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Relative Quantitation of Glycoisoforms of Intact Apolipoprotein C3 in Human Plasma by Liquid Chromatography-High-Resolution Mass Spectrometry

机译:液相色谱-高分辨率质谱法定量测定人血浆中完整载脂蛋白C3糖同工型

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Glycosylation is one of the most important posttranslational modifications to mammalian proteins. Distribution of different glycoisoforms of certain proteins may reflect disease conditions and, therefore, can potentially be utilized as biomarkers. Apolipoprotein C3 (ApoC3) is one of the many plasma glycoproteins extensively studied for association with disease states. ApoC3 exists in three main glycoisoforms, including ApoC3-1 and ApoC3-2, which contain an O-linked carbohydrate moiety consisting of three and four monosaccharide residues, respectively, and ApoC3-0 that lacks the entire glycosylation chain. Changes in the ratio of different glycoisoforms of ApoC3 have been observed in pathological conditions such as kidney disease, liver disease, and diabetes. They may provide important information for diagnosis, prognosis, and evaluation of therapeutic response for metabolic conditions. In this current work, a liquid chromatography(LC)-high-resolution (HR) time-of-flight (TOF) mass spectrometry (MS) method was developed for relative quantitation of different glycoisoforms of intact ApoC3 in human plasma. The samples were processed using a solid-phase extraction (SPE) method and then subjected to LC-full scan HRMS analysis. Isotope peaks for each targeted glycoisoform at two charge states were extracted using a window of 50 mDa and integrated into a chromatographic peak. The peak area ratios of ApoC3-1/ApoC3-0 and ApoC3-2/ApoC3-0 were calculated and evaluated for assay performance. The results indicated that the ratio can be determined with excellent reproducibility in multiple subjects. It has also been observed that the ratios remained constant in plasma exposed to room temperature, freeze-thaw cycles, and long-term frozen storage. The method was applied in preliminary biomarker research of diabetes by analyzing plasma samples collected from normal, prediabetic, and diabetic subjects. Significant differences were revealed in the ApoC3-1/ ApoC3-0 ratio and in the ApoC3-2/ApoC3-0 ratio among the three groups. The workflow of intact protein analysis using full scan HRMS established in this current work can be potentially extended to relative quantitation of other glycosylated proteins. To our best knowledge, this is the first time that a systematic approach of relative quantitation of targeted intact protein glycoisoforms using LC-MS has been established and utilized in biomarker research.
机译:糖基化是哺乳动物蛋白最重要的翻译后修饰之一。某些蛋白质的不同糖同工型的分布可能反映疾病状况,因此有可能被用作生物标记。载脂蛋白C3(ApoC3)是广泛研究与疾病状态相关的众多血浆糖蛋白之一。 ApoC3存在三种主要的糖同工型,包括ApoC3-1和ApoC3-2,它们分别包含由三个和四个单糖残基组成的O-连接的碳水化合物部分,以及缺乏完整糖基化链的ApoC3-0。在诸如肾脏疾病,肝脏疾病和糖尿病的病理状况中已经观察到ApoC3的不同糖同工型的比例的变化。它们可能为代谢状况的诊断,预后和评估治疗反应提供重要信息。在当前的工作中,开发了一种液相色谱(LC)-高分辨率(HR)飞行时间(TOF)质谱(MS)方法,用于相对定量地测定人血浆中完整ApoC3的不同糖型。使用固相萃取(SPE)方法处理样品,然后进行LC全扫描HRMS分析。使用50 mDa的窗口提取处于两个电荷状态的每个目标糖基异构体的同位素峰,并将其整合到色谱峰中。计算ApoC3-1 / ApoC3-0和ApoC3-2 / ApoC3-0的峰面积比,并评估其测定性能。结果表明该比率可以在多个受试者中以优异的再现性确定。还已经观察到,在暴露于室温,冻融循环和长期冷冻保存的血浆中,比率保持恒定。通过分析从正常,糖尿病前期和糖尿病受试者中采集的血浆样本,该方法被用于糖尿病的初步生物标记研究。三组之间的ApoC3-1 / ApoC3-0比率和ApoC3-2 / ApoC3-0比率显示出显着差异。使用本工作中建立的全扫描HRMS进行完整蛋白质分析的工作流程可以潜在地扩展到其他糖基化蛋白质的相对定量。据我们所知,这是首次建立使用LC-MS相对定量靶向完整蛋白质糖同工型的系统方法,并将其用于生物标记研究。

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