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具核梭杆菌主要外膜蛋白FomA的蛋白质-脂质相互作用:自旋标记电子顺磁共振和偏振红外光谱法

Protein-lipid interactions with Fusobacterium nucleatum major outer membrane protein FomA: spin-label EPR and polarized infrared spectroscopy.

作者信息

Anbazhagan V, Vijay N, Kleinschmidt J H, Marsh D

机构信息

Max-Planck-Institut fur biophysikalische Chemie, Abt. Spektroskopie, 37070 Gottingen, Germany.

出版信息

Biochemistry. 2008 Aug 12;47(32):8414-23. doi: 10.1021/bi800750s. Epub 2008 Jul 19.

DOI:10.1021/bi800750s
PMID:18642853
Abstract

FomA, the major outer membrane protein of Fusobacterium nucleatum, was expressed and purified in Escherichia coli and reconstituted from detergent in bilayer membranes of phosphatidylcholines with chain lengths from C(12:0) to C(17:0). The conformation and orientation of membrane-incorporated FomA were determined from polarized, attenuated total reflection, infrared (IR) spectroscopy, and lipid-protein interactions with FomA were characterized by using electron paramagnetic resonance (EPR) spectroscopy of spin-labeled lipids. Approximately 190 residues of membranous FomA are estimated to be in a beta-sheet configuration from IR band fitting, which is consistent with a 14-strand transmembrane beta-barrel structure. IR dichroism of FomA indicates that the beta-strands are tilted by approximately 45 degrees relative to the sheet/barrel axis and that the order parameter of the latter displays a discontinuity corresponding to hydrophobic matching with fluid C(13:0) lipid chains. The stoichiometry ( N b = 23 lipids/monomer) of lipid-protein interaction from EPR demonstrates that FomA is not trimeric in membranes of diC(14:0) phosphatidylcholine and is consistent with a monomeric beta-barrel of 14-16 strands. The pronounced selectivity of interaction found with anionic spin-labeled lipids places basic residues of the protein in the vicinity of the polar-apolar membrane interfaces, consistent with current topology models. Comparison with similar data from the 8- to 22-stranded E. coli outer membrane proteins, OmpA, OmpG, and FhuA, supports the above conclusions.

摘要

具核梭杆菌的主要外膜蛋白FomA在大肠杆菌中表达并纯化,然后从去污剂中重构到链长从C(12:0)到C(17:0)的磷脂酰胆碱双层膜中。通过偏振衰减全反射红外(IR)光谱确定膜整合FomA的构象和取向,并使用自旋标记脂质的电子顺磁共振(EPR)光谱表征FomA与脂质的相互作用。通过IR谱带拟合估计,膜结合FomA中约190个残基处于β-折叠构象,这与14链跨膜β-桶结构一致。FomA的红外二色性表明,β-链相对于片层/桶轴倾斜约45度,并且后者的序参量显示出与流动性C(13:0)脂质链疏水匹配相对应的不连续性。EPR得出的脂质-蛋白质相互作用的化学计量比(Nb = 23脂质/单体)表明,FomA在二C(14:0)磷脂酰胆碱膜中不是三聚体,与14 - 16链的单体β-桶一致。与阴离子自旋标记脂质相互作用的明显选择性将蛋白质的碱性残基置于极性-非极性膜界面附近,这与当前的拓扑模型一致。与8至22链大肠杆菌外膜蛋白OmpA、OmpG和FhuA的类似数据比较支持上述结论。

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