基础医学与临床 ›› 2022, Vol. 42 ›› Issue (12): 1885-1890.doi: 10.16352/j.issn.1001-6325.2022.12.1885

• 研究论文 • 上一篇    下一篇

H1N1流感病毒HA蛋白疫苗构建策略的筛选

郑宁晨, 杨姣姣, 张婷, 王志荣, 许雪梅*   

  1. 中国医学科学院基础医学研究所 北京协和医学院基础学院 生物物理及结构生物学系,北京 100005
  • 收稿日期:2022-07-18 修回日期:2022-09-26 出版日期:2022-12-05 发布日期:2022-11-23
  • 通讯作者: * xuemeixu@vip.sina.cn
  • 基金资助:
    中国医学科学院医学与健康科技创新工程(2021-I2M-1-043); 国家自然科学基金(31970867)

Screening of strategies for HA protein vaccine for influenza virus H1N1

ZHENG Ning-chen, YANG Jiao-jiao, ZHANG Ting, WANG Zhi-rong, XU Xue-mei*   

  1. Department of Biophysics and Structure Biology,Institute of Basic Medical Sciences CAMS,School of Basic Medicine PUMC, Beijing 100005,China
  • Received:2022-07-18 Revised:2022-09-26 Online:2022-12-05 Published:2022-11-23
  • Contact: * xuemeixu@vip.sina.cn

摘要: 目的 筛选并确立流感病毒H1N1 A/Nebraska/14/2019 血凝素(HA)的最佳蛋白疫苗策略。方法 分别构建HA全长、HA胞外区C端不同的突变体及共表达HA/M1的重组杆状病毒,感染昆虫细胞表达80 h后,收取培养上清,Western blot鉴定重组抗原的表达,同时采用血凝试验间接分析其免疫原性。然后大量表达HA/M1蛋白,Core700纯化后分析蛋白颗粒的理化性质、血凝活性及稳定性。结果 2种HA胞外区的C端突变体虽均以三聚体形式表达,但表达上清无血凝活性;HA全长三聚体具有较好的血凝活性,但为膜蛋白,纯化难度大。HA/M1共表达上清具有血凝活性,HA/M1表达上清经Core700纯化,透射电子显微镜分析显示为80 nm~150 nm病毒样颗粒(VLP)。HA-M1-VLP的血凝效价高达26,动态光散射显示HA-M1-VLP在4 ℃保存3个月性质稳定。结论 HA-M1-VLP易于表达纯化、稳定性好,且血凝活性高,可用于流感病毒H1N1蛋白疫苗的研究。

关键词: H1N1, 血凝素(HA), 基质蛋白(M1), 病毒样颗粒(VLP)

Abstract: Objective To screen and establish the optimal expression strategy of influenza virus H1N1 A/Nebraska/14/2019 HA, and lay a foundation for the development of protein vaccines. Methods The recombinant baculovirus of HA full-length, different C-terminal mutants of the extra cellular regions and co-expressing HA/M1 were constructed respectively. After 80 hours of infection in insect cells, the culture supernatant was collected, and the expression of recombinant antigen was identified by Western blot. Hemagglutination test indirectly analyzes its immunogenic. Then, HA/M1 protein was expressed in large quantities, and the physicochemical properties, hemagglutination activity and stability were analyzed after Core700 purification. Results The two C-terminal mutants of the extra cellular region of HA were all expressed in the form of trimers, but the expression supernatants had no hemagglutination activity; the full-length HA trimers had good hemagglutination activity, but they were membrane proteins thus were difficult to be purified. M1/HA co-expression supernatant also had hemagglutination activity. Electron microscopy of expression product purified by Core700 showed virus-like particles (VLPs) of 80 nm~150 nm. The hemagglutination titer of HA-M1-VLP reached 26 and was stable for three months at 4 ℃ as shown by light scattering. Conclusions HA-M1-VLP is easy to express and to be purified. The product has good stability, and hemagglutination activity, so can be used for the research of influenza virus protein vaccine.

Key words: H1N1, hemagglutinin (HA), matrix protein(M1), virus-like particle (VLP)

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