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一种新的小麦粉过敏原分离与鉴定方法。

A new approach to the isolation and characterization of wheat flour allergens.

机构信息

Institute of Microbiology, Academy of Sciences of Czech Republic, Prague, Czech Republic.

出版信息

Clin Exp Allergy. 2011 Jul;41(7):1031-43. doi: 10.1111/j.1365-2222.2011.03766.x. Epub 2011 May 31.

Abstract

BACKGROUND

The incidence of food allergy to wheat is increasing. Its diagnosis depends on the purity of major allergens and their inclusion in tests. Isolation and characterization of wheat allergens are therefore of utmost importance.

OBJECTIVE

To purify and identify wheat flour allergens most frequently recognized by patients' IgE antibodies and to study their allergenicity.

METHODS

Water/salt-soluble extracts from wheat flour were prepared and separated using a combination of ultrafiltration, isoelectric focusing and liquid chromatography. Purified proteins were analysed by immunoblotting using pooled sera from patients with atopic dermatitis who possessed IgE specific to wheat. Wheat proteins found to bind IgE were subsequently identified by matrix-assisted laser desorption/ionisation-time of flight mass spectrometry. The frequency and intensity of IgE binding of isolated proteins were tested using individual sera from patients and controls.

RESULTS

We developed a procedure that allows isolation of wheat allergens from natural sources. Twenty-seven potential wheat allergens have been successfully identified; of these, the following seven are newly reported in food allergy: endogenous α-amylase/subtilisin inhibitor, trypsin/α-amylase inhibitor (AAI) CMX1/CMX3, thaumatin-like protein (TLP), xylanase inhibitor protein-1, β-glucosidase, class II chitinase and 26 kDa endochitinase. TLP and wheatwin were shown to activate patients' basophils to a similar extent as two well-known allergens, lipid transfer protein (Tri a 14) and AAI 0.19 (Tri a 28.0101).

CONCLUSION AND CLINICAL RELEVANCE

Our new approach enables the isolation of water/salt-soluble wheat allergens in their native form in amounts sufficient both for biological testing (in vivo and in vitro) and for physicochemical characterization. Such studies will lead to a more detailed knowledge of allergenicity of wheat proteins and to improved accuracy of diagnostic tests.

摘要

背景

小麦食物过敏的发病率正在上升。其诊断取决于主要过敏原的纯度及其是否包含在检测中。因此,分离和鉴定小麦过敏原至关重要。

目的

纯化和鉴定小麦面粉中最常被患者 IgE 抗体识别的过敏原,并研究其变应原性。

方法

采用超滤、等电聚焦和液相色谱相结合的方法,从小麦粉中提取水溶性和盐溶性提取物。使用来自特应性皮炎患者的混合血清(这些患者的 IgE 对小麦具有特异性)通过免疫印迹分析纯化的蛋白质。随后通过基质辅助激光解吸/电离-飞行时间质谱鉴定与 IgE 结合的小麦蛋白。使用来自患者和对照的个体血清测试分离蛋白的 IgE 结合的频率和强度。

结果

我们开发了一种从天然来源中分离小麦过敏原的程序。已成功鉴定出 27 种潜在的小麦过敏原;其中,以下七种在食物过敏中为新报告:内源性α-淀粉酶/枯草杆菌蛋白酶抑制剂、胰蛋白酶/α-淀粉酶抑制剂(AAI)CMX1/CMX3、硫素蛋白(TLP)、木聚糖酶抑制剂蛋白-1、β-葡糖苷酶、II 类几丁质酶和 26 kDa 内几丁质酶。TLP 和 wheatwin 被证明能够以与两种知名过敏原(脂质转移蛋白(Tri a 14)和 AAI 0.19(Tri a 28.0101))相似的程度激活患者的嗜碱性粒细胞。

结论和临床相关性

我们的新方法能够以足够的量分离出天然形式的水溶性和盐溶性小麦过敏原,用于生物学测试(体内和体外)和理化特性分析。这些研究将导致对小麦蛋白变应原性的更详细了解,并提高诊断测试的准确性。

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