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鉴定志贺氏菌属多肽聚糖去乙酰化酶 SfPgdA,该酶是志贺氏菌属在多形核中性粒细胞内持续存在所必需的。

Characterization of SfPgdA, a Shigella flexneri peptidoglycan deacetylase required for bacterial persistence within polymorphonuclear neutrophils.

机构信息

Laboratoire de Bactériologie Moléculaire, Faculté de Médecine, Université Libre de Bruxelles, Route de Lennik 808, 1070 Bruxelles, Belgium.

出版信息

Microbes Infect. 2012 Jul;14(7-8):619-27. doi: 10.1016/j.micinf.2012.01.009. Epub 2012 Jan 23.

DOI:10.1016/j.micinf.2012.01.009
PMID:22307019
Abstract

Peptidoglycan deacetylases protect the Gram-positive bacteria cell wall from host lysozymes by deacetylating peptidoglycan. Sequence analysis of the genome of Shigella flexneri predicts a putative polysaccharide deacetylase encoded by the plasmidic gene orf185, renamed here SfpgdA. We demonstrated a peptidoglycan deacetylase (PGD) activity with the purified SfPgdA in vitro. To investigate the role SfPgdA in virulence, we constructed a SfpgdA mutant and studied its phenotype in vitro. The mutant showed an increased sensitivity to lysozyme compared to the parental strain. Moreover, the mutant was rapidly killed by polymorphonuclear neutrophils (PMNs). Specific substitution of histidines residues 120 and 125, located within the PGD catalytic domain, by phenylalanine abolished SfPgdA function. SfPgdA expression is controlled by PhoP. Mutation of phoP increases sensitivity to lysozyme compared to the SfpgdA mutant. Here, we confirmed that SfPgdA expression is enhanced under low magnesium concentration and not produced by the phoP mutant. Ectopic expression of SfPgdA in the phoP mutant restored lysozyme resistance and parental bacterial persistence within PMNs. Together our results indicate that PG deacetylation mechanism likely contributes to Shigella persistence by subverting detection by the host immune system.

摘要

肽聚糖脱乙酰基酶通过脱乙酰化肽聚糖来保护革兰氏阳性细菌细胞壁免受宿主溶菌酶的侵害。对福氏志贺菌基因组的序列分析预测了一种由质粒基因 orf185 编码的假定多糖脱乙酰酶,我们将其重新命名为 SfpgdA。我们在体外纯化的 SfPgdA 中证明了一种肽聚糖脱乙酰酶 (PGD) 活性。为了研究 SfPgdA 在毒力中的作用,我们构建了 SfpgdA 突变体,并在体外研究了其表型。与亲本菌株相比,突变体对溶菌酶的敏感性增加。此外,突变体被多形核粒细胞 (PMN) 迅速杀死。位于 PGD 催化结构域内的组氨酸残基 120 和 125 的特异性取代为苯丙氨酸,使 SfPgdA 功能丧失。SfPgdA 的表达受 PhoP 控制。与 SfpgdA 突变体相比, phoP 突变增加了对溶菌酶的敏感性。在这里,我们证实 SfPgdA 的表达在低镁浓度下增强,并且不是由 phoP 突变体产生的。在 phoP 突变体中异位表达 SfPgdA 恢复了溶菌酶抗性和亲本细菌在 PMN 中的持续存在。我们的研究结果表明,PG 脱乙酰化机制可能通过改变宿主免疫系统的检测来促进志贺氏菌的持续存在。

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