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PilN、PilO 和 PilP 型 IVa 菌毛亚基复合物的特性研究。

Characterization of the PilN, PilO and PilP type IVa pilus subcomplex.

机构信息

Program in Molecular Structure and Function, The Hospital for Sick Children, Toronto, Ontario, M5G 1X8, Canada.

出版信息

Mol Microbiol. 2011 Dec;82(6):1496-514. doi: 10.1111/j.1365-2958.2011.07903.x. Epub 2011 Nov 18.

DOI:10.1111/j.1365-2958.2011.07903.x
PMID:22053789
Abstract

Type IVa pili are bacterial nanomachines required for colonization of surfaces, but little is known about the organization of proteins in this system. The Pseudomonas aeruginosa pilMNOPQ operon encodes five key members of the transenvelope complex facilitating pilus function. While PilQ forms the outer membrane secretin pore, the functions of the inner membrane-associated proteins PilM/N/O/P are less well defined. Structural characterization of a stable C-terminal fragment of PilP (PilP(Δ71)) by NMR revealed a modified β-sandwich fold, similar to that of Neisseria meningitidis PilP, although complementation experiments showed that the two proteins are not interchangeable likely due to divergent surface properties. PilP is an inner membrane putative lipoprotein, but mutagenesis of the putative lipobox had no effect on the localization and function of PilP. A larger fragment, PilP(Δ18-6His), co-purified with a PilN(Δ44)/PilO(Δ51) heterodimer as a stable complex that eluted from a size exclusion chromatography column as a single peak with a molecular weight equivalent to two heterotrimers with 1:1:1 stoichiometry. Although PilO forms both homodimers and PilN-PilO heterodimers, PilP(Δ18-6His) did not interact stably with PilO(Δ51) alone. Together these data demonstrate that PilN/PilO/PilP interact directly to form a stable heterotrimeric complex, explaining the dispensability of PilP's lipid anchor for localization and function.

摘要

IVa 型菌毛是细菌表面定植所必需的纳米机器,但人们对该系统中蛋白质的组织知之甚少。铜绿假单胞菌 pilMNOPQ 操纵子编码五个关键的跨膜复合物成员,促进菌毛功能。虽然 PilQ 形成外膜分泌孔,但内膜相关蛋白 PilM/N/O/P 的功能定义较少。通过 NMR 对 PilP 的稳定 C 端片段(PilP(Δ71))进行结构表征,揭示了一种改良的β-三明治折叠,类似于脑膜炎奈瑟菌 PilP,但互补实验表明,这两种蛋白质不能互换,可能是由于表面性质的差异。PilP 是一种内膜假定的脂蛋白,但假定的脂盒突变对 PilP 的定位和功能没有影响。更大的片段 PilP(Δ18-6His)与 PilN(Δ44)/PilO(Δ51)异源二聚体一起共纯化,形成一个稳定的复合物,该复合物在分子筛层析柱上作为一个单一峰洗脱,分子量相当于两个具有 1:1:1 化学计量比的异三聚体。尽管 PilO 形成同源二聚体和 PilN-PilO 异源二聚体,但 PilP(Δ18-6His)不能与单独的 PilO(Δ51)稳定相互作用。这些数据表明,PilN/PilO/PilP 直接相互作用形成一个稳定的异三聚体复合物,解释了 PilP 的脂质锚对于定位和功能的非必需性。

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