Veterinary Diagnostic Laboratory, Veterinary Diagnostic and Production Animal Medicine, Iowa State University, Ames, IA, USA.
Department of Veterinary Microbiology, Faculty of Veterinary Science, Chulalongkorn University, Bangkok, Thailand.
Vet Microbiol. 2024 Nov;298:110266. doi: 10.1016/j.vetmic.2024.110266. Epub 2024 Oct 2.
Senecavirus A (SVA) is an RNA virus in the family Picornaviridae that has been detected in swine-production systems and is associated with vesicular disease and neonate mortality. The viral capsid is composed of four structural proteins: VP1-VP4. Although the VP1 protein has been reported to be the most immunogenic protein in vivo, no information on the immunodominant regions of the SVA polyprotein is available. The objective of this study was to identify the immunodominant regions of SVA polyprotein using an enzyme-linked immunosorbent assay (ELISA) epitope-mapping approach. The binding effect of SVA polyclonal antibody (SVA-pAb), SVA-VP1 monoclonal antibodies (SVA-mAb), and SVA-positive sera from clinically affected animals were characterized using a set of 18 overlapping SVA VP1-derived peptides by indirect and blocking ELISAs. All VP1 peptides yielded significant signal against SVA-pAb and SVA-VP1-mAb upon indirect ELISA. One peptide (aa 1-20) showed significantly high optical density on SVA recombinant VP1 protein (rVP1) and whole-virus-based indirect ELISAs. The blocking ELISA results demonstrated that peptides spanning aa 165-185 and 225-245 had a 50 % or greater inhibitory effect on SVA-pAb, while six groups of overlapping peptides spanning aa 1-35, 45-80, 90-140, 150-170, 195-230, and 240-264 and two groups of overlapping peptides spanning aa 1-50 and 60-264 showed a 50 % inhibitory effect or greater on swine VP1-mAb and SVA-seropositive swine serum, respectively, against SVA rVP1. Three-dimensional protein homology modeling showed that the peptides binding SVA-pAb are located on the outer surface of the viral capsid, while SVA mAbs and swine-positive sere can bind to epitopes located in both the inner and outer surfaces of the capsid. These linear epitopes showed differential binding and inhibitory activity on mAb and pAb; however, further studies will be necessary to evaluate whether they can act as decoy or neutralizing epitopes. Because mAb antibodies demonstrated a high binding affinity for this set of peptides, this information could lay the foundation for generating and screening specific antibodies for therapeutic potential.
塞尼卡病毒 A(SVA)是一种 RNA 病毒,属于小 RNA 病毒科,已在猪生产系统中检测到,并与水疱病和新生仔猪死亡有关。病毒衣壳由四个结构蛋白组成:VP1-VP4。虽然 VP1 蛋白已被报道为体内最具免疫原性的蛋白,但关于 SVA 多蛋白的免疫优势区尚无信息。本研究旨在使用酶联免疫吸附试验(ELISA)表位作图方法鉴定 SVA 多蛋白的免疫优势区。使用一组 18 个重叠的 SVA VP1 衍生肽通过间接和阻断 ELISA 来表征 SVA 多克隆抗体(SVA-pAb)、SVA-VP1 单克隆抗体(SVA-mAb)和来自临床受影响动物的 SVA 阳性血清的结合效应。间接 ELISA 显示所有 VP1 肽与 SVA-pAb 和 SVA-VP1-mAb 均产生显著信号。一个肽(aa1-20)在 SVA 重组 VP1 蛋白(rVP1)和基于全病毒的间接 ELISA 中表现出显著高的光密度。阻断 ELISA 结果表明,跨越 aa165-185 和 225-245 的肽对 SVA-pAb 具有 50%或更大的抑制作用,而跨越 aa1-35、45-80、90-140、150-170、195-230 和 240-264 的六组重叠肽和跨越 aa1-50 和 60-264 的两组重叠肽对 SVA-rVP1 分别对猪 VP1-mAb 和 SVA 阳性猪血清具有 50%或更大的抑制作用。三维蛋白质同源建模表明,与 SVA-pAb 结合的肽位于病毒衣壳的外表面,而 SVA mAbs 和猪阳性血清可与衣壳内外表面的表位结合。这些线性表位对 mAb 和 pAb 表现出不同的结合和抑制活性;然而,还需要进一步研究来评估它们是否可以作为诱饵或中和表位。由于 mAb 抗体对这组肽表现出高的结合亲和力,因此这些信息可以为产生和筛选具有治疗潜力的特异性抗体奠定基础。
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