严重急性呼吸综合征相关冠状病毒截短的刺突-核衣壳融合蛋白的表达及抗原性

The expression and antigenicity of a truncated spike-nucleocapsid fusion protein of severe acute respiratory syndrome-associated coronavirus.

作者信息

Mu Feng, Niu Dongsheng, Mu Jingsong, He Bo, Han Weiguo, Fan Baoxing, Huang Shengyong, Qiu Yan, You Bo, Chen Weijun

机构信息

Beijing Institute of Genomics, Chinese Academy of Sciences, Beijing, PR China.

出版信息

BMC Microbiol. 2008 Nov 28;8:207. doi: 10.1186/1471-2180-8-207.

DOI:10.1186/1471-2180-8-207

PMID:19038059

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2613400/

Abstract

BACKGROUND

In the absence of effective drugs, controlling SARS relies on the rapid identification of cases and appropriate management of the close contacts, or effective vaccines for SARS. Therefore, developing specific and sensitive laboratory tests for SARS as well as effective vaccines are necessary for national authorities.

RESULTS

Genes encoding truncated nucleocapsid (N) and spike (S) proteins of SARSCoV were cloned into the expression vector pQE30 and fusionally expressed in Escherichia coli M15. The fusion protein was analyzed for reactivity with SARS patients' sera and with anti-sera against the two human coronaviruses HCoV 229E and HCoV OC43 by ELISA, IFA and immunoblot assays. Furthermore, to evaluate the antigen-specific humoral antibody and T-cell responses in mice, the fusion protein was injected into 6-week-old BALB/c mice and a neutralization test as well as a T-cell analysis was performed. To evaluate the antiviral efficacy of immunization, BALB/c mice were challenged intranasally with SARSCoV at day 33 post injection and viral loads were determined by fluorescent quantitative RT-PCR. Serological results showed that the diagnostic sensitivity and specificity of the truncated S-N fusion protein derived the SARS virus were > 99% (457/460) and 100.00% (650/650), respectively. Furthermore there was no cross-reactivity with other two human coronaviruses. High titers of antibodies to SRASCoV appeared in the immunized mice and the neutralization test showed that antibodies to the fusion protein could inhibit SARSCoV. The T cell proliferation showed that the fusion protein could induce an antigen-specific T-cell response. Fluorescent quantitative RT-PCR showed that BALB/c mice challenged intranasally with SARSCoV at day 33 post injection were completely protected from virus replication.

CONCLUSION

The truncated S-N fusion protein is a suitable immunodiagnostic antigen and vaccine candidate.

摘要

背景

在缺乏有效药物的情况下，控制严重急性呼吸综合征（SARS）依赖于快速识别病例并对密切接触者进行适当管理，或依赖于有效的SARS疫苗。因此，开发针对SARS的特异性和敏感性实验室检测方法以及有效的疫苗对国家当局来说是必要的。

结果

将编码SARS冠状病毒截短核衣壳（N）蛋白和刺突（S）蛋白的基因克隆到表达载体pQE30中，并在大肠杆菌M15中融合表达。通过酶联免疫吸附测定（ELISA）、间接免疫荧光法（IFA）和免疫印迹分析，分析融合蛋白与SARS患者血清以及针对两种人类冠状病毒HCoV-229E和HCoV-OC43的抗血清的反应性。此外，为了评估小鼠体内抗原特异性体液抗体和T细胞反应，将融合蛋白注射到6周龄的BALB/c小鼠体内，并进行中和试验以及T细胞分析。为了评估免疫的抗病毒效果，在注射后第33天对BALB/c小鼠进行鼻内SARS冠状病毒攻击，并通过荧光定量逆转录聚合酶链反应（RT-PCR）测定病毒载量。血清学结果表明，源自SARS病毒的截短S-N融合蛋白的诊断敏感性和特异性分别>99%（457/460）和100.00%（650/650）。此外，与其他两种人类冠状病毒无交叉反应。免疫小鼠体内出现了高滴度的抗SARS冠状病毒抗体，中和试验表明融合蛋白抗体可抑制SARS冠状病毒。T细胞增殖表明融合蛋白可诱导抗原特异性T细胞反应。荧光定量RT-PCR表明第33天鼻内接种SARS冠状病毒的BALB/c小鼠完全受到保护，免受病毒复制。