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Papers In Press, published online ahead of print May 27, 2005
J. Biol. Chem, 10.1074/jbc.M414017200
Submitted on December 14, 2004
Accepted on May 27, 2005

Cross-species sequence analysis reveals multiple charged residue-rich domains that regulate nuclear/cytoplasmic partitioning and membrane localization of AKAP 12 (SSeCKS/Gravin)

Jeffrey W. Streb and Joseph M. Miano

Department of Medicine, University of Rochester, Rochester, NY 14642

Corresponding Author: j.m.miano{at}rochester.edu

A Kinase Anchoring Proteins (AKAP) assemble and compartmentalize multiprotein signaling complexes at discrete subcellular locales and thus confer specificity to transduction cascades using ubiquitous signaling enzymes, such as PKA. Intrinsic targeting domains in each AKAP determine the subcellular localization of these complexes and, along with protein-protein interaction domains, are the core of AKAP function. As a foundational step towards elucidating the relationship between location and function, we have used cross-species sequence analysis and deletion mapping to facilitate the identification of the targeting determinants of AKAP12 (also known as SSeCKS or Gravin). Three charged residue-rich regions were identified that regulate two aspects of AKAP12 localization: nuclear/cytoplasmic partitioning and perinuclear/cell periphery targeting. Using deletion mapping and GFP chimeras, we uncovered a heretofore unrecognized nuclear localization potential. Five nuclear localization signals, including a novel class of NLS, are found in the central region of AKAP12 and are important for nuclear targeting. However, this nuclear localization is suppressed by the negatively charge C-terminus that mediates nuclear exclusion. In this condition, the distribution of AKAP12 is regulated by an N-terminal targeting domain that simultaneously directs perinuclear and peripheral AKAP12 localization. Three basic residue-rich regions in the N-terminal targeting region have similarity to the MARCKS proteins and were found to control AKAP12 localization to ganglioside-rich regions at the cell periphery. Our data suggest that AKAP12 localization is regulated by a hierarchy of targeting domains and that the localization of AKAP12-assembled signaling complexes may be dynamically regulated.


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