reciprocally coupled residues crucial for protein kinase pak2 activity calculated by statistical coupling analysis相反地耦合残留的关键蛋白激酶pak2活动由统计耦合分析计算.pdfVIP
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reciprocally coupled residues crucial for protein kinase pak2 activity calculated by statistical coupling analysis相反地耦合残留的关键蛋白激酶pak2活动由统计耦合分析计算
Reciprocally Coupled Residues Crucial for Protein Kinase
Pak2 Activity Calculated by Statistical Coupling Analysis
Yuan-Hao Hsu*, Jolinda A. Traugh
Department of Biochemistry, University of California Riverside, Riverside, California, United States of America
Abstract
Regulation of Pak2 activity involves at least two mechanisms: (i) phosphorylation of the conserved Thr402 in the activation
loop and (ii) interaction of the autoinhibitory domain (AID) with the catalytic domain. We collected 482 human protein
kinase sequences from the kinome database and globally mapped the evolutionary interactions of the residues in the
catalytic domain with Thr402 by sequence-based statistical coupling analysis (SCA). Perturbation of Thr402 (34.6%) suggests a
communication pathway between Thr402 in the activation loop, and Phe387 (DDE387F,402T = 2.80) in the magnesium
positioning loop, Trp427 (DDE427W,402T = 3.12) in the F-helix, and Val404 (DDE404V,402T = 4.43) and Gly405 (DDE405G,402T = 2.95) in
the peptide positioning loop. When compared to the cAMP-dependent protein kinase (PKA) and Src, the perturbation
pattern of threonine phosphorylation in the activation loop of Pak2 is similar to that of PKA, and different from the tyrosine
phosphorylation pattern of Src. Reciprocal coupling analysis by SCA showed the residues perturbed by Thr402 and the
reciprocal coupling pairs formed a network centered at Trp427 in the F-helix. Nine pairs of reciprocal coupling residues
crucial for enzymatic activity and structural stabilization were identified. Pak2, PKA and Src share four pairs. Reciprocal
coupling residues expos
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