Abstract
The calcium calmodulin-dependent protein kinase II (CaMKII) is a dodecameric holoenzyme important for encoding memory. Its activation, triggered by binding of calcium-calmodulin, persists autonomously after calmodulin dissociation. One (receiver) kinase captures and subsequently phosphorylates the regulatory domain peptide of a donor kinase forming a chained dimer as the first stage of autonomous activation. Protein dynamics simulations examined the conformational changes triggered by dimer formation and phosphorylation, aimed to provide a molecular rationale for human mutations that result in learning disabilities. Ensembles generated from X-ray crystal structures were characterized by network centrality and community analysis. Mutual information related collective motions to local fragment dynamics encoded with a structural alphabet. Implicit solvent tCONCOORD conformational ensembles revealed the dynamic architecture of inactive kinase domains was co-opted in the activated dimer but the network hub shifted from the nucleotide binding cleft to the captured peptide. Explicit solvent molecular dynamics (MD) showed nucleotide and substrate binding determinants formed coupled nodes in long-range signal relays between regulatory peptides in the dimer. Strain in the extended captured peptide was balanced by reduced flexibility of the receiver kinase C-lobe core. The relays were organized around a hydrophobic patch between the captured peptide and a key binding helix. The human mutations aligned along the relays. Thus, these mutations could disrupt the allosteric network alternatively, or in addition, to altered binding affinities. Non-binding protein sectors distant from the binding sites mediated the allosteric signalling; providing possible targets for inhibitor design. Phosphorylation of the peptide modulated the dielectric of its binding pocket to strengthen the patch, non-binding sectors, domain interface and temporal correlations between parallel relays. These results provide the molecular details underlying the reported positive kinase cooperativity to enrich the discussion on how autonomous activation by phosphorylation leads to long-term behavioural effects.
Highlights
The calcium calmodulin-dependent protein kinase (CaMKII) is a multifunctional, multi-subunit eukaryotic protein kinase (EPK)
The multi-subunit kinase, calmodulin-dependent protein kinase II (CaMKII) is activated by calcium-calmodulin upon calcium jumps produced by synaptic stimulation
We have computationally generated interaction networks to map the conformational plasticity of the kinase domains where most mutations localize
Summary
The calcium calmodulin-dependent protein kinase (CaMKII) is a multifunctional, multi-subunit eukaryotic protein kinase (EPK). It has key roles in calcium regulation of neuronal and cardiovascular physiology [1,2,3]. The canonical EPK has a distinctive bi-lobed structure that exploits diverse strategies to achieve allosteric regulation [4]. CaMKII has a canonical kinase domain (KD) tethered via a linker to an well-conserved association domain (AD) that forms a central hub of the dodecameric holoenzyme with two hexamer rings that stack with mirror symmetry. The kinase is activated by rises in cellular calcium that enable calcium-calmodulin (Ca2+/CaM) to bind to and displace an autoinhibitory regulatory domain. The tuning frequency depends on the switching kinetics between the holoenzyme open and closed states [7]
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