Posttranslational Modifications of the 5′-AMP-activated Protein Kinase β1 Subunit

Abstract The AMP-activated protein kinase (AMPK) consists of catalytic α and noncatalytic β and γ subunits and is responsible for acting as a metabolic sensor for AMP levels. There are multiple genes for each subunit and the rat liver AMPK α1 and α2 catalytic subunits are associated with β1 and γ1 noncatalytic subunits. We find that the isolated γ1 subunit is N-terminally acetylated with no other posttranslational modification. The isolated β1 subunit is N-terminally myristoylated. Transfection of COS cells with AMPK subunit cDNAs containing a nonmyristoylatable β1 reduces, but does not eliminate, membrane binding of AMPK heterotrimer. The isolated β1subunit is partially phosphorylated at three sites, Ser24/25, Ser182, and Ser108. The Ser24/25 and Ser108 sites are substoichiometrically phosphorylated and can be autophosphorylatedin vitro. The Ser-Pro site in the sequence LSSS182PPGP is stoichiometrically phosphorylated, and no additional phosphate is incorporated into this site with autophosphorylation. Based on labeling studies in transfected cells, we conclude that α1 Thr172 is a major, although not exclusive, site of both basal and stimulated α1phosphorylation by an upstream AMPK kinase.