Synergistic computational and experimental studies of a phosphoglycosyl transferase membrane/ligand ensemble.

The Journal of Biological Chemistry Pub Date : 2023-10-01 Epub Date: 2023-08-25 DOI:10.1016/j.jbc.2023.105194
Ayan Majumder, Nemanja Vuksanovic, Leah C Ray, Hannah M Bernstein, Karen N Allen, Barbara Imperiali, John E Straub
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Abstract

Complex glycans serve essential functions in all living systems. Many of these intricate and byzantine biomolecules are assembled employing biosynthetic pathways wherein the constituent enzymes are membrane-associated. A signature feature of the stepwise assembly processes is the essentiality of unusual linear long-chain polyprenol phosphate-linked substrates of specific isoprene unit geometry, such as undecaprenol phosphate (UndP) in bacteria. How these enzymes and substrates interact within a lipid bilayer needs further investigation. Here, we focus on a small enzyme, PglC from Campylobacter, structurally characterized for the first time in 2018 as a detergent-solubilized construct. PglC is a monotopic phosphoglycosyl transferase that embodies the functional core structure of the entire enzyme superfamily and catalyzes the first membrane-committed step in a glycoprotein assembly pathway. The size of the enzyme is significant as it enables high-level computation and relatively facile, for a membrane protein, experimental analysis. Our ensemble computational and experimental results provided a high-level view of the membrane-embedded PglC/UndP complex. The findings suggested that it is advantageous for the polyprenol phosphate to adopt a conformation in the same leaflet where the monotopic membrane protein resides as opposed to additionally disrupting the opposing leaflet of the bilayer. Further, the analysis showed that electrostatic steering acts as a major driving force contributing to the recognition and binding of both UndP and the soluble nucleotide sugar substrate. Iterative computational and experimental mutagenesis support a specific interaction of UndP with phosphoglycosyl transferase cationic residues and suggest a role for critical conformational transitions in substrate binding and specificity.

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磷酸糖基转移酶膜/配体系综的协同计算和实验研究。
复杂聚糖在所有生命系统中都具有重要功能。这些复杂的拜占庭生物分子中的许多是通过生物合成途径组装的,其中组成酶是膜相关的。逐步组装过程的一个标志性特征是具有特定异戊二烯单元几何形状的不同寻常的线性长链聚丙烯醇磷酸酯连接底物的重要性,例如细菌中的十一碳烯醇磷酸酯(UndP)。这些酶和底物如何在脂质双层中相互作用还需要进一步研究。在这里,我们关注的是一种来自弯曲杆菌的小酶PglC,它在2018年首次在结构上被表征为一种可溶解洗涤剂的构建体。PglC是一种单主题磷酸糖基转移酶,它体现了整个酶超家族的功能核心结构,并催化糖蛋白组装途径中的第一个膜结合步骤。酶的大小是重要的,因为它能够进行高水平的计算,并且对于膜蛋白来说,实验分析相对容易。我们的整体计算和实验结果提供了膜嵌入的PglC/UndP复合物的高级视图。研究结果表明,与额外破坏双层的相对小叶相比,聚丙醛磷酸酯在单主题膜蛋白所在的同一小叶中采用构象是有利的。此外,分析表明,静电操纵是有助于识别和结合UndP和可溶性核苷酸糖底物的主要驱动力。迭代计算和实验诱变支持UndP与磷酸糖基转移酶阳离子残基的特异性相互作用,并表明关键构象转变在底物结合和特异性中的作用。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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