Direct Imaging of Protein-Specific Methylation in Mammalian Cells

被引:5
|
作者
Doll, Franziska [1 ,2 ]
Steimbach, Raphael R. [1 ]
Zumbusch, Andreas [1 ,2 ]
机构
[1] Univ Konstanz, Dept Chem, Univ Str 10, D-78457 Constance, Germany
[2] Konstanz Res Sch Chem Biol, Univ Str 10, D-78457 Constance, Germany
关键词
fluorescence; FRET; methylation; proteins; protein modifications; FOXO TRANSCRIPTION FACTORS; HISTONE METHYLATION; ARGININE METHYLATION; ADOMET ANALOG; VISUALIZATION; MARK;
D O I
10.1002/cbic.201800787
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Abundant post-translational modification through methylation alters the function, stability, and/or localization of a protein. Malfunctions in post-translational modification are associated with severe diseases. To unravel protein methylation sites and their biological functions, chemical methylation reporters have been developed. However, until now, their usage was limited to cell lysates. Herein, we present the first generally applicable approach for imaging methylation of individual proteins in human cells, which is based on a combination of chemical reporter strategies, bioorthogonal ligation reactions, and FRET detected by means of fluorescence lifetime imaging microscopy. Through this approach, methylation of histone 4 and the non-histone proteins tumor suppressor p53, kinase Akt1, and transcription factor Foxo1 in two human cell lines has been successfully imaged. To further demonstrate its potential, the localization-dependent methylation state of Foxo1 in the cellular context has been visualized.
引用
收藏
页码:1315 / 1325
页数:11
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