1. Identification of a novel B-cell epitope in the spike protein of porcine epidemic diarrhea virus
- Author
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Hua Wang, Dage Sun, Hao Zheng, Yongguang Wu, Qiong Meng, Yewen Zuo, Ning Kong, Hai Yu, Yongjie Xu, Guangzhi Tong, Tongling Shan, Wu Tong, Sujie Dong, Yajuan Jiao, and Huanjie Zhai
- Subjects
0301 basic medicine ,Monoclonal antibody ,040301 veterinary sciences ,medicine.drug_class ,Spike protein ,Epitope ,PEDV ,lcsh:Infectious and parasitic diseases ,0403 veterinary science ,Mice ,03 medical and health sciences ,Virology ,Chlorocebus aethiops ,medicine ,Animals ,lcsh:RC109-216 ,Vero Cells ,Antiserum ,Mice, Inbred BALB C ,biology ,Linear epitope ,Immunodominant Epitopes ,Research ,Porcine epidemic diarrhea virus ,Antibodies, Monoclonal ,04 agricultural and veterinary sciences ,biology.organism_classification ,Antibodies, Neutralizing ,030104 developmental biology ,Infectious Diseases ,Pepscan ,Polyclonal antibodies ,Spike Glycoprotein, Coronavirus ,biology.protein ,Epitopes, B-Lymphocyte ,Female ,Antibody - Abstract
Background Porcine epidemic diarrhea virus (PEDV) infection causes an acute enteric tract infectious disease characterized by vomiting, anorexia, dehydration, weight loss and high mortality in neonatal piglets. During PEDV infection, the spike protein (S) is a major virion structural protein interacting with receptors and inducing neutralizing antibodies. However, the neutralizing B-cell epitopes within PEDV S protein have not been well studied. Methods To accurately identify the important immunodominant region of S1, the purified truncated S1 proteins (SA, SB, SC, SD and SE) were used to immunize BALB/c mice to prepare polyclonal antibodies. The antisera titers were determined by indirect ELISA, western blot and IFA after four immunizations to find the important immunodominant region of S1, and then purified the immunodominant region of S1 protein and immunized mice to generate the special antibodies, and then used recombinant peptides to determine the B-cell epitopes of monoclonal antibodies. Results Five antisera of recombinant proteins of the spike protein region of PEDV were generated and we found that only the polyclonal antibody against part of the S1 region (signed as SE protein, residues 666–789) could recognize the native PEDV. Purified SE protein was used to immunize BALB/c mice and generate mAb 2E10. Pepscan of the SE protein demonstrated that SE16 (722SSTFNSTREL731) is the minimal linear epitope required for reactivity with the mAb 2E10. Further investigation indicated that the epitope SE16 was localized on the surface of PEDV S protein in the 3D structure. Conclusions A mAb 2E10 that is specifically bound to PEDV was generated and identified a specific linear B-cell epitope (SE16, 722SSTFNSTREL731) of the mAb. The epitope region of PEDV S1 localized in the different regions in comparison with the earlier identified epitopes. These findings enhance the understanding of the PEDV spike protein structure for vaccine design and provide a potential use for developing diagnostic methods to detect PEDV.
- Published
- 2020