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lambda S 的 N 端跨膜结构域对于溶菌素但不是抗溶菌素功能是必需的。

The N-terminal transmembrane domain of lambda S is required for holin but not antiholin function.

机构信息

Department of Biochemistry and Biophysics, Texas A&M University, 2128 TAMU, College Station, TX 77843-2128, USA.

出版信息

J Bacteriol. 2010 Feb;192(3):725-33. doi: 10.1128/JB.01263-09. Epub 2009 Nov 6.

DOI:10.1128/JB.01263-09
PMID:19897658
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2812449/
Abstract

The lambda S gene encodes a holin, S105, and an antiholin, S107, which differs by its Met-Lys N-terminal extension. The model for the lysis-defective character of S107 stipulates that the additional N-terminal basic residue keeps S107 from assuming the topology of S105, which is N-out, C-in, with three transmembrane domains (TMDs). Here we show that the N terminus of S105 retains its fMet residue but that the N terminus of S107 is fully deformylated. This supports the model that in S105, TMD1 inserts into the membrane very rapidly but that in S107, it is retained in the cytoplasm. Further, it reveals that, compared to S105, S107 has two extra positively charged moieties, Lys2 and the free N-terminal amino group, to hinder its penetration into an energized membrane. Moreover, an allele, S105(DeltaTMD1), with TMD1 deleted, was found to be defective in lysis, insensitive to membrane depolarization, and dominant to the wild-type allele, indicating that the lysis-defective, antiholin character of S107 is due to the absence of TMD1 from the bilayer rather than to its ectopic localization at the inner face of the cytoplasmic membrane. Finally, the antiholin function of the deletion protein was compromised by the substitution of early-lysis missense mutations in either the deletion protein or parental S105 but restored when both S105(DeltaTMD1) and holin carried the substitution.

摘要

Lambda S 基因编码一个溶菌素(holin)S105 和一个抗溶菌素(antiholin)S107,后者的 N 端延伸由 Met-Lys 组成。关于 S107 裂解缺陷特征的模型规定,额外的 N 端碱性残基阻止 S107 呈现 N 出 C 入拓扑结构,具有三个跨膜结构域(TMDs)。本文表明 S105 的 N 端保留其 fMet 残基,但 S107 的 N 端完全去甲酰化。这支持了这样的模型,即在 S105 中,TMD1 非常迅速地插入膜中,但在 S107 中,它被保留在细胞质中。此外,它表明与 S105 相比,S107 具有两个额外的带正电荷的部分,Lys2 和游离的 N 端氨基,以阻碍其穿透能量化的膜。此外,发现一个等位基因 S105(DeltaTMD1)缺失了 TMD1,其裂解缺陷,对膜去极化不敏感,并且对野生型等位基因具有显性,表明 S107 的裂解缺陷抗溶菌素特征是由于 TMD1 从双层中缺失,而不是其异位定位于细胞质膜的内表面。最后,缺失蛋白的抗溶菌素功能因缺失蛋白或亲本 S105 中的早期裂解错义突变的取代而受损,但当 S105(DeltaTMD1)和 holin 都携带取代时,其功能得到恢复。

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