Non-radioactive Protein Lysine Methyltransferase Microplate Assay Based on Reading Domains

被引:8
|
作者
Kudithipudi, Srikanth [1 ]
Kusevic, Denis [1 ]
Jeltsch, Albert [1 ]
机构
[1] Univ Stuttgart, Inst Biochem, D-70569 Stuttgart, Germany
关键词
enzyme assays; high-throughput screening; inhibitors; protein lysine methylation; ADENOSYLMETHIONINE-DEPENDENT METHYLTRANSFERASES; SMALL-MOLECULE INHIBITOR; B-CELL LYMPHOMAS; HISTONE H3; CHROMATIN-STRUCTURE; SOMATIC MUTATIONS; STRUCTURAL BASIS; METHYLATION; EZH2; G9A;
D O I
10.1002/cmdc.201300111
中图分类号
R914 [药物化学];
学科分类号
100701 ;
摘要
New protein lysine methyltransferase (PKMT) assays are needed to facilitate screening for improved PKMT inhibitors, because PKMTs are mutated or overexpressed in several cancers. In cells, methylated lysine residues are recognized by reading domains such as the chromodomain of HP1, which bind to target proteins in a lysine-methylation-specific manner. Herein we describe a sensitive, robust, and non-radioactive high-throughput PKMT assay that employs the HP1 chromodomain to detect the methylation of peptide substrates by the human SUV39H1 and SUV39H2 PKMTs. The assay has a very good dynamic range and high signal-to-noise ratio. It can be used to screen for PKMT inhibitors, as illustrated by analyzing the inhibition of SUV39H1 by chaetocin. The IC50 value of this inhibition was found to be 480nM, which is close to its published value. Our data indicate that natural reading domains can be used as alternates to methyl-specific antibodies in PKMT assays. Reading domains can be produced recombinantly in E.coli at low cost and consistent quality, and they are accessible to protein design.
引用
收藏
页码:554 / 559
页数:6
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