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A Quantitative Chemical Proteomics Approach for Site-specific Stoichiometry Analysis of Ubiquitination

机译:一种定量化学蛋白质组学方法,用于泛素化的特异性化学化学计量分析

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摘要

Stoichiometric analysis of post-translational modifications is an emerging strategy for absolute quantification of the fractional abundance of the modification. Herein, a quantitative chemical proteomic workflow for stoichiometric analysis of ubiquitination is reported, named isotopically balanced quantification of ubiquitination (IBAQ-Ub). The strategy utilizes a new amine-reactive chemical tag (AcGG-NHS) that is structurally homologous to the GG remnant of ubiquitin on modified lysine after trypsin cleavage and therefore enables the generation of structurally identical peptides from ubiquitinated and unmodified lysine residues following trypsin digestion and secondary stable isotopic labeling. The strategy is highly robust, sensitive, and accurate with a wide dynamic range using either protein standards or complex cell lysates. Thus, this work provides an efficient chemical proteomics tool for quantitative stoichiometric analysis of ubiquitination signaling pathways.
机译:转换后修改的化学计量分析是一种新出现的策略,用于绝对量化修饰的分数丰富。 这里,报道了泛素化化化学计量分析的定量化学蛋白质组学工作流程,命名为泛素化的同位素平衡量化(IBAQ-UB)。 该策略利用新的胺 - 反应性化学标签(ACGG-NHS),其在胰蛋白酶切割后的改性赖氨酸上的泛素的GG残余物在结构上同源,因此能够在胰蛋白酶消化后产生从普适染发剂和未改性的赖氨酸残基的结构上相同的肽。 二次稳定同位素标记。 该策略具有高度稳健,敏感,并且使用蛋白质标准或复杂的细胞裂解物的宽动态范围。 因此,这项工作为泛素线信号传导途径进行了有效的化学蛋白质组学工具,用于定量化学计量分析。

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