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Quantitative profiling of differentiation-induced microsomal proteins using isotope-coded affinity tags and mass spectrometry

机译:使用同位素编码的亲和标签和质谱对分化诱导的微粒体蛋白进行定量分析

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摘要

An approach to the systematic identification and quantification of the proteins contained in the microsomal fraction of cells is described. It consists of three steps: (1) preparation of microsomal fractions from cells or tissues representing different states; (2) covalent tagging of the proteins with isotope-coded affinity tag (ICAT) reagents followed by proteolysis of the combined labeled protein samples; and (3) isolation, identification, and quantification of the tagged peptides by multidimensional chromatography, automated tandem mass spectrometry, and computational analysis of the obtained data. The method was used to identify and determine the ratios of abundance of each of 491 proteins contained in the microsomal fractions of naïve and in vitro–differentiated human myeloid leukemia (HL-60) cells. The method and the new software tools to support it are well suited to the large-scale, quantitative analysis of membrane proteins and other classes of proteins that have been refractory to standard proteomics technology.
机译:描述了一种系统鉴定和定量细胞微粒体级分中所含蛋白质的方法。它包括三个步骤:(1)从代表不同状态的细胞或组织中制备微粒体级分; (2)用同位素编码的亲和标签(ICAT)试剂共价标记蛋白质,然后对合并的标记蛋白质样品进行蛋白水解; (3)通过多维色谱法,自动串联质谱法和获得的数据的计算分析来分离,鉴定和定量标记的肽。该方法用于鉴定和测定幼稚和体外分化的人类骨髓性白血病(HL-60)细胞微粒体级分中所含491种蛋白质的丰度比。该方法和支持它的新软件工具非常适合大规模,定量分析膜蛋白和对标准蛋白质组学技术无能为力的其他类型的蛋白。

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