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猪圆环病毒 3 衣壳蛋白线性 B 细胞表位的精细定位。

Fine mapping of linear B cell epitopes on capsid protein of porcine circovirus 3.

机构信息

School of Life Sciences, Zhengzhou University, Zhengzhou, 450001, China.

Key Laboratory of Animal Immunology, Henan Academy of Agricultural Sciences, Zhengzhou, 450002, China.

出版信息

Appl Microbiol Biotechnol. 2020 Jul;104(14):6223-6234. doi: 10.1007/s00253-020-10664-2. Epub 2020 May 22.

DOI:10.1007/s00253-020-10664-2
PMID:32445000
Abstract

Porcine circovirus type 3 (PCV3) is an emerging swine pathogen associated with acute porcine dermatitis and nephropathy syndrome (PDNS)-like clinical signs, reproductive failure, and multisystemic inflammation. Current evidence shows that PCV3 is spread worldwide, and its high incidence may pose a threat to the global pig industry. Capsid (Cap) protein is the sole structural protein which plays an important role in inducing protective immunity against PCV3 infection. In this study, monoclonal antibodies (mAbs) against Cap protein of PCV3 were produced by the hybridoma technique. Subsequently, 12 serial overlapping peptides (P1 to P12) spanning the entire region of Cap were synthesized to determine the B cell epitope regions using the mAbs. Results from dot-blot and peptide ELISA identified that P3, P9, and P10 were the major B cell antigenic regions. Fine mapping by shorter N- and C-terminal truncated peptides confirmed that the motifs NKPWH, KHSRYFT, and QSLFFF were linear B cell epitopes, which were highly conserved among different PCV3 strains. Interestingly, we found that the motif KHSRYFT was highly conserved in all reported types of PCVs (i.e., PCV1, PCV2, PCV3, and PCV4), except for the substitution (Y → K → R) of the first residue. This is the first research to identify B cell epitopes of PCV3 Cap, and these findings may lead to a better understanding of the antibody-antigen interaction and provide some guidance for PCV3 vaccine design.Key points• The recombinant Cap protein of PCV3 was expressed and purified in soluble form. • PCV3 Cap-specific mAbs prepared in this study had no cross-reactivity with PCV1/PCV2 Cap. • This is the first report of three conserved linear B cell epitopes on PCV3 Cap. • The minimal residues of the epitopes were 57-61 aa, 140-146 aa, and 161-166 aa.

摘要

猪圆环病毒 3 型(PCV3)是一种新兴的猪病原体,与急性猪皮炎和肾病综合征(PDNS)样临床症状、繁殖失败和多系统炎症有关。目前的证据表明,PCV3 在全球范围内传播,其高发病率可能对全球养猪业构成威胁。衣壳(Cap)蛋白是唯一的结构蛋白,在诱导对 PCV3 感染的保护性免疫中起着重要作用。在本研究中,采用杂交瘤技术制备了针对 PCV3 Cap 蛋白的单克隆抗体(mAbs)。随后,合成了 12 个连续重叠肽(P1 至 P12),跨越 Cap 的整个区域,使用 mAbs 确定 B 细胞表位区域。斑点印迹和肽 ELISA 的结果表明,P3、P9 和 P10 是主要的 B 细胞抗原区域。通过较短的 N-和 C-末端截断肽进行精细作图证实, motifsNKPWH、KHSRYFT 和 QSLFFF 是线性 B 细胞表位,在不同的 PCV3 株之间高度保守。有趣的是,我们发现 motifKHSRYFT 在所有报道的 PCV 类型(即 PCV1、PCV2、PCV3 和 PCV4)中都高度保守,除了第一个残基的取代(Y→K→R)。这是首次鉴定 PCV3 Cap 的 B 细胞表位的研究,这些发现可能有助于更好地理解抗体-抗原相互作用,并为 PCV3 疫苗设计提供一些指导。关键点• 以可溶形式表达和纯化了 PCV3 Cap 的重组蛋白。• 本研究制备的 PCV3 Cap 特异性 mAbs 与 PCV1/PCV2 Cap 无交叉反应性。• 这是首次报道 PCV3 Cap 上三个保守的线性 B 细胞表位。• 表位的最小残基为 57-61 aa、140-146 aa 和 161-166 aa。

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