Wong K K, Brinkman F S, Benz R S, Hancock R E
Department of Microbiology and Immunology, University of British Columbia, Vancouver, British Columbia, Canada V6T 1Z3.
J Bacteriol. 2001 Jan;183(1):367-74. doi: 10.1128/JB.183.1.367-374.2001.
The outer membrane protein OprM of Pseudomonas aeruginosa is involved in intrinsic and mutational multiple-antibiotic resistance as part of two resistance-nodulation-division efflux systems. The crystal structure of TolC, a homologous protein in Escherichia coli, was recently published (V. Koronakis, A. Sharff, E. Koronakis, B. Luisl, and C. Hughes, Nature 405:914-919, 2000), demonstrating a distinctive architecture comprising outer membrane beta-barrel and periplasmic helical-barrel structures, which assemble differently from the common beta-barrel-only conformation of porins. Based on their sequence similarity, a similar content of alpha-helical and beta-sheet structure determined by circular dichroism spectroscopy, and our observation that OprM, like TolC, reconstitutes channels in planar bilayer membranes, OprM and TolC were considered to be structurally homologous, and a model of OprM was constructed by threading its sequence to the TolC crystal structure. Residues thought to be important for the TolC structure were conserved in space in this OprM model. Analyses of deletion mutants and previously isolated insertion mutants of OprM in the context of this model allowed us to propose roles for different protein domains. Our data indicate that the helical barrel of the protein is critical for both the function and the integrity of the protein, while a C-terminal domain localized around the equatorial plane of this helical barrel is dispensable. Extracellular loops appear to play a lesser role in substrate specificity for this efflux protein compared to classical porins, and there appears to be a correlation between the change in antimicrobial activity for OprM mutants and the pore size. Our model and channel formation studies support the "iris" mechanism of action for TolC and permit us now to form more focused hypotheses about the functional domains of OprM and its related family of efflux proteins.
铜绿假单胞菌的外膜蛋白OprM作为两个耐药-结瘤-分裂(RND)外排系统的一部分,参与固有和突变型多重抗生素耐药。最近发表了大肠杆菌中同源蛋白TolC的晶体结构(V. Koronakis、A. Sharff、E. Koronakis、B. Luisl和C. Hughes,《自然》405:914 - 919,2000),显示出一种独特的结构,由外膜β桶和周质螺旋桶结构组成,其组装方式不同于孔蛋白常见的仅含β桶的构象。基于它们的序列相似性、通过圆二色光谱法测定的α螺旋和β折叠结构的相似含量,以及我们观察到OprM与TolC一样能在平面双层膜中重构通道,OprM和TolC被认为在结构上是同源的,并通过将OprM的序列穿线到TolC晶体结构上构建了OprM模型。在这个OprM模型中,被认为对TolC结构重要的残基在空间上是保守的。在这个模型背景下对OprM缺失突变体和先前分离的插入突变体的分析使我们能够提出不同蛋白质结构域的作用。我们的数据表明,该蛋白的螺旋桶对蛋白的功能和完整性都至关重要,而位于该螺旋桶赤道平面周围的C末端结构域是可有可无的。与经典孔蛋白相比,细胞外环在这种外排蛋白的底物特异性方面似乎作用较小,并且OprM突变体抗菌活性的变化与孔径之间似乎存在相关性。我们的模型和通道形成研究支持了TolC的“虹膜”作用机制,现在使我们能够对OprM及其相关外排蛋白家族的功能结构域形成更有针对性的假设。
