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Applications of selected reaction monitoring (SRM)-mass spectrometry (MS) for quantitative measurement of signaling pathways

机译:所选反应监测(SRM)-质谱(MS)在信号通路定量测量中的应用

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Quantitative measurement of the major regulatory proteins in signaling networks poses several technical challenges, including low abundance, the presence of post-translational modifications (PTMs), and the lack of suitable affinity detection reagents. Using the innate immune response (IIR) as a model signaling pathway, we illustrate the approach of stable isotope dilution (SID)-selected reaction monitoring (SRM)-mass spectrometry (MS) assays for quantification of low abundance signaling proteins. A work flow for SID-SRM-MS assay development is established for proteins with experimentally observed MS spectra and for those without. Using the interferon response factor (IRF)-3 transcription factor as an example, we illustrate the steps in high responding signature peptide identification, SID-SRM-MS assay optimization, and evaluation. SRM assays for normalization of IIR abundance to invariant housekeeping proteins are presented. We provide an example of SID-SRM assay development for post-translational modification (PTM) detection using an activating phospho-Ser modified NF-κB/RelA transcription factor, and describe challenges inherent in PTM-SID-SRM-MS assay development. Application of highly qualified quantitative, SID-SRM-MS assays will enable a systems-level approach to understanding the dynamics and kinetics of signaling in host cells, such as the IIR.
机译:信号网络中主要调节蛋白的定量测定带来了一些技术挑战,包括低丰度,翻译后修饰(PTM)的存在以及缺乏合适的亲和力检测试剂。使用先天免疫应答(IIR)作为模型信号传导途径,我们阐明了稳定同位素稀释(SID)选择反应监测(SRM)质谱(MS)分析法对低丰度信号蛋白定量的方法。针对具有实验观察到的MS光谱的蛋白质和没有实验观察到的MS光谱的蛋白质,建立了SID-SRM-MS分析开发的工作流程。以干扰素反应因子(IRF)-3转录因子为例,我们说明了高响应特征肽鉴定,SID-SRM-MS分析优化和评估中的步骤。提出了将IIR丰度标准化为不变管家蛋白的SRM分析方法。我们提供了使用激活的磷酸化Ser修饰的NF-κB/ RelA转录因子进行翻译后修饰(PTM)检测的SID-SRM分析开发的示例,并描述了PTM-SID-SRM-MS分析开发固有的挑战。高质量定量SID-SRM-MS分析的应用将使系统级方法能够理解宿主细胞(如IIR)中信号传导的动力学和动力学。

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