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一种基于快速、全面的液相色谱-质谱(LC-MS)的方法,用于检测人白内障晶状体中天冬酰胺异构体。

A rapid, comprehensive liquid chromatography-mass spectrometry (LC-MS)-based survey of the Asp isomers in crystallins from human cataract lenses.

机构信息

Research Reactor Institute, Kyoto University Kumatori-cho, Sennan-gun, Osaka 590-0494, Japan.

出版信息

J Biol Chem. 2012 Nov 16;287(47):39992-40002. doi: 10.1074/jbc.M112.399972. Epub 2012 Sep 24.

Abstract

Cataracts are caused by clouding of the eye lens and may lead to partial or total loss of vision. The mechanism of cataract development, however, is not well understood. It is thought that abnormal aggregates of lens proteins form with age, causing loss of lens clarity and development of the cataract. Lens proteins are composed of soluble α-, β-, and γ-crystallins, and as long lived proteins, they undergo post-translational modifications including isomerization, deamidation, and oxidation, which induce insolubilization, aggregation, and loss of function that may lead to cataracts. Therefore, analysis of post-translational modifications of individual amino acid residues in proteins is important. However, detection of the optical isomers of amino acids formed in these proteins is difficult because optical resolution is only achieved using complex methodology. In this study, we describe a new method for the analysis of isomerization of individual Asp residues in proteins using LC-MS and the corresponding synthetic peptides containing the Asp isomers. This makes it possible to analyze isomers of Asp residues in proteins precisely and quickly. We demonstrate that Asp-58, -76, -84, and -151 of αA-crystallin and Asp-62 and -96 of αB-crystallin are highly converted to lβ-, dβ-, and dα-isomers. The amount of isomerization of Asp is greater in the insoluble fraction at all Asp sites in lens proteins, therefore indicating that isomerization of these Asp residues affects the higher order structure of the proteins and contributes to the increase in aggregation, insolubilization, and disruption of function of proteins in the lens, leading to the cataract.

摘要

白内障是由眼睛晶状体混浊引起的,可能导致部分或完全失明。然而,白内障的发展机制尚不清楚。据认为,晶状体蛋白的异常聚集随着年龄的增长而形成,导致晶状体清晰度丧失和白内障的发展。晶状体蛋白由可溶性α-、β-和γ-晶状体组成,作为长寿命蛋白,它们经历翻译后修饰,包括异构化、脱酰胺和氧化,这些修饰诱导不溶、聚集和功能丧失,可能导致白内障。因此,分析蛋白质中单个氨基酸残基的翻译后修饰非常重要。然而,由于仅使用复杂的方法才能实现光学分辨率,因此很难检测到这些蛋白质中形成的氨基酸的光学异构体。在这项研究中,我们描述了一种使用 LC-MS 分析蛋白质中单个 Asp 残基异构化的新方法,以及含有 Asp 异构体的相应合成肽。这使得能够精确和快速地分析蛋白质中 Asp 残基的异构体。我们证明αA-晶状体蛋白中的 Asp-58、-76、-84 和-151 和αB-晶状体蛋白中的 Asp-62 和-96 高度转化为 lβ-、dβ-和 dα-异构体。在所有晶状体蛋白的 Asp 位点的不溶性部分中,Asp 的异构化量更大,因此表明这些 Asp 残基的异构化会影响蛋白质的高级结构,并导致蛋白质聚集、不溶和功能丧失增加,导致白内障。

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