Characterization of structural features that mediate the tethering of Caenorhabditis elegans protein kinase A to a novel A kinase anchor protein -: Insights into the anchoring of PKAI isoforms

被引:31
作者
Angelo, RG [1 ]
Rubin, CS [1 ]
机构
[1] Yeshiva Univ Albert Einstein Coll Med, Dept Mol Pharmacol, Atran Labs, Bronx, NY 10461 USA
关键词
D O I
10.1074/jbc.275.6.4351
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Caenorhabditis elegans protein kinase A (PKAI(CE)) is tethered to organelles in vivo. A unique A kinase anchor protein (AKAP(CE)) avidly binds the RI-like regulatory subunits (R-CE) of PKAI(CE) and stringently discriminates against RII alpha and RII beta subunits, the preferred ligands for classical AKAPs, We elucidated structural features that stabilize AKAP(CE).R-CE complexes and confer atypical R isoform specificity on the anchor protein. Three large aliphatic amino acids (Leu(236), Ile(248), and Leu(252)) in the tethering domain of AKAP(CE) (residues 236-255) are crucial for ligation of R-CE. Their side chains apparently generate a precisely configured hydrophobic binding pocket that accommodates an apolar surface on RCE dimers, Basic residues (His(254)-Arg(255)-Lys(256)) at the C terminus of the tethering site set an upper limit on affinity for R-CE. A central dipeptide (phe(243)-Ser(244)) contributes critical and distinctive properties of the tethering site. Ser(244) is essential for selective binding of R-CE and exclusion of RII isoforms, The aromatic hydrophobic character of phe(243) ensures maximal R-CE binding activity, thereby supporting a "gatekeeper" function of Ser(244). Substitution of phe(243)-Ser(244) With Leu-Val generated an RII-specific AKAP. R-CE and RII subunits contain similar dimerization domains. AKAP-binding domains of R-CE (residues 23-47) and RII differ markedly in size, amino acid sequence, and docking specificity. Four hydrophobic residues (Cys(23), Val(27), Ile(32), and Cys(44)) in R-CE are crucial for avid binding with AKAP(CE), whereas side chains from Leu(20), Leu(35), Val(36), Ile(40), and Ile(41) have little impact on complex formation. Tyr(26) is embedded in the docking domain, but its aromatic ring is required for R-CE-R-CE dimerization. Residues 236-255 in AKAP(CE) also constitute a binding site for mammalian RI alpha. RI alpha (PKAI alpha) is tightly sequestered by AKAP(CE) in vitro (K-D = similar to 10 10 nM) and in the environment of intact cells. The tethering domain of AKAP(CE) provides a molecular module for manipulating intracellular localization of RI and elucidating functions of anchored PKAI in eukaryotes.
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页码:4351 / 4362
页数:12
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