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鸡IgY在CH3/CH4界面结合其受体的方式与人类IgA:FcαRI相互作用类似。

Chicken IgY binds its receptor at the CH3/CH4 interface similarly as the human IgA: Fc alpha RI interaction.

作者信息

Pürzel Jana, Schmitt Ramona, Viertlboeck Birgit C, Göbel Thomas W

机构信息

Department of Veterinary Sciences, University of Munich, Munich, Germany.

出版信息

J Immunol. 2009 Oct 1;183(7):4554-9. doi: 10.4049/jimmunol.0901699. Epub 2009 Sep 11.

DOI:10.4049/jimmunol.0901699
PMID:19748988
Abstract

Chicken IgY, the ancestral form of mammalian IgE and IgG, is recognized by the high-affinity FcY receptor CHIR-AB1, a member of the leukocyte receptor family. In this study, we have characterized the receptor ligand interaction site by consecutive truncations of the Fcv IgY domains and mutational analyses of selected residues. Using several fusion proteins that linked the human Cgamma2 and Cgamma3 domains with the Fcv IgY domains, a binding assay revealed that both the Fcv3 and Fcv4 domains were essential for the IgY CHIR-AB1 interaction. Sequence comparisons of chicken IgY with human IgA demonstrated that 11 of the 19 contact residues important for the IgA FcalphaRI interaction have been conserved in chicken IgY, although the overall amino acid identity is only 34%. Among the 19 amino acids at respective positions in IgY, the mutation of two residues in the Fcv3 and two in the Fcv4 domain completely abolished the IgY to CHIR-AB1 binding revealed by two independent assays. Three further mutations substantially altered the interaction. Molecular modeling on the Cv3 to Cv4 crystal structure revealed that all critical residues, although on two domains, are in close proximity. The importance of N-linked carbohydrates was demonstrated by the failure of the CHIR-AB1 interaction after mutation of the glycosylation site. The identification of the IgY Cv3/Cv4 interdomain region as critical for binding to CHIR-AB1 significantly enhances our understanding of the IgY receptor interaction and allows further conclusions regarding the FcR phylogeny.

摘要

鸡IgY是哺乳动物IgE和IgG的原始形式,可被白细胞受体家族成员高亲和力Fcγ受体CHIR-AB1识别。在本研究中,我们通过连续截短Fcγ IgY结构域和对选定残基进行突变分析,对受体-配体相互作用位点进行了表征。使用几种将人Cγ2和Cγ3结构域与Fcγ IgY结构域连接的融合蛋白,结合试验表明Fcγ3和Fcγ4结构域对于IgY与CHIR-AB1的相互作用都是必不可少的。鸡IgY与人IgA的序列比较表明,尽管总体氨基酸同一性仅为34%,但对IgA FcαRI相互作用重要的19个接触残基中有11个在鸡IgY中保守。在IgY各自位置的19个氨基酸中,Fcγ3结构域中的两个残基和Fcγ4结构域中的两个残基发生突变,通过两项独立试验表明完全消除了IgY与CHIR-AB1的结合。另外三个突变显著改变了相互作用。对Cγ3至Cγ4晶体结构的分子建模表明,所有关键残基虽然位于两个结构域上,但彼此靠近。糖基化位点突变后CHIR-AB1相互作用失败证明了N-连接碳水化合物的重要性。将IgY Cγ3/Cγ4结构域间区域鉴定为与CHIR-AB1结合的关键区域,显著增强了我们对IgY受体相互作用的理解,并允许对FcR系统发育得出进一步结论。

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