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Engineering His-Tagged Senecavirus A for One-Step Purification of Viral Antigens.Vaccines (Basel).2022 Jan 22;10(2):170.doi: 10.3390/vaccines10020170

Junhao Fan,Peiyu Xiao,Dongni Kong,Xinran Liu,Liang Meng,Tongqing An,Xuehui Cai,Haiwei Wang,Li Yu


Vaccines (Basel).2022 Jan 22;10(2):170.doi: 10.3390/vaccines10020170.


Abstract

Senecavirus A (SVA) is a picornavirus that causes vesicular disease in swine, and the inactivated vaccine is used to prevent and control SVA infection. To develop a new chromatography strategy for the purification and concentration of SVA vaccine antigens, we inserted a 6×His-tag at the VP1 C-terminal of the SVA/HLJ/CHA/2016 in an infectious clone to rescue a His-tagged SVA. The constructed and rescued recombinant virus, named as rSVA-His, exhibited similar growth kinetics to that of its parental virus. In addition, the expression of a 6×His-tag on the surface of SVA showed genetic stability in cell passages in vitro, which allowed one-step purification of SVA antigens by Ni2+ affinity columns. Furthermore, the immunogenicity of the inactivated rSVA-His was evaluated by inoculating rabbits and detecting neutralizing antibodies. The animals receiving two doses of the inactivated rSVA-His emulsified with oil adjuvant developed a high titer of neutralizing antibodies, indicating that SVA VP1 is tolerant to His-tag insertion without detriment to its antigenicity. In summary, the constructed 6×His-tagged SVA may offer a feasible approach to the affinity purification and concentration of antigens in the process of SVA inactivated vaccine production.


Keywords: His-tagged virus; Senecavirus A; antigen purification.


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