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基于胆碱结合蛋白的抗肺炎链球菌疫苗制剂的评估

Evaluation of a vaccine formulation against Streptococcus pneumoniae based on choline-binding proteins.

作者信息

Miyaji Eliane N, Vadesilho Cintia F M, Oliveira Maria Leonor S, Zelanis André, Briles David E, Ho Paulo L

机构信息

Centro de Biotecnologia, Instituto Butantan, São Paulo, SP, Brazil

Centro de Biotecnologia, Instituto Butantan, São Paulo, SP, Brazil.

出版信息

Clin Vaccine Immunol. 2015 Feb;22(2):213-20. doi: 10.1128/CVI.00692-14. Epub 2014 Dec 17.

DOI:10.1128/CVI.00692-14
PMID:25520146
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4308862/
Abstract

Streptococcus pneumoniae has proteins that are attached to its surface by binding to phosphorylcholine of teichoic and lipoteichoic acids. These proteins are known as choline-binding proteins (CBPs). CBPs are an interesting alternative for the development of a cost-effective vaccine, and PspA (pneumococcal surface protein A) is believed to be the most important protective component among the different CBPs. We sought to use CBPs eluted from pneumococci as an experimental vaccine. Since PspA shows variability between isolates, we constructed strains producing different PspAs. We used the nonencapsulated Rx1 strain, which produces PspA from clade 2 (PspA2), to generate a pspA-knockout strain (Rx1 ΔpspA) and strains expressing PspA from clade 1 (Rx1 pspA1) and clade 4 (Rx1 pspA4). We grew Rx1, Rx1 ΔpspA, Rx1 pspA1, and Rx1 pspA4 in Todd-Hewitt medium containing 0.5% yeast extract and washed cells in 2% choline chloride (CC). SDS-PAGE analysis of the proteins recovered by a CC wash showed few bands, and the CBPs PspA and PspC (pneumococcal surface protein C) were identified by mass spectrometry analysis. Subcutaneous immunization of mice with these full-length native proteins without adjuvant led to significantly higher rates of survival than immunization with diluent after an intranasal lethal challenge with two pneumococcal strains and also after a colonization challenge with one strain. Importantly, immunization with recombinant PspA4 (rPspA4) without adjuvant did not elicit significant protection.

摘要

肺炎链球菌具有通过与磷壁酸和脂磷壁酸的磷酰胆碱结合而附着于其表面的蛋白质。这些蛋白质被称为胆碱结合蛋白(CBPs)。CBPs是开发具有成本效益疫苗的一个有趣选择,并且肺炎球菌表面蛋白A(PspA)被认为是不同CBPs中最重要的保护性成分。我们试图使用从肺炎球菌中洗脱的CBPs作为实验性疫苗。由于PspA在分离株之间表现出变异性,我们构建了产生不同PspA的菌株。我们使用了不产荚膜的Rx1菌株,其产生来自进化枝2的PspA(PspA2),以生成pspA基因敲除菌株(Rx1 ΔpspA)以及表达来自进化枝1(Rx1 pspA1)和进化枝4(Rx1 pspA4)的PspA的菌株。我们在含有0.5%酵母提取物的托德-休伊特培养基中培养Rx1、Rx1 ΔpspA、Rx1 pspA1和Rx1 pspA4,并在2%氯化胆碱(CC)中洗涤细胞。对通过CC洗涤回收的蛋白质进行SDS-PAGE分析显示条带很少,并且通过质谱分析鉴定出了CBPs PspA和肺炎球菌表面蛋白C(PspC)。用这些无佐剂的全长天然蛋白对小鼠进行皮下免疫,在经两种肺炎球菌菌株鼻内致死攻击以及经一种菌株进行定植攻击后,导致的存活率显著高于用稀释剂免疫。重要的是,用无佐剂的重组PspA4(rPspA4)免疫未引发显著的保护作用。

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