Preparation of monoclonal antibody and identification of two novel B cell epitopes to VP1 protein of porcine sapelovirus

表位 单克隆抗体 免疫原性 生物 重组DNA 同型 病毒学 抗体 血清学 抗原 融合蛋白 表位定位 线性表位 分子生物学 免疫学 基因 遗传学
作者
Chenlin Hao,Haojie Ren,Xingyi Wu,Xiangli Shu,Zhaoyang Li,Yating Hu,Quan Zeng,Yucan Zhang,Shaopo Zu,Jin Yuan,Honglei Zhang,Hui Hu
出处
期刊:Veterinary Microbiology [Elsevier]
卷期号:275: 109593-109593 被引量:2
标识
DOI:10.1016/j.vetmic.2022.109593
摘要

Porcine sapelovirus (PSV) is an important emerging swine pathogen that causes diarrhoea, respiratory distress, severe reproductive system and neurological disorders in pigs, posing huge threat to swine industry. However, there are no effective serological diagnostic products and the epitope characterization of PSV VP1 protein is still largely unknown. In current study, we successfully expressed recombinant His-VP1 protein by prokaryotic expression system and the recombinant VP1 protein had good immunogenicity. BALB/C mice were then selected and immunized with purified recombinant VP1 protein, and two monoclonal antibodies (Mabs) 9F10 and 15E4 against VP1 were successfully prepared by hybrioma technology. The isotype of these two Mabs were identified and showed that Mab 9F10 with the heavy chain subtype was IgG1 and the light chain subtype was kappa. Mab 15E4 was identified as IgG2 for the heavy chain subtype and Kappa for the light chain subtype. The antigen epitopes of prepared two VP1 Mabs were clearly identified. The minimal unit of B cell specific epitope recognized by Mab 15E4 was 203YDGDG207 and conserved in different strain genotypes of PSV, indicating this epitope may be a good target for serological detection of PSV. However, the epitope recognized by Mab 9F10 was 8QAIVNRT14 and varied greatly among different PSV strains. Structural modeling analysis showed that the identified two novel B cell epitopes were located on the surface of VP1. Our study provides useful tool for the establishment the serological detection methods of PSV and may support the study of VP1 protein function.
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