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鉴定对IgE与牛κ-酪蛋白连续表位结合至关重要的氨基酸以及这些表位与相应人κ-酪蛋白序列的相似性。

Identification of amino acids critical for IgE-binding to sequential epitopes of bovine kappa-casein and the similarity of these epitopes to the corresponding human kappa-casein sequence.

作者信息

Han N, Järvinen K M, Cocco R R, Busse P J, Sampson H A, Beyer K

机构信息

Division of Pediatric Allergy & Immunology, Jaffe Institute for Food Allergy, The Mount Sinai School of Medicine, New York, NY 10029-6574, USA.

出版信息

Allergy. 2008 Feb;63(2):198-204. doi: 10.1111/j.1398-9995.2007.01539.x.

DOI:10.1111/j.1398-9995.2007.01539.x
PMID:18186809
Abstract

BACKGROUND

The delineation of allergenic (i.e. IgE-binding) epitopes in cow's milk proteins and the amino acids (AAs) critical for IgE-binding is necessary to understand better the structural properties of an allergen and to develop more efficacious immunotherapeutic reagents. Furthermore, this information may enable us to understand better cross-sensitivity between different allergens.

METHODS

Eleven peptides, 10-14 AAs in length, representing the IgE-binding epitopes of kappa-casein were synthesized on a derivatized cellulose membrane with single AA substitutions at each position. Membranes were incubated with pooled sera from 15 milk-allergic patients and individual sera from 10 of the patients included in the pool.

RESULTS

For 10/11 allergenic peptides, one to five different single AA substitutions resulted in elimination of IgE-binding of pooled patient sera. Overall at least one mutated peptide could be found for these 10 IgE-binding sites that resulted in a reduction of IgE-binding in at least 80% of the patients who recognized the native protein. Furthermore, the IgE-binding region at AA104-112 on bovine kappa-casein showed a high degree of similarity with the human kappa-casein, respectively, including the AAs critical for IgE-binding.

CONCLUSION

This finding suggests that critical AAs should be assessed with both pooled and individual patient sera to account for the B-cell epitope heterogeneity between patients, with cow's milk allergy. In addition, we identified two potentially cross-reactive peptides between bovine and human caseins of unknown clinical relevance.

摘要

背景

明确牛奶蛋白中的变应原性(即IgE结合)表位以及对IgE结合至关重要的氨基酸,对于更好地理解变应原的结构特性和开发更有效的免疫治疗试剂是必要的。此外,这些信息可能使我们能更好地理解不同变应原之间的交叉敏感性。

方法

合成了11条长度为10 - 14个氨基酸的肽段,它们代表κ-酪蛋白的IgE结合表位,在衍生化的纤维素膜上合成,每个位置有单个氨基酸替换。将膜与15名牛奶过敏患者的混合血清以及混合血清中10名患者的个体血清一起孵育。

结果

对于10/11个变应原性肽段,一到五个不同的单个氨基酸替换导致混合患者血清的IgE结合消除。总体而言,对于这10个IgE结合位点,至少可以找到一种突变肽,其导致至少80%识别天然蛋白的患者的IgE结合减少。此外,牛κ-酪蛋白上第104 - 112位氨基酸的IgE结合区域分别与人κ-酪蛋白显示出高度相似性,包括对IgE结合至关重要的氨基酸。

结论

这一发现表明,对于牛奶过敏患者,应使用混合血清和个体患者血清评估关键氨基酸,以考虑患者之间B细胞表位的异质性。此外,我们鉴定出两种牛和人酪蛋白之间潜在的交叉反应性肽段,其临床相关性未知。

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