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天疱疮抗体识别的主要自身免疫表位定位于桥粒芯糖蛋白的N端黏附区域。

Dominant autoimmune epitopes recognized by pemphigus antibodies map to the N-terminal adhesive region of desmogleins.

作者信息

Sekiguchi M, Futei Y, Fujii Y, Iwasaki T, Nishikawa T, Amagai M

机构信息

Department of Dermatology, Keio University School of Medicine, Tokyo, Japan.

出版信息

J Immunol. 2001 Nov 1;167(9):5439-48. doi: 10.4049/jimmunol.167.9.5439.

DOI:10.4049/jimmunol.167.9.5439
PMID:11673563
Abstract

Desmoglein (Dsg) is a cadherin-type adhesion molecule found in desmosomes. Dsg1 and Dsg3 are the target Ags in the autoimmune blistering diseases pemphigus foliaceus (PF) and pemphigus vulgaris (PV), respectively. To map conformational epitopes of Dsg1 and Dsg3 in PF and PV, we generated Dsg1- and Dsg3-domain-swapped molecules and point-mutated Dsg3 molecules with Dsg1-specific residues by baculovirus expression. The swapped domains were portions of the N-terminal extracellular domains of Dsg1 (1-496) and Dsg3 (1-566), which have similar structures but distinct epitopes. The binding of autoantibodies to the mutant molecules was assessed by competition ELISAs. Domain-swapped molecules containing the N-terminal 161 residues of Dsg1 and Dsg3 yielded >50% competition in 30/43 (69.8%) PF sera and 31/40 (77.5%) PV sera, respectively. Furthermore, removal of Abs against the 161 N-terminal residues of Dsg1 by immunoadsorption eliminated the ability of PF sera to induce cutaneous blisters in neonatal mice. Within these N-terminal regions, most of the epitopes were mapped to residues 26-87 of Dsg1 and 25-88 of Dsg3. Furthermore, a point-mutated Dsg3 molecule containing Dsg1-specific amino acid substitutions (His(25), Cys(28), Ala(29)) reacted with anti-Dsg1 IgG, thus defining one of the epitopes of Dsg1. Using the predicted three-dimensional structure of classic cadherins as a model, these findings suggest that the dominant autoimmune epitopes in both PF and PV are found in the N-terminal adhesive surfaces of Dsgs.

摘要

桥粒芯糖蛋白(Dsg)是一种存在于桥粒中的钙黏蛋白型黏附分子。Dsg1和Dsg3分别是自身免疫性水疱病落叶型天疱疮(PF)和寻常型天疱疮(PV)中的靶抗原。为了定位PF和PV中Dsg1和Dsg3的构象表位,我们通过杆状病毒表达产生了Dsg1和Dsg3结构域交换分子以及具有Dsg1特异性残基的点突变Dsg3分子。交换的结构域是Dsg1(1 - 496)和Dsg3(1 - 566)N端细胞外结构域的部分,它们具有相似的结构但不同的表位。通过竞争ELISA评估自身抗体与突变分子的结合。含有Dsg1和Dsg3 N端161个残基的结构域交换分子在30/43(69.8%)的PF血清和31/40(77.5%)的PV血清中分别产生了>50%的竞争。此外,通过免疫吸附去除针对Dsg1 N端161个残基的抗体消除了PF血清诱导新生小鼠皮肤水疱的能力。在这些N端区域内,大多数表位定位于Dsg1的26 - 87位残基和Dsg3的25 - 88位残基。此外,一个含有Dsg1特异性氨基酸取代(His(25)、Cys(28)、Ala(29))的点突变Dsg3分子与抗Dsg1 IgG反应,从而确定了Dsg1的一个表位。以经典钙黏蛋白的预测三维结构为模型,这些发现表明PF和PV中的主要自身免疫表位都存在于Dsg的N端黏附表面。

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