Robust Fluorescent Detection of Protein Fatty-Acylation with Chemical Reporters

被引:246
|
作者
Charron, Guillaume [1 ]
Zhang, Mingzi M. [1 ]
Yount, Jacob S. [1 ]
Wilson, John [1 ]
Raghavan, Anuradha S. [1 ]
Shamir, Eliah [1 ]
Hang, Howard C. [1 ]
机构
[1] Rockefeller Univ, Lab Chem Biol & Microbial Pathogenesis, New York, NY 10065 USA
关键词
COPPER(I)-CATALYZED AZIDE-ALKYNE; N-MYRISTOYL TRANSFERASE; IN-VIVO; BOUND MYRISTOYLCOA; RAFT LOCALIZATION; TERMINAL ALKYNES; MAMMALIAN-CELLS; CLICK CHEMISTRY; RAPID DETECTION; WNT PROTEIN;
D O I
10.1021/ja810122f
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
Fatty-acylation of proteins in eukaryotes is associated with many fundamental cellular processes but has been challenging to study due to limited tools for rapid and robust detection of protein fatty-acylation in cells. The development of azido-fatty acids enabled the nonradioactive detection of fatty-acylated proteins in mammalian cells using the Staudinger ligation and biotinylated phosphine reagents. However, the visualization of protein fatty-acylation with streptavidin blotting is highly variable and not ideal for robust detection of fatty-acylated proteins. Here we report the development of alkynyl-fatty acid chemical reporters and improved bioorthogonal labeling conditions using the Cu-I-catalyzed Huisgen [3 + 2] cycloaddition that enables specific and sensitive fluorescence detection of fatty-acylated proteins in mammalian cells. These improvements allow the rapid and robust biochemical analysis of fatty-acylated proteins expressed at endogenous levels in mammalian cells by in-gel fluorescence scanning. In addition, alkynyl-fatty acid chemical reporters enable the visualization of fatty-acylated proteins in cells by fluorescence microscopy and flow cytometry. The ability to rapidly visualize protein fatty-acylation in cells using fluorescence detection methods therefore provides new opportunities to interrogate the functions and regulatory mechanisms of fatty-acylated proteins in physiology and disease.
引用
收藏
页码:4967 / 4975
页数:9
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