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A new method for quantitative analysis of cell surface glycoproteome

机译:a new method for quantitative analysis of cell surface glycoproteome

摘要

As the altered glycosylation expressions of cell surface proteins are associated with many diseases, glycoproteomics approach has been widely applied to characterization of surface glycosylation alteration. In general, the abundances of proteolytic glycopeptides derived from corresponding glycoproteins can be measured to determine the abundances of glycoproteins. However, this quantification strategy cannot distinguish whether the changes are results from changes of protein abundance or changes in glycosite occupancy. For the accurate and specific quantification of the cell surface glycosylation profile, we proposed a modified cell surface-capturing strategy where the glycopeptides were submitted to LC-MS/MS analysis directly for identification of glycoproteins and the non-glycopeptides were isotopically labelled for quantification of glycoproteins. This strategy was applied to comparatively analyze cell surface glycoproteins of two human cell lines, i.e. Chang Liver and HepG2 cells. Totally 341 glycoproteins were identified with 82.4% specificity for cell membrane proteins and 33 glycoproteins were quantified with significant expression change between the two cell lines. The differential expressions of two selected proteins (EMMPRIN and BCAM) were validated by Western blotting. This method enables specific and accurate analysis of the cell surface glycoproteins and may have broad application in the field of biomarker and drug target discovery.
机译:由于细胞表面蛋白糖基化表达的改变与许多疾病有关,糖蛋白组学方法已被广泛应用于表征表面糖基化改变。通常,可以测量衍生自相应糖蛋白的蛋白水解糖肽的丰度,以确定糖蛋白的丰度。但是,这种量化策略无法区分这些变化是蛋白质丰度变化还是糖位占有率变化造成的。为了准确,特异性地定量细胞表面糖基化谱,我们提出了一种改进的细胞表面捕获策略,其中将糖肽直接提交LC-MS / MS分析以鉴定糖蛋白,并通过同位素标记非糖肽以定量糖蛋白。该策略被用于比较分析两种人类细胞系,即Chang Liver和HepG2细胞的细胞表面糖蛋白。总共鉴定出341种糖蛋白,对细胞膜蛋白的特异性为82.4%,定量了33种糖蛋白,两种细胞系之间的表达均有明显变化。通过蛋白质印迹验证了两种选择的蛋白质(EMMPRIN和BCAM)的差异表达。该方法能够对细胞表面糖蛋白进行特异性和准确的分析,并可能在生物标志物和药物靶标发现领域中得到广泛应用。

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