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黑麦草花粉主要过敏原Lol p 5的IgE识别分子基础。

Molecular basis of IgE-recognition of Lol p 5, a major allergen of rye-grass pollen.

作者信息

Suphioglu C, Blaher B, Rolland J M, McCluskey J, Schäppi G, Kenrick J, Singh M B, Knox R B

机构信息

School of Botany, University of Melbourne, Parkville, Victoria, Australia.

出版信息

Mol Immunol. 1998 Apr;35(5):293-305. doi: 10.1016/s0161-5890(98)00050-9.

DOI:10.1016/s0161-5890(98)00050-9
PMID:9747889
Abstract

Grass pollen, especially of rye-grass (Lolium perenne). represents an important cause of type I allergy. Identification of IgE-binding (allergenic) epitopes of major grass pollen allergens is essential for understanding the molecular basis of interaction between allergens and human IgE antibodies and therefore facilitates the devising of safer and more effective diagnostic and immunotherapy reagents. The aim of this study was to identify the allergenic epitopes of Lol p 5, a major allergen of rye-grass pollen, immunodissect these epitopes further so that the amino acid residues critical for antibody binding can be determined and investigate the conservation and nature of these epitopes within the context of the natural grass pollen allergens. Peptides, 12-13 amino acid residues long and overlapping each other by 4 amino acid residues, based on the entire deduced amino acid sequence of the coding region of Lol p 5, were synthesised and assayed for IgE-binding. Two strong IgE-binding epitopes (Lol p 5 (49-60) and (265-276), referred to as peptides 7 and 34, respectively) were identified. These epitopes were further resolved by truncated peptides and amino acid replacement studies and the amino acid residues critical for IgE-binding determined (Lol p 5 (49-60) residue Lys57 and (265-276) residue Lys275). Sequences of these epitopes were conserved in related allergens and may form the conserved allergenic domains responsible for the cross-reactivity observed between pollen allergens of taxonomically related grasses. Furthermore, due to its strong IgE-reactivity, synthetic peptide Lol p 5 (265-276) was used to affinity-purify specific IgE antibodies which recognised proteins of other clinically important grass pollens. further indicating presence of allergenic cross-reactivity at the level of allergenic epitope. Moreover, Lol p 5 (265 276) demonstrated a strong capacity to inhibit IgE-binding to natural rye-grass pollen proteins highlighting the antibody accessibility to these sequences within the context of the natural allergens. Strong IgE-binding epitopes of Lol p 5 have been identified down to single critical amino acid residues and are shown to occur as linear or continuous domains in the natural conformation of natural Lol p 5 and other group 5 grass pollen allergens. The fact that such an allergenic synthetic epitope has the capacity to strongly inhibit IgE-binding to natural allergens highlight its potential for use as a candidate in future therapeutics to treat pollen-associated allergies.

摘要

草花粉,尤其是黑麦草(多年生黑麦草)的花粉,是I型过敏的一个重要诱因。鉴定主要草花粉过敏原的IgE结合(致敏)表位,对于理解过敏原与人类IgE抗体之间相互作用的分子基础至关重要,因此有助于设计更安全、更有效的诊断和免疫治疗试剂。本研究的目的是鉴定黑麦草花粉主要过敏原Lol p 5的致敏表位,进一步对这些表位进行免疫剖析,以确定对抗体结合至关重要的氨基酸残基,并在天然草花粉过敏原的背景下研究这些表位的保守性和性质。根据Lol p 5编码区推导的完整氨基酸序列,合成了长度为12 - 13个氨基酸残基且彼此重叠4个氨基酸残基的肽段,并检测其IgE结合能力。鉴定出两个强IgE结合表位(Lol p 5 (49 - 60) 和 (265 - 276),分别称为肽段7和34)。通过截短肽段和氨基酸置换研究进一步解析了这些表位,并确定了对IgE结合至关重要的氨基酸残基(Lol p 5 (49 - 60) 中的赖氨酸57和 (265 - 276) 中的赖氨酸275)。这些表位的序列在相关过敏原中保守,可能形成负责分类学上相关草类花粉过敏原之间交叉反应的保守致敏结构域。此外,由于其强烈的IgE反应性,合成肽Lol p 5 (265 - 276) 被用于亲和纯化识别其他临床重要草花粉蛋白的特异性IgE抗体,进一步表明在致敏表位水平存在致敏交叉反应。此外,Lol p 5 (265 - 276) 表现出强大的抑制IgE与天然黑麦草花粉蛋白结合的能力,突出了在天然过敏原背景下抗体对这些序列的可及性。已鉴定出Lol p 5的强IgE结合表位直至单个关键氨基酸残基,并显示在天然Lol p 5和其他第5组草花粉过敏原的天然构象中以线性或连续结构域形式存在。这种致敏合成表位能够强烈抑制IgE与天然过敏原结合这一事实,突出了其作为未来治疗花粉相关过敏候选物的潜力。

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