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用丙二酸二乙酯乙氧基甲基烯酸酯衍生化后,采用高效液相色谱法测定生物样品中的N-ε-(2-丙烯醛)赖氨酸。

High-performance liquid chromatographic determination of N-epsilon-(2-propenal)lysine in biological samples after derivatization with diethylethoxymethylenemalonate.

作者信息

Girón J, Alaiz M, Vioque E

机构信息

Instituto de la Grasa y sus Derivados (CSIC), Seville, Spain.

出版信息

Anal Biochem. 1992 Oct;206(1):155-60. doi: 10.1016/s0003-2697(05)80026-0.

DOI:10.1016/s0003-2697(05)80026-0
PMID:1456428
Abstract

A recently reported methodology for amino acid analysis by HPLC has been adapted for quantification of N-epsilon-(2-propenal)lysine (a modified lysine by reaction with malondialdehyde that has been found in enzymatic digests of foods and in urine) in biological samples. We describe its use for investigating the in vitro degradation of N-epsilon-(2-propenal)lysine using rat tissue homogenates. Lysine dipeptide, used as a control in the incubation mixtures, and the lysine released by the hydrolytic action of the homogenates in the in vitro incubations are quantified in the same way. The samples are subjected to a cleanup prederivatization step using PD-10 disposable columns (Pharmacia). This allows precolumn derivatization with diethylethoxymethylenemalonate (50 min, 50 degrees C) and resolution of the derivatives of the compounds of interest by reversed-phase HPLC (binary gradient, 45 min) with quantification based on the uv absorption of the derivatives at 280 nm (detection limits below 1 pmol). The entire analysis takes 110 min. This method can be of general use for the determination of N-epsilon-(2-propenal)lysine in the context of research dealing with protein deterioration by reaction with malondialdehyde in biological systems and in foods. A method for the synthesis of N-epsilon-(2-propenal)lysine, used as external standard for the HPLC analysis, is described.

摘要

最近报道的一种通过高效液相色谱法进行氨基酸分析的方法,已被应用于生物样品中N-ε-(2-丙烯醛)赖氨酸(一种通过与丙二醛反应修饰的赖氨酸,已在食物的酶消化物和尿液中发现)的定量分析。我们描述了其在使用大鼠组织匀浆研究N-ε-(2-丙烯醛)赖氨酸体外降解中的应用。在孵育混合物中用作对照的赖氨酸二肽,以及在体外孵育中由匀浆的水解作用释放的赖氨酸,以相同方式进行定量分析。样品使用PD-10一次性柱(Pharmacia)进行净化前衍生化步骤。这允许用丙二酸二乙酯乙氧基甲基酯进行柱前衍生化(50分钟,50℃),并通过反相高效液相色谱法(二元梯度,45分钟)分离目标化合物的衍生物,基于衍生物在280nm处的紫外吸收进行定量分析(检测限低于1皮摩尔)。整个分析过程耗时110分钟。该方法可普遍用于在研究生物系统和食物中蛋白质与丙二醛反应导致的变质情况下测定N-ε-(2-丙烯醛)赖氨酸。本文还描述了一种用作高效液相色谱分析外标的N-ε-(2-丙烯醛)赖氨酸的合成方法。

相似文献

1
High-performance liquid chromatographic determination of N-epsilon-(2-propenal)lysine in biological samples after derivatization with diethylethoxymethylenemalonate.用丙二酸二乙酯乙氧基甲基烯酸酯衍生化后,采用高效液相色谱法测定生物样品中的N-ε-(2-丙烯醛)赖氨酸。
Anal Biochem. 1992 Oct;206(1):155-60. doi: 10.1016/s0003-2697(05)80026-0.
2
Identification of N-epsilon-(2-propenal)lysine as a major urinary metabolite of malondialdehyde.鉴定N-ε-(2-丙烯醛)赖氨酸为丙二醛的主要尿液代谢产物。
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Identification of N-epsilon-(2-propenal)lysine as the main form of malondialdehyde in food digesta.鉴定N-ε-(2-丙烯醛)赖氨酸为食物消化物中丙二醛的主要形式。
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Protein modification by lipid peroxidation products: formation of malondialdehyde-derived N(epsilon)-(2-propenol)lysine in proteins.脂质过氧化产物对蛋白质的修饰:蛋白质中丙二醛衍生的N(ε)-(2-丙烯醇)赖氨酸的形成。
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