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粉尘螨过敏原 Der f 21 的晶体结构和表位分析。

Crystal structure and epitope analysis of house dust mite allergen Der f 21.

机构信息

Institute of Systems Biology, Universiti Kebangsaan Malaysia, 43600 UKM Bangi, Selangor, Malaysia.

Department of Pathology, Faculty of Medicine and Health Sciences, Universiti Putra Malaysia, 43400 UPM Serdang, Selangor, Malaysia.

出版信息

Sci Rep. 2019 Mar 20;9(1):4933. doi: 10.1038/s41598-019-40879-x.

Abstract

Group 21 and 5 allergens are homologous house dust mite proteins known as mid-tier allergens. To reveal the biological function of group 21 allergens and to understand better the allergenicity of the rDer f 21 allergen, we determined the 1.5 Å crystal structure of rDer f 21 allergen from Dermatophagoides farinae. The rDer f 21 protein consists of a three helical bundle, similar to available structures of group 21 and homologous group 5 allergens. The rDer f 21 dimer forms a hydrophobic binding pocket similar to the one in the Der p 5 allergen, which indicates that both of the homologous groups could share a similar function. By performing structure-guided mutagenesis, we mutated all 38 surface-exposed polar residues of the rDer f 21 allergen and carried out immuno-dot blot assays using 24 atopic sera. Six residues, K10, K26, K42, E43, K46, and K48, which are located in the region between the N-terminus and the loop 1 of rDer f 21 were identified as the major IgE epitopes of rDer f 21. Epitope mapping of all potential IgE epitopes on the surface of the rDer f 21 crystal structure revealed heterogeneity in the sIgE recognition of the allergen epitopes in atopic individuals. The higher the allergen-sIgE level of an individual, the higher the number of epitope residues that are found in the allergen. The results illustrate the clear correlation between the number of specific major epitope residues in an allergen and the sIgE level of the atopic population.

摘要

组 21 和 5 过敏原是同源的屋尘螨蛋白,被称为中层过敏原。为了揭示组 21 过敏原的生物学功能,并更好地了解 rDer f 21 过敏原的变应原性,我们测定了来自屋尘螨的 rDer f 21 过敏原的 1.5 Å 晶体结构。rDer f 21 蛋白由三个螺旋束组成,与现有的组 21 和同源组 5 过敏原结构相似。rDer f 21 二聚体形成一个疏水性结合口袋,类似于 Der p 5 过敏原中的结合口袋,这表明这两个同源组可能具有相似的功能。通过进行结构导向的突变,我们突变了 rDer f 21 过敏原所有 38 个表面暴露的极性残基,并使用 24 份特应性血清进行免疫斑点印迹分析。鉴定出位于 rDer f 21 的 N 端和环 1 之间的区域的 6 个残基 K10、K26、K42、E43、K46 和 K48 是 rDer f 21 的主要 IgE 表位。rDer f 21 晶体结构表面所有潜在 IgE 表位的表位作图显示,特应性个体对过敏原表位的 sIgE 识别存在异质性。个体的过敏原-sIgE 水平越高,过敏原中发现的表位残基数量就越高。结果表明,过敏原中特定主要表位残基的数量与特应性人群的 sIgE 水平之间存在明显的相关性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/74f3/6426935/c6801fdb8fc1/41598_2019_40879_Fig1_HTML.jpg

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