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通过质谱分析全面表征胰岛素受体磷酸化动力学

Comprehensive insulin receptor phosphorylation dynamics profiled by mass spectrometry.

作者信息

Liao Zhongping, Zhang Chen, Ding Liyun, Moyers Julie S, Tang Jason X, Beals John M

机构信息

Lilly Research Laboratories, Eli Lilly and Company, Lilly Corporate Center, Indianapolis, IN, USA.

出版信息

FEBS J. 2022 May;289(9):2657-2671. doi: 10.1111/febs.16299. Epub 2021 Dec 13.

DOI:10.1111/febs.16299
PMID:34826178
Abstract

Insulin receptor (IR) phosphorylation is critical for the assessment of the extent of IR agonism and nuances in the downstream signaling cascade. A thorough identification and monitoring of the phosphorylation events is important for understanding the process of insulin signaling transduction and regulation. Although IR phosphorylation has been studied extensively in the past decades, only a handful of phosphorylation sites can be identified by either traditional antibody-based assays or recent large-scale mass spectrometry-based phosphoproteomics approaches. In the present study, the most exhaustive assessment of the IR phosphorylation was conducted using nano-liquid chromatography-tandem mass spectrometry, in which 13 IR phosphorylation sites and 22 combinations thereof were analyzed. The kinetic analysis included Y965, Y972, S968/969, and S974/976 in the juxtamembrane region; Y1158, Y1162, and Y1163 in the kinase domain; and Y1328, Y1334, S1278, S1320, S1321, and T1348 in the C-terminal region. Employing two different receptor agonists (i.e. insulin and an IR peptide agonist), the data revealed contrasting phosphorylation kinetics across these sites with dynamics far more diverse than expected for known IR agonists. Notably, cell trafficking experiments revealed that the IR peptide agonist was incapable of inducing IR to the early endosome, which is probably linked to a difference in IR phosphorylation. The present study provides a powerful tool for investigating IR signaling and trafficking that will benefit the design of IR agonists with improved therapeutic utility.

摘要

胰岛素受体(IR)磷酸化对于评估IR激动程度及下游信号级联反应中的细微差别至关重要。全面识别和监测磷酸化事件对于理解胰岛素信号转导和调节过程很重要。尽管在过去几十年中对IR磷酸化进行了广泛研究,但通过传统的基于抗体的检测方法或最近基于大规模质谱的磷酸蛋白质组学方法,只能鉴定出少数几个磷酸化位点。在本研究中,使用纳升液相色谱-串联质谱对IR磷酸化进行了最详尽的评估,分析了13个IR磷酸化位点及其22种组合。动力学分析包括近膜区域的Y965、Y972、S968/969和S974/976;激酶结构域的Y1158、Y1162和Y1163;以及C末端区域的Y1328、Y1334、S1278、S1320、S1321和T1348。使用两种不同的受体激动剂(即胰岛素和一种IR肽激动剂),数据显示这些位点的磷酸化动力学存在差异,其动态变化远比已知IR激动剂预期的更为多样。值得注意的是,细胞转运实验表明,IR肽激动剂无法将IR诱导至早期内体,这可能与IR磷酸化的差异有关。本研究为研究IR信号传导和转运提供了一个强大的工具,这将有利于设计具有更高治疗效用的IR激动剂。

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