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不同模式下的互补决定区可塑性促进抗体应答中的分子模拟。

Paratope plasticity in diverse modes facilitates molecular mimicry in antibody response.

作者信息

Krishnan Lavanya, Lomash Suvendu, Raj Beena Patricia Jeevan, Kaur Kanwal J, Salunke Dinakar M

机构信息

National Institute of Immunology, Aruna Asaf Ali Road, New Delhi-100067, India.

出版信息

J Immunol. 2007 Jun 15;178(12):7923-31. doi: 10.4049/jimmunol.178.12.7923.

DOI:10.4049/jimmunol.178.12.7923
PMID:17548630
Abstract

The immune response against methyl-alpha-D-mannopyranoside mimicking 12-mer peptide (DVFYPYPYASGS) was analyzed at the molecular level towards understanding the equivalence of these otherwise disparate Ags. The Ab 7C4 recognized the immunizing peptide and its mimicking carbohydrate Ag with comparable affinities. Thermodynamic analyses of the binding interactions of both molecules suggested that the mAb 7C4 paratope lacks substantial conformational flexibility, an obvious possibility for facilitating binding to chemically dissimilar Ags. Favorable changes in entropy during binding indicated the importance of hydrophobic interactions in recognition of the mimicking carbohydrate Ag. Indeed, the topology of the Ag-combining site was dominated by a cluster of aromatic residues, contributed primarily by the specificity defining CDR H3. Epitope-mapping analysis demonstrated the critical role of three aromatic residues of the 12-mer in binding to the Ab. Our studies delineate a mechanism by which mimicry is manifested in the absence of either structural similarity of the epitopes or conformational flexibility in the paratope. An alternate mode of recognition of dissimilar yet mimicking Ags by the anti-peptide Ab involves plasticity associated with aromatic/hydrophobic and van der Waals interactions. Thus, antigenic mimicry may be a consequence of paratope-specific modulations rather than being dependent only on the properties of the epitope. Such modulations may have evolved toward minimizing the consequences of antigenic variation by invading pathogens.

摘要

为了理解这些原本不同的抗原的等效性,在分子水平上分析了针对模拟12肽(DVFYPYPYASGS)的甲基-α-D-甘露吡喃糖苷的免疫反应。抗体7C4以相当的亲和力识别免疫肽及其模拟碳水化合物抗原。对这两种分子结合相互作用的热力学分析表明,单克隆抗体7C4的互补决定区缺乏显著的构象灵活性,而构象灵活性是促进与化学性质不同的抗原结合的一种明显可能性。结合过程中有利的熵变表明疏水相互作用在识别模拟碳水化合物抗原中的重要性。实际上,抗原结合位点的拓扑结构主要由一簇芳香族残基主导,这些残基主要由定义特异性的互补决定区H3贡献。表位映射分析证明了12肽中的三个芳香族残基在与抗体结合中的关键作用。我们的研究描述了一种机制,通过该机制,在表位没有结构相似性或互补决定区没有构象灵活性的情况下,模拟现象得以表现。抗肽抗体识别不同但模拟的抗原的另一种模式涉及与芳香族/疏水相互作用和范德华相互作用相关联的可塑性。因此,抗原模拟可能是互补决定区特异性调节的结果,而不仅仅取决于表位的性质。这种调节可能已经进化,以尽量减少入侵病原体引起的抗原变异的后果。

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