高通量评估激酶组激活状态。

High-Throughput Assessment of Kinome-wide Activation States.

机构信息

Biomolecular Mass Spectrometry and Proteomics, Bijvoet Center for Biomolecular Research and Utrecht Institute for Pharmaceutical Sciences, Utrecht University, Padualaan 8, 3584 CH Utrecht, the Netherlands; Netherlands Proteomics Center, Padualaan 8, 3584 CH Utrecht, the Netherlands.

Sanquin Research, Department of Molecular and Cellular Hemostasis, Amsterdam, the Netherlands.

出版信息

Cell Syst. 2019 Oct 23;9(4):366-374.e5. doi: 10.1016/j.cels.2019.08.005. Epub 2019 Sep 11.

Abstract

Aberrant kinase activity has been linked to a variety of disorders; however, methods to probe kinase activation states in cells have been lacking. Until now, kinase activity has mainly been deduced from either protein expression or substrate phosphorylation levels. Here, we describe a strategy to directly infer kinase activation through targeted quantification of T-loop phosphorylation, which serves as a critical activation switch in a majority of protein kinases. Combining selective phosphopeptide enrichment with robust targeted mass spectrometry, we provide highly specific assays for 248 peptides, covering 221 phosphosites in the T-loop region of 178 human kinases. Using these assays, we monitored the activation of 63 kinases through 73 T-loop phosphosites across different cell types, primary cells, and patient-derived tissue material. The sensitivity of our assays is highlighted by the reproducible detection of TNF-α-induced RIPK1 activation and the detection of 46 T-loop phosphorylation sites from a breast tumor needle biopsy.

摘要

异常的激酶活性与多种疾病有关;然而,探测细胞中激酶激活状态的方法一直缺乏。到目前为止,激酶活性主要是根据蛋白质表达或底物磷酸化水平来推断的。在这里,我们描述了一种通过靶向定量 T 环磷酸化来直接推断激酶激活的策略,T 环磷酸化是大多数蛋白激酶中的一个关键激活开关。通过选择性磷酸肽富集和强大的靶向质谱分析,我们提供了 248 个肽的高度特异性检测方法,涵盖了 178 个人类激酶 T 环区域中的 221 个磷酸化位点。使用这些检测方法,我们监测了 73 个 T 环磷酸化位点在不同细胞类型、原代细胞和患者来源组织材料中 63 种激酶的激活情况。我们的检测方法具有较高的灵敏度,可重复性地检测到 TNF-α诱导的 RIPK1 激活,并且可以从乳腺肿瘤针活检中检测到 46 个 T 环磷酸化位点。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9814/6838672/2cbde511b7b3/fx1.jpg

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