The tobacco PK12 is induced by the plant hormone ethylene and is a member o
f the LAMMER family of protein kinases. Members of this family contain in t
heir C-terminus a unique 'EHLAMMERI/VLGPLP' motif of unknown function, and
are related to cyclin- and mitogen-activated protein (MAP)-dependent kinase
s. The animal members of this class play a role in differentiation. They ph
osphorylate and physically interact with serine/arginine-rich (SR) splicing
factors in vivo to alter their activity and the splicing of target mRNAs.
SR proteins have been recently described in plants. The capability of PK12
LAMMER kinase to bind and phosphorylate SR proteins was tested in vitro by
kinase and binding assays. The tobacco PK12 phosphorylated both animal and
plant SR proteins and specifically interacted with the plant splicing facto
r atSRp34/SR1. In addition, by site-directed mutagenesis, the LAMMER motif
was found to be required for PK12 kinase activity but was not necessary for
substrate binding. Consistent with a role in phosphorylation of splicing f
actors, PK12 was found to localize to the nucleus when transiently over-exp
ressed in suspension cells.