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F菌毛蛋白作为大肠杆菌K12内膜成分的特性研究。

Characterization of F-pilin as an inner membrane component of Escherichia coli K12.

作者信息

Paiva W D, Grossman T, Silverman P M

机构信息

Program in Molecular and Cell Biology, Oklahoma Medical Research Foundation, Oklahoma City 73104.

出版信息

J Biol Chem. 1992 Dec 25;267(36):26191-7.

PMID:1464628
Abstract

Antipeptide antibodies were used to detect, purify, and characterize nonfilament F-pilin in the cell envelope of an F'tra+ strain of Escherichia coli. Affinity-purified goat antibodies raised against a peptide corresponding to the amino-terminal 14 amino acids of F-pilin detected F-pilin in immuno-overlay ("Western") blots of electrophoretically separated inner and outer membrane proteins. As expected, the molecule was absent from inner membrane preparations of F- or F'traA[Am] strains. Immunoreactive material was purified from inner membrane fractions and shown to be F-pilin by amino acid analysis. The anti-peptide antibodies also detected membrane forms of F-pilin produced by cells containing plasmid pTG801 (Grossman, T. & Silverman, P. (1989) J. Bacteriol. 171, 650-656). Most cell envelope pilin was in the inner membrane fraction, but a significant quantity fractionated with the outer membrane as well. The hydropathy profile of F-pilin suggested that the molecule is an integral membrane protein with two membrane-spanning domains. In confirmation, F-pilin and pTG801 pilins in inner membrane preparations were solubilized by a single extraction with the nonionic detergents Nonidet P-40 (2%) or Triton X-100 (2%), but not by 2 M KCl or 0.1 M NaOH. Moreover, analysis of traA'-'phoA constructs indicated that both the amino and carboxyl termini of F-pilin face the periplasm. The periplasmic location of the amino terminus was confirmed by immunoelectron microscopy of spheroplasts from F' and pTG801 strains, using a monoclonal antibody that recognizes an amino-terminal epitope. These data suggest a specific structure for membrane F-pilin. We discuss that structure in relation to the probable structure of filament F-pilin.

摘要

抗肽抗体被用于检测、纯化和鉴定大肠杆菌F'tra+菌株细胞膜中的非丝状F菌毛蛋白。针对与F菌毛蛋白氨基末端14个氨基酸对应的肽段制备的亲和纯化山羊抗体,在电泳分离的内膜和外膜蛋白的免疫印迹(“Western”印迹)中检测到了F菌毛蛋白。正如预期的那样,在F-或F'traA[Am]菌株的内膜制剂中没有该分子。从内膜组分中纯化出免疫反应性物质,并通过氨基酸分析表明其为F菌毛蛋白。抗肽抗体还检测到含有质粒pTG801的细胞产生的F菌毛蛋白的膜形式(格罗斯曼,T.和西尔弗曼,P.(1989年)《细菌学杂志》171,650 - 656)。大多数细胞膜菌毛蛋白存在于内膜组分中,但也有相当数量的菌毛蛋白与外膜一起分级分离。F菌毛蛋白的亲水性图谱表明该分子是一种具有两个跨膜结构域的整合膜蛋白。经证实,内膜制剂中的F菌毛蛋白和pTG801菌毛蛋白用非离子去污剂Nonidet P - 40(2%)或Triton X - 100(2%)单次提取即可溶解,但用2 M KCl或0.1 M NaOH则不能溶解。此外,对traA'-'phoA构建体的分析表明,F菌毛蛋白的氨基末端和羧基末端都面向周质空间。使用识别氨基末端表位的单克隆抗体,通过对F'和pTG801菌株原生质球的免疫电子显微镜观察,证实了氨基末端位于周质空间。这些数据表明了膜F菌毛蛋白的特定结构。我们讨论了该结构与丝状F菌毛蛋白可能结构的关系。

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