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A fast and efficient method for quantitative measurement of S-adenosyl-l-methionine-dependent methyltransferase activity with protein substrates.

Anal Biochem.. 2010-03;  398(2):218-24
Suh-Lailam BB, Hevel JM. a Department of Chemistry and Biochemistry, Utah State University, Logan, UT 84322, USAb Center for Integrated Biosystems, Utah State University, Logan, UT 84322, USA
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摘要

Modification of protein residues by S-adenosyl-l-methionine (AdoMet)-dependent methyltransferases impacts an array of cellular processes. Here we describe a new approach to quantitatively measure the rate of methyl transfer that is compatible with using protein substrates. The method relies on the ability of reverse-phase resin packed at the end of a pipette tip to quickly separate unreacted AdoMet from radiolabeled protein products. Bound radiolabeled protein products are eluted directly into scintillation vials and counted. In addition to decreasing analysis time, the sensitivity of this protocol allows the determination of initial rate data. The utility of this protocol was shown by generating a Michaelis&nd... More

关键词

S-adenosyl-methionine; AdoMet; SAM; Methyltransferase; PRMT; PKMT; Protein arginine methylation; Protein lysine methylation; Kinetics; Quantification of methyltransfer; Kinetic assay
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