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通过TransitID对活细胞内和细胞间蛋白质组运输进行动态映射。

Dynamic mapping of proteome trafficking within and between living cells by TransitID.

作者信息

Xu Wei Qin, Cheah Joleen S, Xu Charles, Messing James, Freibaum Brian D, Boeynaems Steven, Taylor J Paul, Udeshi Namrata D, Carr Steven A, Ting Alice Y

出版信息

bioRxiv. 2023 Feb 8:2023.02.07.527548. doi: 10.1101/2023.02.07.527548.

Abstract

The ability to map trafficking for thousands of endogenous proteins at once in living cells would reveal biology currently invisible to both microscopy and mass spectrometry. Here we report TransitID, a method for unbiased mapping of endogenous proteome trafficking with nanometer spatial resolution in living cells. Two proximity labeling (PL) enzymes, TurboID and APEX, are targeted to source and destination compartments, and PL with each enzyme is performed in tandem via sequential addition of their small-molecule substrates. Mass spectrometry identifies the proteins tagged by both enzymes. Using TransitID, we mapped proteome trafficking between cytosol and mitochondria, cytosol and nucleus, and nucleolus and stress granules, uncovering a role for stress granules in protecting the transcription factor JUN from oxidative stress. TransitID also identifies proteins that signal intercellularly between macrophages and cancer cells. TransitID introduces a powerful approach for distinguishing protein populations based on compartment or cell type of origin.

摘要

能够在活细胞中一次性对数千种内源性蛋白质的运输进行映射,将揭示目前显微镜和质谱技术都无法看到的生物学现象。在此,我们报告了TransitID,一种在活细胞中以纳米空间分辨率对内源性蛋白质组运输进行无偏映射的方法。两种邻近标记(PL)酶,TurboID和APEX,被靶向到源区室和目的区室,并且通过依次添加它们的小分子底物,对每种酶进行串联PL。质谱法鉴定由两种酶标记的蛋白质。使用TransitID,我们绘制了蛋白质组在细胞质和线粒体、细胞质和细胞核以及核仁与应激颗粒之间的运输图谱,揭示了应激颗粒在保护转录因子JUN免受氧化应激方面的作用。TransitID还鉴定了在巨噬细胞和癌细胞之间进行细胞间信号传导的蛋白质。TransitID引入了一种强大的方法,可根据蛋白质的来源区室或细胞类型来区分蛋白质群体。

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