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通过选择性邻近蛋白质组学对活细胞中的细胞质信号复合物进行时空分析。

Spatiotemporal profiling of cytosolic signaling complexes in living cells by selective proximity proteomics.

机构信息

Department of Chemistry, School of Science, Southern University of Science and Technology, Shenzhen, China.

Molecular and Cell Biology Laboratory, Salk Institute for Biological Studies, La Jolla, CA, USA.

出版信息

Nat Commun. 2021 Jan 4;12(1):71. doi: 10.1038/s41467-020-20367-x.

Abstract

Signaling complexes are often organized in a spatiotemporal manner and on a minute timescale. Proximity labeling based on engineered ascorbate peroxidase APEX2 pioneered in situ capture of spatiotemporal membrane protein complexes in living cells, but its application to cytosolic proteins remains limited due to the high labeling background. Here, we develop proximity labeling probes with increased labeling selectivity. These probes, in combination with label-free quantitative proteomics, allow exploring cytosolic protein assemblies such as phosphotyrosine-mediated protein complexes formed in response to minute-scale EGF stimulation. As proof-of-concept, we systematically profile the spatiotemporal interactome of the EGFR signaling component STS1. For STS1 core complexes, our proximity proteomics approach shows comparable performance to affinity purification-mass spectrometry-based temporal interactome profiling, while also capturing additional-especially endosomally-located-protein complexes. In summary, we provide a generic approach for exploring the interactome of mobile cytosolic proteins in living cells at a temporal resolution of minutes.

摘要

信号复合物通常在时空上组织,并在微小的时间尺度上进行。基于工程化抗坏血酸过氧化物酶 APEX2 的邻近标记方法开创了在活细胞中捕获时空膜蛋白复合物的原位方法,但由于标记背景较高,其在细胞质蛋白中的应用仍然有限。在这里,我们开发了具有更高标记选择性的邻近标记探针。这些探针与无标记定量蛋白质组学相结合,可用于研究细胞质蛋白组装体,例如对微小尺度 EGF 刺激作出反应而形成的磷酸酪氨酸介导的蛋白质复合物。作为概念验证,我们系统地描绘了 EGFR 信号成分 STS1 的时空相互作用组。对于 STS1 核心复合物,我们的邻近蛋白质组学方法与基于亲和纯化-质谱的时间相互作用组分析具有相当的性能,同时还捕获了其他 - 特别是内体定位 - 蛋白质复合物。总之,我们提供了一种通用的方法,可在微小的时间分辨率下探索活细胞中移动的细胞质蛋白的相互作用组。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/45d1/7782698/92e762e0e62e/41467_2020_20367_Fig1_HTML.jpg

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