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金黄色葡萄球菌N端截短重组β-溶血素的制备与应用

Production and applications of an N-terminally-truncated recombinant beta-haemolysin from Staphylococcus aureus.

作者信息

Singh M, Singh A, Sharma A

机构信息

ICAR Centre of Advanced Faculty Training, Department of Veterinary Microbiology, Lala Lajpat Rai University of Veterinary & Animal Sciences, Hisar, 125004 Haryana, India.

出版信息

Biologicals. 2014 Jul;42(4):191-8. doi: 10.1016/j.biologicals.2014.05.003. Epub 2014 Jun 16.

DOI:10.1016/j.biologicals.2014.05.003
PMID:24948115
Abstract

The beta-haemolysin of Staphylococcus aureus (SA-hlb) is a secreted neutral sphingomyelinase (nSMase) implicated in the pathogenesis of infection and responsible for the characteristic in vitro 'hot-cold' haemolytic ability of the bacterium. Here, we describe the production of a biologically active N-terminally-truncated recombinant SA-hlb protein for use in in vitro assays and as a research tool. Using local isolates of S. aureus, we PCR-amplified an SA-hlb DNA sequence of 891 nucleotides, 99 nucleotides shorter than the full-length molecule, before cloning and sequencing (GenBank accession no. JN580071). The pQE.TriSystem vector (Qiagen, Germany) was used to express recombinant SA-hlb (r-SA-hlb) with a C-terminal 8xHis tag in Escherichia coli JM107 cells. Both JM107 lysate and the purified r-SA-hlb possessed hot-cold lytic activity against sheep and buffalo erythrocytes, which was abolished by incubation at ≥90 °C for 30 min or exposure to dithiothreitol, and could be neutralized by bovine immune sera. Purified r-SA-hlb was also cytotoxic to buffalo mononuclear cells and was effective as a coating antigen for indirect ELISA to screen for reactive sera. Importantly, the r-SA-hlb was suitable for use as a β-toxin in the modified CAMP test. We conclude that the r-SA-hlb protein produced was functionally active and has numerous potential applications.

摘要

金黄色葡萄球菌的β-溶血素(SA-hlb)是一种分泌型中性鞘磷脂酶(nSMase),与感染的发病机制有关,并且是该细菌在体外具有特征性“热-冷”溶血能力的原因。在此,我们描述了一种具有生物活性的N端截短重组SA-hlb蛋白的产生,用于体外试验并作为一种研究工具。利用金黄色葡萄球菌的本地分离株,我们通过PCR扩增了一个891个核苷酸的SA-hlb DNA序列,比全长分子短99个核苷酸,然后进行克隆和测序(GenBank登录号:JN580071)。使用pQE.TriSystem载体(德国Qiagen公司)在大肠杆菌JM107细胞中表达带有C端8xHis标签的重组SA-hlb(r-SA-hlb)。JM107裂解物和纯化的r-SA-hlb对绵羊和水牛红细胞均具有热-冷裂解活性,在≥90°C孵育30分钟或暴露于二硫苏糖醇后该活性被消除,并且可以被牛免疫血清中和。纯化的r-SA-hlb对水牛单核细胞也具有细胞毒性,并且作为间接ELISA的包被抗原用于筛选反应性血清时效果良好。重要的是,r-SA-hlb适用于改良CAMP试验中的β毒素。我们得出结论,所产生的r-SA-hlb蛋白具有功能活性并且有许多潜在应用。

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