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Global protein identification and quantification technology using two-dimensional liquid chromatography nanospray mass spectrometry

机译:使用二维液相色谱纳米喷雾质谱技术进行全球蛋白质鉴定和定量技术

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摘要

A simple and reliable method is described here for the identification and relative quantification of proteins in complex mixtures using two-dimensional liquid chromatography/tandem. mass spectrometry. The method is based on the classical proteomic analysis where proteins are digested with trypsin and the resulting peptides are separated by multidimensional liquid chromatography. The separated peptides are analyzed by tandem mass spectrometry and identified via a database search algorithm such as SEQUEST. The peak areas (integrated ion counts over the peptide elution time) of all identified peptides are calculated, and the relative concentration of each protein is determined by comparing the peak areas of all peptides from that protein in one sample versus those from the other. Using this strategy, we compared the relative level of protein expression of A431 cells (an epidermal cell line) grown in the presence or absence of epidermal growth factor (EGF). Our results are consistent with the published observations of the transient effects of EGF. In addition, the difference in the concentrations of several phosphopeptides determined in our studies suggests the possibility of several new targets involved in the EGF cell-signaling pathway. This global protein identification and quantification technology should prove to be a valuable means for comparing proteomes in biological samples subjected to differential treatments. [References: 18]
机译:本文描述了一种简单可靠的方法,用于使用二维液相色谱/串联法鉴定和定量复杂混合物中的蛋白质。质谱。该方法基于经典的蛋白质组学分析,其中用胰蛋白酶消化蛋白质,然后通过多维液相色谱法分离所得的肽。通过串联质谱分析分离的肽,并通过数据库搜索算法(例如SEQUEST)进行鉴定。计算所有已鉴定肽段的峰面积(肽段洗脱时间内的总离子计数),并通过比较一个样品中该蛋白与其他样品中所有肽的峰面积,确定每种蛋白的相对浓度。使用这种策略,我们比较了在存在或不存在表皮生长因子(EGF)的情况下生长的A431细胞(一种表皮细胞系)的相对蛋白表达水平。我们的结果与EGF的瞬时效应的已发表观察结果一致。此外,在我们的研究中确定的几种磷酸肽浓度的差异表明,EGF细胞信号通路中可能涉及到几个新的靶标。这种全球蛋白质鉴定和定量技术应该被证明是比较经过差异处理的生物样品中蛋白质组的一种有价值的手段。 [参考:18]

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