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脂多糖与周质蛋白LptA结合。

Lipopolysaccharide binding to the periplasmic protein LptA.

作者信息

Schultz Kathryn M, Lundquist Tanner J, Klug Candice S

机构信息

Department of Biophysics, Medical College of Wisconsin, Milwaukee, Wisconsin, 53226.

出版信息

Protein Sci. 2017 Aug;26(8):1517-1523. doi: 10.1002/pro.3177. Epub 2017 Apr 30.

Abstract

Lipopolysaccharide (LPS) and the periplasmic protein, LptA, are two essential components of Gram-negative bacteria. LPS, also known as endotoxin, is found asymmetrically distributed in the outer leaflet of the outer membrane of Gram-negative bacteria such as Escherichia coli and plays a role in the organism's natural defense in adverse environmental conditions. LptA is a member of the lipopolysaccharide transport protein (Lpt) family, which also includes LptC, LptDE, and LptBFG , that functions to transport LPS through the periplasm to the outer leaflet of the outer membrane after MsbA flips LPS across the inner membrane. It is hypothesized that LPS binds to LptA to cross the periplasm and that the acyl chains of LPS bind to the central pocket of LptA. The studies described here are the first to comprehensively characterize and quantitate the binding of LPS by LptA. Using site-directed spin-labeling electron paramagnetic resonance (EPR) spectroscopy, data were collected for 15 spin-labeled residues in and around the proposed LPS binding pocket on LptA to observe the mobility changes caused by the presence of exogenous LPS and identify the binding location of LPS to LptA. The EPR data obtained suggest a 1:1 ratio for the LPS:LptA complex and allow the first calculation of dissociation constants for the LptA-LPS interaction. The results indicate that the entire protein is affected by LPS binding, the N-terminus unfolds in the presence of LPS, and a mutant LptA protein unable to form oligomers has an altered affinity for LPS.

摘要

脂多糖(LPS)和周质蛋白LptA是革兰氏阴性菌的两个重要组成部分。LPS也被称为内毒素,在大肠杆菌等革兰氏阴性菌的外膜外小叶中呈不对称分布,在生物体应对不利环境条件的天然防御中发挥作用。LptA是脂多糖转运蛋白(Lpt)家族的成员之一,该家族还包括LptC、LptDE和LptBFG,其功能是在MsbA将LPS翻转穿过内膜后,将LPS通过周质转运到外膜的外小叶。据推测,LPS与LptA结合以穿过周质,并且LPS的酰基链与LptA的中央口袋结合。本文所述的研究首次全面表征和定量了LptA与LPS的结合。使用定点自旋标记电子顺磁共振(EPR)光谱,收集了LptA上拟议的LPS结合口袋及其周围15个自旋标记残基的数据,以观察外源LPS的存在引起的流动性变化,并确定LPS与LptA的结合位置。获得的EPR数据表明LPS:LptA复合物的比例为1:1,并首次计算了LptA-LPS相互作用的解离常数。结果表明,整个蛋白质受到LPS结合的影响,N端在LPS存在下展开,并且无法形成寡聚体的突变LptA蛋白对LPS的亲和力发生了改变。

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