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桦树花粉主要过敏原Bet v 1的主要IgE结合表位,通过X射线晶体学和定点诱变进行表征。

Dominating IgE-binding epitope of Bet v 1, the major allergen of birch pollen, characterized by X-ray crystallography and site-directed mutagenesis.

作者信息

Spangfort Michael D, Mirza Osman, Ipsen Henrik, Van Neerven R J Joost, Gajhede Michael, Larsen Jørgen N

机构信息

ALK-Abelló, Research Department, Hørsholm, Denmark.

出版信息

J Immunol. 2003 Sep 15;171(6):3084-90. doi: 10.4049/jimmunol.171.6.3084.

DOI:10.4049/jimmunol.171.6.3084
PMID:12960334
Abstract

Specific allergy vaccination is an efficient treatment for allergic disease; however, the development of safer vaccines would enable a more general use of the treatment. Determination of molecular structures of allergens and allergen-Ab complexes facilitates epitope mapping and enables a rational approach to the engineering of allergen molecules with reduced IgE binding. In this study, we describe the identification and modification of a human IgE-binding epitope based on the crystal structure of Bet v 1 in complex with the BV16 Fab' fragment. The epitope occupies approximately 10% of the molecular surface area of Bet v 1 and is clearly conformational. A synthetic peptide representing a sequential motif in the epitope (11 of 16 residues) did not inhibit the binding of mAb BV16 to Bet v 1, illustrating limitations in the use of peptides for B cell epitope characterization. The single amino acid substitution, Glu(45)-Ser, was introduced in the epitope and completely abolished the binding of mAb BV16 to the Bet v 1 mutant within a concentration range 1000-fold higher than wild type. The mutant also showed up to 50% reduction in the binding of human polyclonal IgE, demonstrating that glutamic acid 45 is a critical amino acid also in a major human IgE-binding epitope. By solving the three-dimensional crystal structure of the Bet v 1 Glu(45)-Ser mutant, it was shown that the change in immunochemical activity is directly related to the Glu(45)-Ser substitution and not to long-range structural alterations or collapse of the Bet v 1 mutant tertiary structure.

摘要

特异性变应原疫苗接种是治疗变应性疾病的一种有效方法;然而,开发更安全的疫苗将使该治疗方法得到更广泛的应用。变应原和变应原 - 抗体复合物分子结构的确定有助于表位作图,并能为设计降低IgE结合能力的变应原分子提供合理方法。在本研究中,我们基于与BV16 Fab'片段形成复合物的Bet v 1晶体结构,描述了一种人IgE结合表位的鉴定和修饰。该表位约占Bet v 1分子表面积的10%,且明显是构象性的。代表该表位中一个连续基序(16个残基中的11个)的合成肽并未抑制单克隆抗体BV16与Bet v 1的结合,这说明了在使用肽进行B细胞表位特征化方面的局限性。在该表位中引入单个氨基酸取代,即Glu(45)-Ser,完全消除了单克隆抗体BV16在比野生型高1000倍的浓度范围内与Bet v 1突变体的结合。该突变体与人多克隆IgE的结合也显示出高达50%的降低,这表明谷氨酸45在主要的人IgE结合表位中也是关键氨基酸。通过解析Bet v 1 Glu(45)-Ser突变体的三维晶体结构,表明免疫化学活性的变化直接与Glu(45)-Ser取代相关,而与Bet v 1突变体三级结构的远程结构改变或塌陷无关。

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