Methylated C-terminal leucine residue of PP2A catalytic subunit is important for binding of regulatory Bα subunit

Methylation of the C-terminal leucine residue (Leu(309)) of protein serine/threonine phosphatase 2A catalytic subunit (PP2A(c)) is known to regulate catalytic activity in vitro, but the functional consequence(s) of this post-translational modification in the context of the cell remain unclear. Alkali-induced demethylation of PP2A(c) in purified PP2A heterotrimer (AB alpha C), but not in purified PP2A heterodimer (AC), indicated that a larger fraction of PP2A, is carboxymethylated in ABaC than in AC. To explore the role of Leu(309) in PP2A holoenzyme assembly, epitope-tagged PP2A catalytic subunit (HA-PP2A) and a mutant of IIA-PP,A containing an alanine residue in place of Leu309 (HA-PP2A-L309A) were transiently expressed in COS cells. Both recombinant proteins exhibited serine/threonine phosphatase activity when immunoisolated from COS cell extracts. HA-PP2A, but not HA-PP2A-L309A, was carboxymethylated ii? vitro. A chromatographic analysis of cell extracts indicated that most endogenous PP2A(c) and HA-PP2A were co-eluted with the A and Ba regulatory subunits of PP2A, whereas most HA-PP2A-L309A seemed to elute with the A subunit as a smaller complex or, alternatively, as free catalytic (C) subunit. The A subunit co-immunoisolated with both tagged proteins; however, substantially less B alpha subunit co-immunoisolated with HA-PP2A-L309A than with HA-PP2A. These results demonstrate that the reversibly methylated C-terminal leucine residue of PP2A, is important for B alpha regulatory subunit binding. Furthermore, the results provide evidence for an interrelationship between PP2A(c), carboxymethylation and PP2A holoenzyme assembly.