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Improved Precision of Proteomic Measurements in Immunoprecipitation Based Purifications Using Relative Quantitation

机译:使用相对定量提高基于免疫沉淀纯化的蛋白质组学测量的精度

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摘要

Mass spectrometry coupled immunoprecipitation (MS-IP) studies are useful in identifying and quantitating potential binding partners of a target protein. However, they are often conducted without appropriate loading controls. Western blots are often used to analyze loading controls, yet there are limitations to their usefulness as analytical tools. One remedy for this is the use of selected reaction monitoring (SRM), where the areas under the curve (AUCs) of peptides from a protein of interest can be normalized to those from the constant regions of the immunoglobulins used for the IP. Using this normalization method, significant changes in relative peptide abundance were observed between samples when there appeared to be an unequal load based on immunoglobulin peptide abundance.
机译:质谱耦合免疫沉淀(MS-IP)研究可用于鉴定和定量目标蛋白的潜在结合伴侣。但是,它们通常在没有适当的加载控制的情况下进行。蛋白质印迹法通常用于分析上样对照,但其作为分析工具的实用性受到限制。一种解决方法是使用选择的反应监测(SRM),其中可以将目标蛋白的肽曲线下面积(AUC)标准化为IP免疫球蛋白恒定区的面积。使用这种归一化方法,当基于免疫球蛋白肽丰度的负载似乎不相等时,在样品之间观察到相对肽丰度的显着变化。

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