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Quantitative proteomic analysis using a MALDI quadrupole time-of-flightmass spectrometer

机译:使用MALDI四极杆飞行时间质谱仪进行蛋白质组学定量分析

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We describe an approach to the quantitative analysis of complex protein mixtures using a MALDI quadrupole time-of-flight (MALDI QqTOF) mass spectrometer and isotope coded affinity tag reagents (Gygi, S, P,; et al. Naf. Biotechnol. 1999, 17, 994-9.). Proteins in mixtures are first labeled on cysteinyl residues using an isotope coded affinity tag reagent, the proteins are enzymatically digested, and the labeled peptides are purified using a multidimensional separation procedure, with the last step being the elution of the labeled peptides from a microcapillary reversed-phase liquid chromatography column directly onto a MALDI sample target. After addition of matrix, the sample spots are analyzed using a MALDI QqTOF mass spectrometer, by first obtaining a mass spectrum of the peptides in each sample spot in order to quantify the ratio of abundance of pairs of isotopically tagged peptides, followed by tandem mass spectrometric analysis to ascertain the sequence of selected peptides for protein identification, an, effectiveness of this approach is demonstrated in the quantification and identification of peptides from a control mixture of proteins of known relative concentrations and also in the comparative analysis of protein expression in Saccharomyces cerevisiae grown on two different carbon sources.
机译:我们描述了一种使用MALDI四极杆飞行时间(MALDI QqTOF)质谱仪和同位素编码的亲和标签试剂对复杂蛋白质混合物进行定量分析的方法(Gygi,S,P等; Naf。Biotechnol。1999, 17,994-9。)。首先使用同位素编码的亲和标签试剂将混合物中的蛋白质标记在半胱氨酸残基上,然后酶切消化蛋白质,然后使用多维分离程序纯化标记的肽,最后一步是从微毛细管反向洗脱洗脱标记的肽相液相色谱柱直接连接到MALDI样品目标上。加入基质后,使用MALDI QqTOF质谱仪分析样品斑点,方法是首先获得每个样品斑点中肽段的质谱图,以便定量同位素标记的肽对的丰度比,然后进行串联质谱分析分析以确定用于蛋白质鉴定的选定肽的序列,这种方法的有效性在从已知相对浓度的蛋白质对照混合物中定量和鉴定肽以及在酿酒酵母中蛋白质表达的比较分析中得到证明在两种不同的碳源上

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