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乳糖和半乳糖对β-乳球蛋白的固态糖基化作用:运用质谱技术对修饰氨基酸进行定位

Solid-state glycation of beta-lactoglobulin by lactose and galactose: localization of the modified amino acids using mass spectrometric techniques.

作者信息

Fenaille François, Morgan François, Parisod Véronique, Tabet Jean-Claude, Guy Philippe A

机构信息

Nestlé Research Center, Nestec Ltd, Vers-Chez-les-Blanc, 1000 Lausanne 26, Switzerland.

出版信息

J Mass Spectrom. 2004 Jan;39(1):16-28. doi: 10.1002/jms.539.

DOI:10.1002/jms.539
PMID:14760609
Abstract

The Maillard reaction is commonly encountered during food processing or storage, and also in human nutrition, hence there is a need for analytical methodologies to identify and characterize the modified proteins. This paper reports specific methods using mass spectrometric techniques to localize protein modifications induced by lactose and galactose on beta-lactoglobulin (beta-Lg) under solid-state glycation conditions. The extent of glycation was first determined by liquid chromatography/electrospray ionization mass spectrometry (LC/ESI-MS). The specific identification of lactose-modified amino acid residues was realized using both NanoESI-MS, NanoESI-MS/MS (neutral loss scanning modes) and matrix-assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI-TOFMS) (with and without guanidination of lysine residues) on unfractionated digests. The results indicated that, after 8.25 h of incubation, the lysine residues were the main targets of lactose-induced modification. In addition to the 15 lysine residues, Leu1 (NH2 terminal) and the Arg124 were also found to be modified, thus leading to a total of 17 different modified amino acid residues (versus 15 found by LC/ESI-MS measurement). In a second set of experiments, different strategies consisting of constant neutral loss and precursor ion scanning were compared to characterize galactose-induced modifications. Owing to the high level of beta-Lg glycation, the combined use of these different strategies appeared to be necessary for determining the galactose-modified sites after 8.25 h of incubation. Thus, among the 22 galactose adducts deduced from the LC/ESI-MS measurement, apart from the N-terminal and classical lysine residues, we also observed a few arginine residues (Arg40, Arg124 and Arg148) that were modified, and also dialkylations on specific lysine residues (Lys47, Lys75).

摘要

美拉德反应在食品加工或储存过程中以及人体营养中普遍存在,因此需要分析方法来鉴定和表征修饰后的蛋白质。本文报道了使用质谱技术在固态糖化条件下定位乳糖和半乳糖诱导的β-乳球蛋白(β-Lg)上蛋白质修饰的具体方法。首先通过液相色谱/电喷雾电离质谱(LC/ESI-MS)确定糖化程度。使用纳升电喷雾电离质谱(NanoESI-MS)、纳升电喷雾电离串联质谱(NanoESI-MS/MS,中性丢失扫描模式)以及基质辅助激光解吸/电离飞行时间质谱(MALDI-TOFMS)(赖氨酸残基胍基化和未胍基化)对未分级消化物进行乳糖修饰氨基酸残基的特异性鉴定。结果表明,孵育8.25小时后,赖氨酸残基是乳糖诱导修饰的主要靶点。除了15个赖氨酸残基外,还发现Leu1(氨基末端)和Arg124也被修饰,从而导致总共17个不同的修饰氨基酸残基(与LC/ESI-MS测量发现的15个相比)。在第二组实验中,比较了由恒定中性丢失和前体离子扫描组成的不同策略,以表征半乳糖诱导的修饰。由于β-Lg糖化水平较高,在孵育8.25小时后,似乎需要联合使用这些不同策略来确定半乳糖修饰位点。因此,从LC/ESI-MS测量推断出的22个半乳糖加合物中,除了N末端和经典的赖氨酸残基外,我们还观察到一些精氨酸残基(Arg40、Arg124和Arg148)被修饰,以及特定赖氨酸残基(Lys47、Lys75)上的二烷基化。

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