Defining the cross-reactivity between peanut allergens Ara h 2 and Ara h 6 using monoclonal antibodies.

IF 3.4 3区 医学 Q3 IMMUNOLOGY
Orlee Marini-Rapoport, Monica L Fernández-Quintero, Tarun Keswani, Guangning Zong, Jane Shim, Lars C Pedersen, Geoffrey A Mueller, Sarita U Patil
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引用次数: 0

Abstract

In peanut allergy, Arachis hypogaea 2 (Ara h 2) and Arachis hypogaea 6 (Ara h 6) are two clinically relevant peanut allergens with known structural and sequence homology and demonstrated cross-reactivity. We have previously utilized X-ray crystallography and epitope binning to define the epitopes on Ara h 2. We aimed to quantitatively characterize the cross-reactivity between Ara h 2 and Ara h 6 on a molecular level using human monoclonal antibodies (mAbs) and structural characterization of allergenic epitopes. We utilized mAbs cloned from Ara h 2 positive single B cells isolated from peanut-allergic, oral immunotherapy-treated patients to quantitatively analyze cross-reactivity between recombinant Ara h 2 (rAra h 2) and Ara h 6 (rAra h 6) proteins using biolayer interferometry and indirect inhibitory ELISA. Molecular dynamics simulations assessed time-dependent motions and interactions in the antibody-antigen complexes. Three epitopes-conformational epitopes 1.1 and 3, and the sequential epitope KRELRNL/KRELMNL-are conserved between Ara h 2 and Ara h 6, while two more conformational and three sequential epitopes are not. Overall, mAb affinity was significantly lower to rAra h 6 than it was to rAra h 2. This difference in affinity was primarily due to increased dissociation of the antibodies from rAra h 6, a phenomenon explained by the higher conformational flexibility of the Ara h 6-antibody complexes in comparison to Ara h 2-antibody complexes. Our results further elucidate the cross-reactivity of peanut 2S albumins on a molecular level and support the clinical immunodominance of Ara h 2.

使用单克隆抗体确定花生过敏原 Ara h 2 和 Ara h 6 之间的交叉反应。
在花生过敏中,Arachis hypogaea 2(Ara h 2)和Arachis hypogaea 6(Ara h 6)是两种与临床相关的花生过敏原,它们在结构上和序列上具有已知的同源性,并显示出交叉反应性。我们以前曾利用 X 射线晶体学和表位分选来确定 Ara h 2 上的表位。我们的目标是利用人类单克隆抗体(mAbs)和过敏原表位的结构特征,在分子水平上定量描述 Ara h 2 和 Ara h 6 之间的交叉反应。我们利用从花生过敏、口服免疫疗法患者体内分离出的 Ara h 2 阳性单 B 细胞克隆出的 mAbs,使用生物层干涉测量法和间接抑制性 ELISA 定量分析了重组 Ara h 2(rAra h 2)和 Ara h 6(rAra h 6)蛋白之间的交叉反应。分子动力学模拟评估了抗体-抗原复合物中随时间变化的运动和相互作用。三个表位--构象表位 1.1 和 3 以及序列表位 KRELRNL/KRELMNL 在 Ara h 2 和 Ara h 6 之间是保守的,而另外两个构象表位和三个序列表位则不保守。总体而言,mAb 与 rAra h 6 的亲和力明显低于与 rAra h 2 的亲和力。这种亲和力上的差异主要是由于抗体与 rAra h 6 的解离度增加所致,与 Ara h 2-抗体复合物相比,Ara h 6-抗体复合物具有更高的构象灵活性。我们的研究结果进一步阐明了花生 2S 蛋白在分子水平上的交叉反应性,并支持 Ara h 2 的临床免疫优势。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
CiteScore
8.40
自引率
2.20%
发文量
101
审稿时长
3-8 weeks
期刊介绍: Clinical & Experimental Immunology (established in 1966) is an authoritative international journal publishing high-quality research studies in translational and clinical immunology that have the potential to transform our understanding of the immunopathology of human disease and/or change clinical practice. The journal is focused on translational and clinical immunology and is among the foremost journals in this field, attracting high-quality papers from across the world. Translation is viewed as a process of applying ideas, insights and discoveries generated through scientific studies to the treatment, prevention or diagnosis of human disease. Clinical immunology has evolved as a field to encompass the application of state-of-the-art technologies such as next-generation sequencing, metagenomics and high-dimensional phenotyping to understand mechanisms that govern the outcomes of clinical trials.
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