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三聚体OmpF孔蛋白的稳定性:闩锁环L2的作用

Stability of trimeric OmpF porin: the contributions of the latching loop L2.

作者信息

Phale P S, Philippsen A, Kiefhaber T, Koebnik R, Phale V P, Schirmer T, Rosenbusch J P

机构信息

Division of Microbiology, Biozentrum, University of Basel, Switzerland.

出版信息

Biochemistry. 1998 Nov 10;37(45):15663-70. doi: 10.1021/bi981215c.

DOI:10.1021/bi981215c
PMID:9843370
Abstract

The channel-forming protein OmpF porin from Escherichia coli spans the bacterial outer membrane. Each of the three monomers comprises a hollow, 16-stranded beta-barrel. These are associated to homotrimers which are unusually stable, due mostly to hydrophobic interactions between the beta-barrels. In addition, a loop, L2 connects one subunit to its neighbor by latching into its channel. Residue E71 on loop 2 is integrated into an ionic network and forms salt bridges and hydrogen bonds with R100 and R132 on the channel wall in the adjacent subunit. To examine these contributions quantitatively, six single-site, two double, and one deletion mutant were constructed on the basis of the atomic coordinates of the protein. Differential scanning calorimetric analysis showed that the salt-bridge, E71-R100, contributes significantly to trimer stability: the substitution E71Q causes a decrease of the transition temperature from 72 to 48 degreesC, with DeltaHcal diminishing from 430 to 201 kcal mol-1. A nearby substitution in the loop, D74N, has lesser effects on thermal stability, while the deletion in L2 (Delta69-77) has an effect comparable to that of E71Q. X-ray structure analysis to 3.0 A resolution revealed only local structural differences in the mutants except for the substitution R100A, where another residue, R132, is found to fill the gap left by the truncated side chain of A100. Functional assays in planar lipid bilayers show significantly increased cation selectivities if the charge distribution was affected.

摘要

来自大肠杆菌的通道形成蛋白OmpF孔蛋白跨越细菌外膜。三个单体中的每一个都包含一个中空的、由16条链组成的β桶。这些单体缔合形成同三聚体,该同三聚体异常稳定,主要归因于β桶之间的疏水相互作用。此外,一个环L2通过嵌入其通道将一个亚基与其相邻亚基相连。环2上的残基E71整合到一个离子网络中,并与相邻亚基通道壁上的R100和R132形成盐桥和氢键。为了定量研究这些作用,基于该蛋白的原子坐标构建了6个单点突变体、2个双点突变体和1个缺失突变体。差示扫描量热分析表明,盐桥E71-R100对三聚体稳定性有显著贡献:E71Q取代导致转变温度从72℃降至48℃,ΔHcal从430 kcal mol-1降至201 kcal mol-1。环上附近的取代D74N对热稳定性的影响较小,而L2中的缺失(Δ69-77)的影响与E71Q相当。分辨率为3.0 Å的X射线结构分析表明,除了R100A取代外,突变体中仅存在局部结构差异,在R100A取代中,发现另一个残基R132填补了A100截断侧链留下的缺口。平面脂质双层中的功能测定表明,如果电荷分布受到影响,阳离子选择性会显著增加。

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