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通过氨基酸取代以及用蜡样芽孢杆菌直系同源物替换来调节单核细胞增生李斯特菌广谱磷脂酶C的酶活性和生物学功能。

Modulation of enzymatic activity and biological function of Listeria monocytogenes broad-range phospholipase C by amino acid substitutions and by replacement with the Bacillus cereus ortholog.

作者信息

Zückert W R, Marquis H, Goldfine H

机构信息

Department of Microbiology, University of Pennsylvania School of Medicine, Philadelphia, Pennsylvania 19104, USA.

出版信息

Infect Immun. 1998 Oct;66(10):4823-31. doi: 10.1128/IAI.66.10.4823-4831.1998.

Abstract

The secreted broad-range phosphatidylcholine (PC)-preferring phospholipase C (PC-PLC) of Listeria monocytogenes plays a role in the bacterium's ability to escape from phagosomes and spread from cell to cell. Based on comparisons with two orthologs, Clostridium perfringens alpha-toxin and Bacillus cereus PLC (PLCBc), we generated PC-PLC mutants with altered enzymatic activities and substrate specificities and analyzed them for biological function in tissue culture and mouse models of infection. Two of the conserved active-site zinc-coordinating histidines were confirmed by single amino acid substitutions H69G and H118G, which resulted in proteins inactive in broth culture and unstable intracellularly. Substitutions D4E and H56Y remodeled the PC-PLC active site to more closely resemble the PLCBc active site, while a gene replacement resulted in L. monocytogenes secreting PLCBc. All of these mutants yielded similar amounts of active enzyme as wild-type PC-PLC both in broth culture and intracellularly. D4E increased activity on and specificity for PC, while H56Y and D4E H56Y showed higher activity on both PC and sphingomyelin, with reduced specificity for PC. As expected, PLCBc expressed by L. monocytogenes was highly specific for PC. During early intracellular growth in human epithelial cells, the D4E mutant and the PLCBc-expressing strain performed significantly better than the wild type, while the H56Y and D4E H56Y mutants showed a significant defect. In assays for cell-to-cell spread, the H56Y and D4E mutants had close to wild-type characteristics, while the spreading efficiency of PLCBc was significantly lower. These studies emphasize the species-specific features of PC-PLC important for growth in mammalian cells.

摘要

单核细胞增生李斯特菌分泌的广谱磷脂酰胆碱(PC)偏好性磷脂酶C(PC-PLC)在该细菌逃离吞噬体并在细胞间传播的能力中发挥作用。基于与两种直系同源物——产气荚膜梭菌α毒素和蜡样芽孢杆菌PLC(PLCBc)的比较,我们构建了具有改变的酶活性和底物特异性的PC-PLC突变体,并在组织培养和感染小鼠模型中分析了它们的生物学功能。通过单氨基酸取代H69G和H118G证实了两个保守的活性位点锌配位组氨酸,这导致蛋白质在肉汤培养中无活性且在细胞内不稳定。取代D4E和H56Y重塑了PC-PLC活性位点,使其更类似于PLCBc活性位点,而基因替换导致单核细胞增生李斯特菌分泌PLCBc。所有这些突变体在肉汤培养和细胞内产生的活性酶量与野生型PC-PLC相似。D4E增加了对PC的活性和特异性,而H56Y和D4E H56Y对PC和鞘磷脂均显示出更高的活性,对PC的特异性降低。正如预期的那样,单核细胞增生李斯特菌表达的PLCBc对PC具有高度特异性。在人上皮细胞的早期细胞内生长过程中,D4E突变体和表达PLCBc的菌株表现明显优于野生型,而H56Y和D4E H56Y突变体则表现出明显缺陷。在细胞间传播试验中,H56Y和D4E突变体具有接近野生型的特征,而PLCBc的传播效率则显著较低。这些研究强调了PC-PLC对在哺乳动物细胞中生长重要的物种特异性特征。

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