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VR9-1(主要虾过敏原Pen a 1(原肌球蛋白)的一种突变体)的变应原性降低

Reduced allergenic potency of VR9-1, a mutant of the major shrimp allergen Pen a 1 (tropomyosin).

作者信息

Reese Gerald, Viebranz Julia, Leong-Kee Susan M, Plante Matthew, Lauer Iris, Randow Stefanie, Moncin Mar San-Miguel, Ayuso Rosalia, Lehrer Samuel B, Vieths Stefan

机构信息

Division of Allergology, Paul Ehrlich Institut, Langen, Germany.

出版信息

J Immunol. 2005 Dec 15;175(12):8354-64. doi: 10.4049/jimmunol.175.12.8354.

DOI:10.4049/jimmunol.175.12.8354
PMID:16339577
Abstract

The major shrimp allergen, tropomyosin, is an excellent model allergen for studying the influence of mutations within the primary structure on the allergenic potency of an allergen; Pen a 1 allows systematic evaluation and comparison of Ab-binding epitopes, because amino acid sequences of both allergenic and nonallergenic tropomyosins are known. Individually recognized IgE Ab-binding epitopes, amino acid positions, and substitutions critical for IgE Ab binding were identified by combinatorial substitution analysis, and 12 positions deemed critical were mutated in the eight major epitopes. The mutant VR9-1 was characterized with regard to allergenic potency by mediator release assays using sera from shrimp-allergic subjects and sera from BALB/c, C57BL/6J, C3H/HeJ, and CBA/J mice sensitized with shrimp extract using alum, cholera toxin, and Bordetella pertussis, as adjuvants. The secondary structure of VR9-1 was not altered; however, the allergenic potency was reduced by 90-98% measuring allergen-specific mediator release from humanized rat basophilic leukemia (RBL) cells, RBL 30/25. Reduced mediator release of RBL-2H3 cells sensitized with sera from mice that were immunized with shrimp extract indicated that mice produced IgE Abs to Pen a 1 and to the same epitopes as humans did. In conclusion, data obtained by mapping sequential epitopes were used to generate a Pen a 1 mutant with significantly reduced allergenic potency. Epitopes that are relevant for human IgE Ab binding are also major binding sites for murine IgE Abs. These results indicate that the murine model might be used to optimize the Pen a 1 mutant for future therapeutic use.

摘要

主要的虾过敏原原肌球蛋白,是研究一级结构内的突变对过敏原致敏效力影响的优秀模型过敏原;Pen a 1有助于对抗体结合表位进行系统评估和比较,因为致敏和非致敏原肌球蛋白的氨基酸序列均已知。通过组合替换分析确定了单个被识别的IgE抗体结合表位、氨基酸位置以及对IgE抗体结合至关重要的替换,并且在八个主要表位中对12个被认为至关重要的位置进行了突变。使用虾过敏受试者的血清以及用明矾、霍乱毒素和百日咳博德特氏菌作为佐剂致敏的BALB/c、C57BL/6J、C3H/HeJ和CBA/J小鼠的血清,通过介质释放试验对突变体VR9-1的致敏效力进行了表征。VR9-1的二级结构未改变;然而,通过测量人源化大鼠嗜碱性白血病(RBL)细胞RBL 30/25中过敏原特异性介质的释放,其致敏效力降低了90%-98%。用虾提取物免疫的小鼠血清致敏的RBL-2H3细胞介质释放减少,表明小鼠产生了针对Pen a 1的IgE抗体,且与人类产生的抗体针对相同的表位。总之,通过绘制连续表位获得的数据被用于生成致敏效力显著降低的Pen a 1突变体。与人类IgE抗体结合相关的表位也是鼠类IgE抗体的主要结合位点。这些结果表明,鼠类模型可用于优化Pen a 1突变体,以供未来治疗使用。

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