Spatially resolved proteomic mapping in living cells with the engineered peroxidase APEX2

细胞培养中氨基酸的稳定同位素标记 生物素化 蛋白质组学 链霉亲和素 化学 生物化学 细胞生物学 细胞室 定量蛋白质组学 蛋白质组 等压标记 计算生物学 生物 生物素 过氧化物酶 细胞 基因
作者
Victoria Hung,Namrata D. Udeshi,Stephanie S Lam,Ken H. Loh,Kurt J. Cox,Kayvon Pedram,Steven A. Carr,Alice Y. Ting
出处
期刊:Nature Protocols [Nature Portfolio]
卷期号:11 (3): 456-475 被引量:512
标识
DOI:10.1038/nprot.2016.018
摘要

In this protocol, Hung et al. describe a method for performing cell compartment–specific proteomics for regions of interest using the engineered ascorbate peroxidase APEX2. This protocol describes a method to obtain spatially resolved proteomic maps of specific compartments within living mammalian cells. An engineered peroxidase, APEX2, is genetically targeted to a cellular region of interest. Upon the addition of hydrogen peroxide for 1 min to cells preloaded with a biotin-phenol substrate, APEX2 generates biotin-phenoxyl radicals that covalently tag proximal endogenous proteins. Cells are then lysed, and biotinylated proteins are enriched with streptavidin beads and identified by mass spectrometry. We describe the generation of an appropriate APEX2 fusion construct, proteomic sample preparation, and mass spectrometric data acquisition and analysis. A two-state stable isotope labeling by amino acids in cell culture (SILAC) protocol is used for proteomic mapping of membrane-enclosed cellular compartments from which APEX2-generated biotin-phenoxyl radicals cannot escape. For mapping of open cellular regions, we instead use a 'ratiometric' three-state SILAC protocol for high spatial specificity. Isotopic labeling of proteins takes 5–7 cell doublings. Generation of the biotinylated proteomic sample takes 1 d, acquiring the mass spectrometric data takes 2–5 d and analysis of the data to obtain the final proteomic list takes 1 week.
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