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Determination of selenocysteine and selenomethionine in edible animal tissues by 2D size-exclusion reversed-phase HPLC-ICP MS following carbamidomethylation and proteolytic extraction

机译:氨基甲酰甲基化和蛋白水解萃取后的二维尺寸排阻反相HPLC-ICP MS测定食用动物组织中的硒代半胱氨酸和硒代蛋氨酸

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摘要

A method was developed for the simultaneous determination of selenomethionine (SeMet) and selenocysteine (SeCys) in meat (chicken and lamb muscles) and different offal tissues (heart, liver, kidney). The analytical procedure was based on the protein extraction with urea under reducing conditions (dithiothreitol), derivatization of SeCys and SeMet by carbamidomethylation with iodoacetamide (IAM) followed by quantitative proteolysis. The mixture of the derivatized Se-amino acids was purified by size-exclusion liquid chromatography (LC) and analysed by ion-paring reversed-phase HPLC–inductively coupled plasma mass spectroscopy (ICP MS). The quantification of SeCys and SeMet was carried out by the method of standard additions. 77SeMet was used to control the SeMet derivatization efficiency and recovery. The method was validated by the determination of the Se mass balance. The Se-amino acids accounted for 91 ± 8% of the total selenium (mean of 95 samples of seven tissues analysed over a period of 18 months). The method was applied to the discrimination of the contribution of selenoproteins (containing SeCys) and other Se-containing proteins (containing SeMet) in tissues of animals during supplementation studies (dose–effect and tolerance).
机译:开发了一种同时测定肉(鸡和羔羊肌肉)和不同内脏组织(心脏,肝脏,肾脏)中硒代蛋氨酸(SeMet)和硒代半胱氨酸(SeCys)的方法。该分析程序基于以下条件:在还原条件下用尿素(二硫苏糖醇)提取蛋白质,通过碘乙酰胺(IAM)的氨基甲酰甲基化将SeCys和SeMet衍生化,然后进行定量蛋白水解。通过尺寸排阻液相色谱(LC)纯化衍生化的Se-氨基酸混合物,并通过离子对反相HPLC-电感耦合等离子体质谱(ICP MS)分析。 SeCys和SeMet的定量通过标准添加方法进行。 77 SeMet用于控制SeMet的衍生效率和回收率。通过测定硒质量平衡验证了该方法。硒氨基酸占总硒的91±8%(在18个月的时间内分析了七个组织的95个样品的平均值)。该方法适用于在补充研究(剂量效果和耐受性)中区分动物组织中的硒蛋白(含SeCys)和其他含硒蛋白(含SeMet)的作用。

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