Massachusetts 01003, United States.

出版信息

J Am Chem Soc. 2020 Apr 29;142(17):7725-7731. doi: 10.1021/jacs.0c01065. Epub 2020 Apr 20.

Abstract

Mycobacteria have a distinctive glycolipid-rich outer membrane, the mycomembrane, which is a critical target for tuberculosis drug development. However, proteins that associate with the mycomembrane, or that are involved in its metabolism and host interactions, are not well-characterized. To facilitate the study of mycomembrane-related proteins, we developed photoactivatable trehalose monomycolate analogues that metabolically incorporate into the mycomembrane in live mycobacteria, enabling photo-cross-linking and click-chemistry-mediated analysis of mycolate-interacting proteins. When deployed in with quantitative proteomics, this strategy enriched over 100 proteins, including the mycomembrane porin (MspA), several proteins with known mycomembrane synthesis or remodeling functions (CmrA, MmpL3, Ag85, Tdmh), and numerous candidate mycolate-interacting proteins. Our approach is highly versatile, as it (i) enlists click chemistry for flexible protein functionalization; (ii) in principle can be applied to any mycobacterial species to identify endogenous bacterial proteins or host proteins that interact with mycolates; and (iii) can potentially be expanded to investigate protein interactions with other mycobacterial lipids. This tool is expected to help elucidate fundamental physiological and pathological processes related to the mycomembrane and may reveal novel diagnostic and therapeutic targets.

摘要

分枝杆菌具有独特的富含糖脂的外层膜,即类脂膜,这是结核病药物开发的关键靶点。然而,与类脂膜相关的蛋白质,或参与其代谢和宿主相互作用的蛋白质,尚未得到很好的描述。为了促进类脂膜相关蛋白的研究,我们开发了光活化海藻糖单酯类似物,这些类似物在活分枝杆菌中代谢掺入类脂膜,能够进行光交联和点击化学介导的类脂酰相互作用蛋白分析。当与定量蛋白质组学结合使用时,这种策略富集了超过 100 种蛋白质,包括类脂膜孔蛋白(MspA)、几种已知具有类脂膜合成或重塑功能的蛋白质(CmrA、MmpL3、Ag85、Tdmh)以及许多候选的类脂酰相互作用蛋白。我们的方法具有高度的通用性,因为它 (i) 利用点击化学进行灵活的蛋白质功能化;(ii) 原则上可以应用于任何分枝杆菌物种,以鉴定与类脂酰相互作用的内源性细菌蛋白或宿主蛋白;和 (iii) 可能扩展到研究与其他分枝杆菌脂质相互作用的蛋白质。该工具有望帮助阐明与类脂膜相关的基本生理和病理过程,并可能揭示新的诊断和治疗靶点。

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