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IncP菌毛蛋白前体的成熟类似于前导肽酶的催化二元样机制。

Maturation of IncP pilin precursors resembles the catalytic Dyad-like mechanism of leader peptidases.

作者信息

Eisenbrandt R, Kalkum M, Lurz R, Lanka E

机构信息

Max-Planck-Institut für Molekulare Genetik, Dahlem, D-14195 Berlin, Germany.

出版信息

J Bacteriol. 2000 Dec;182(23):6751-61. doi: 10.1128/JB.182.23.6751-6761.2000.

Abstract

The pilus subunit, the pilin, of conjugative IncP pili is encoded by the trbC gene. IncP pilin is composed of 78 amino acids forming a ring structure (R. Eisenbrandt, M. Kalkum, E.-M. Lai, C. I. Kado, and E. Lanka, J. Biol. Chem. 274:22548-22555, 1999). Three enzymes are involved in maturation of the pilin: LepB of Escherichia coli for signal peptide removal and a yet-unidentified protease for removal of 27 C-terminal residues. Both enzymes are chromosome encoded. Finally, the inner membrane-associated IncP TraF replaces a four-amino-acid C-terminal peptide with the truncated N terminus, yielding the cyclic polypeptide. We refer to the latter process as "prepilin cyclization." We have used site-directed mutagenesis of trbC and traF to unravel the pilin maturation process. Each of the mutants was analyzed for its phenotypes of prepilin cyclization, pilus formation, donor-specific phage adsorption, and conjugative DNA transfer abilities. Effective prepilin cyclization was determined by matrix-assisted laser desorption-ionization-mass spectrometry using an optimized sample preparation technique of whole cells and trans-3-indolyl acrylic acid as a matrix. We found that several amino acid exchanges in the TrbC core sequence allow prepilin cyclization but disable the succeeding pilus assembly. We propose a mechanism explaining how the signal peptidase homologue TraF attacks a C-terminal section of the TrbC core sequence via an activated serine residue. Rather than cleaving and releasing hydrolyzed peptides, TraF presumably reacts as a peptidyl transferase, involving the N terminus of TrbC in the aminolysis of a postulated TraF-acetyl-TrbC intermediate. Under formal loss of a C-terminal tetrapeptide, a new peptide bond is formed in a concerted action, connecting serine 37 with glycine 114 of TrbC.

摘要

接合型 IncP 菌毛的菌毛亚基菌毛蛋白由 trbC 基因编码。IncP 菌毛蛋白由 78 个氨基酸组成,形成一个环状结构(R. 艾森布兰特、M. 卡尔库姆、E.-M. 赖、C. I. 卡多和 E. 兰卡,《生物化学杂志》274:22548 - 22555,1999 年)。有三种酶参与菌毛蛋白的成熟过程:大肠杆菌的 LepB 用于去除信号肽,还有一种尚未鉴定的蛋白酶用于去除 27 个 C 末端残基。这两种酶都是由染色体编码的。最后,与内膜相关的 IncP TraF 用截短的 N 末端取代了一个四氨基酸的 C 末端肽,产生环状多肽。我们将后一过程称为“前菌毛蛋白环化”。我们利用 trbC 和 traF 的定点诱变来阐明菌毛蛋白的成熟过程。对每个突变体进行了前菌毛蛋白环化、菌毛形成、供体特异性噬菌体吸附和接合性 DNA 转移能力的表型分析。使用全细胞优化样品制备技术并以反式 -3 - 吲哚基丙烯酸作为基质,通过基质辅助激光解吸 - 电离 - 质谱法确定有效的前菌毛蛋白环化。我们发现 TrbC 核心序列中的几个氨基酸交换允许前菌毛蛋白环化,但会使后续的菌毛组装失效。我们提出了一种机制,解释信号肽酶同源物 TraF 如何通过活化的丝氨酸残基攻击 TrbC 核心序列的 C 末端部分。TraF 大概不是切割并释放水解肽,而是作为肽基转移酶起作用,在假定的 TraF - 乙酰 - TrbC 中间体的氨解过程中涉及 TrbC 的 N 末端。在 C 末端四肽正式缺失的情况下,在协同作用中形成一个新的肽键,将 TrbC 的丝氨酸 37 与甘氨酸 114 连接起来。

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