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首页> 外文期刊>Journal of proteomics >Determination of Cystatin C in human serum by isotope dilution mass spectrometry using mass overlapping peptides
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Determination of Cystatin C in human serum by isotope dilution mass spectrometry using mass overlapping peptides

机译:同位素稀释质谱法用质量重叠肽测定人血清中胱抑素C.

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We propose a peptide-based isotope dilution mass spectrometry approach for Cystatin C determination in human serum samples, a clinical marker for renal status for which backup by a mass spectrometry based primary method has been missing so far. In contrast to common protocols, the isotope labelled version of the proteotypic signature peptide is designed such as keeping the isotopic difference as little as possible with respect to the peptide released from the protein. Peptides labelled in two C-13 atoms are added to the serum samples just before proteolysis. After two steps of chromatographic purification the sample is measured by selected reaction monitoring using a LC-MS/MS. Resolution of the first quadrupole is reduced to transmit the whole parent ion cluster to the collision cell for monitoring accurate isotopic distributions of the molecular fragments. Molar fractions of labelled and natural abundance peptides are directly obtained from the experimental mass spectra of the in-cell fragment ions. Thus, the natural abundance protein concentration is obtained from the fragment-ion spectrum of the sample without resorting to extra calibration runs. Applicability of the approach is demonstrated by the measurement of the serum concentration of Cystatin C in Reference Material ERM R-DA471/IFCC and real samples.
机译:我们提出了一种基于肽的同位素稀释质谱法,用于人血清样品中的胱抑素C测定,缺少基于质谱的主要方法的肾脏状态的肾脏状况的临床标志物。与常见方案相比,设计了蛋白质型特征肽的同位素标记的版本,例如,保持同位素差异尽可能少地相对于蛋白质释放的肽。在蛋白水解之前,在两个C-13原子中标记的肽在血清样品中加入到血清样品中。经过两步的色谱柱纯化,通过使用LC-MS / MS选择的反应监测来测量样品。将第一四轴的分辨率降低以将整个母体离子聚类传递给碰撞细胞以监测分子片段的精确同位素分布。标记和天然丰度肽的摩尔级分直接从细胞片段离子离子离子的实验质谱中获得。因此,自然丰度蛋白质浓度是从样品的片段 - 离子光谱获得,而不借助额外的校准运行。通过测量参考资料ERM R-DA471 / IFCC和真实样品的胱抑素C的血清浓度来证明该方法的适用性。

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