Epitope delimitation: A new method for defining epitopes of human IgG‐reactive antigenic peptides based on rabbit‐recognized epitope motifs

Author:

Tang Hai‐Ping1,He Ya‐Ping1ORCID,Wang Jian1,Zhan Jian‐Min1,Lian Wen‐Bo1,Xue Feng2,Wang Li2,Li Yijie3,Zhang Ailian3,Zhang Fuchun3,Xu Chen2,Li Jinyao3,Xu Wan‐Xiang1

Affiliation:

1. NHC Key Lab of Reproduction Regulation, Shanghai Engineering Research Center of Reproductive Health Drug and Devices Shanghai Institute for Biomedical and Pharmaceutical Technologies Shanghai China

2. Department of Histo‐Embryology Genetics and Developmental Biology Shanghai Jiao Tong University School of Medicine Shanghai China

3. Xinjiang Key Laboratory of Biological Resources and Genetic Engineering, College of Life Science and Technology Xinjiang University Urumqi China

Abstract

AbstractThe use of precise epitope peptides as antigens is essential for accurate serological diagnosis of viral‐infected individuals, but now it remains an unsolvable problem for mapping precise B cell epitopes (BCEs) recognized by human serum. To address this challenge, we propose a novel epitope delimitation (ED) method to uncover BCEs in the delineated human IgG‐reactive (HR) antigenic peptides (APs). Specifically, the method based on the rationale of similarities in humoral immune responses between mammalian species consists of a pair of elements: experimentally delineated HR‐AP and rabbit‐recognized (RR) BCE motif and corresponding pair of sequence alignment analysis. As a result of using the ED approach, after decoding four RR‐epitomes of human papillomavirus types 16/18‐E6 and E7 proteins utilizing rabbit serum against each recombinant protein and sequence alignment analysis of HR‐APs and RR‐BCEs, 19 fine BCEs in 17 of 22 known HR‐APs were defined based on each corresponding RR‐BCE motifs, including the type‐specificity of each delimited BCE in homologous proteins. The test with 22 known 16/20mer HR‐APs demonstrated that the ED method is effective and efficient, indicating that it can be used as an alternative method to the conventional identification of fine BCEs using overlapping 8mer peptides.

Publisher

Wiley

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