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通过一种基于新型嵌合体的过敏原表位定位策略,鉴定出了橡胶素(Hev b6.02)的主要构象性IgE结合表位。

The major conformational IgE-binding epitopes of hevein (Hev b6.02) are identified by a novel chimera-based allergen epitope mapping strategy.

作者信息

Karisola Piia, Alenius Harri, Mikkola Jari, Kalkkinen Nisse, Helin Jari, Pentikäinen Olli T, Repo Susanna, Reunala Timo, Turjanmaa Kristiina, Johnson Mark S, Palosuo Timo, Kulomaa Markku S

机构信息

Department of Biological and Environmental Science, University of Jyväskylä, P. O. Box 35 (YAB), FIN-40014 University of Jyvaskyla, Finland.

出版信息

J Biol Chem. 2002 Jun 21;277(25):22656-61. doi: 10.1074/jbc.M201076200. Epub 2002 Mar 21.

DOI:10.1074/jbc.M201076200
PMID:11909866
Abstract

A novel approach to localize and reconstruct conformational IgE-binding epitope regions of hevein (Hev b6.02), a major natural rubber latex allergen, is described. An antimicrobial protein (AMP) from the amaranth Amaranthus caudatus was used as an immunologically non-IgE-binding adaptor molecule to which terminal or central parts of hevein were fused. Hevein and AMP share a structurally identical core region but have different N-terminal and C-terminal regions. Only 1 of 16 hevein-allergic patients showed weak IgE binding to purified native or recombinant AMP. Chimeric AMP with the hevein N terminus was recognized by IgE from 14 (88%) patients, and chimeric AMP with the hevein C terminus was recognized by IgE from 6 (38%) patients. In contrast, chimeric AMP containing the hevein core region was recognized by IgE from only two patients. When both the N-terminal and C-terminal regions of hevein were fused with the AMP core, IgE from all 16 patients bound to the chimera. This chimera was also able to significantly inhibit (>70%) IgE binding to the native hevein. On the contrary, linear synthetic peptides corresponding to hevein regions in the AMP chimeras showed no significant IgE binding capacity in either enzyme-linked immunosorbent assay or inhibition enzyme-linked immunosorbent assay. These results suggest that the IgE binding ability of hevein is essentially determined by its N-terminal and C-terminal regions and that major IgE-binding epitopes of hevein are conformational. The chimera-based epitope mapping strategy described here provides a valuable tool for defining structural epitopes and creating specific reagents for allergen immunotherapy.

摘要

本文描述了一种定位和重建主要天然橡胶乳胶过敏原橡胶素(Hev b6.02)构象性IgE结合表位区域的新方法。来自尾穗苋的一种抗菌蛋白(AMP)被用作免疫非IgE结合衔接分子,橡胶素的末端或中央部分与之融合。橡胶素和AMP具有结构相同的核心区域,但N端和C端区域不同。16名橡胶素过敏患者中只有1名对纯化的天然或重组AMP表现出弱IgE结合。含有橡胶素N端的嵌合AMP被14名(88%)患者的IgE识别,含有橡胶素C端的嵌合AMP被6名(38%)患者的IgE识别。相比之下,含有橡胶素核心区域的嵌合AMP仅被两名患者的IgE识别。当橡胶素的N端和C端区域都与AMP核心融合时,所有16名患者的IgE都与该嵌合体结合。该嵌合体也能够显著抑制(>70%)IgE与天然橡胶素的结合。相反,与AMP嵌合体中橡胶素区域相对应的线性合成肽在酶联免疫吸附测定或抑制酶联免疫吸附测定中均未显示出显著的IgE结合能力。这些结果表明,橡胶素的IgE结合能力主要由其N端和C端区域决定,且橡胶素的主要IgE结合表位是构象性的。本文所述的基于嵌合体的表位定位策略为定义结构表位和创建用于变应原免疫治疗的特异性试剂提供了一种有价值的工具。

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