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Allosteric activation of proto-oncogene kinase Src by GPCR–beta-arrestin complexes

Natalia Pakharukova, Ali Masoudi, Biswaranjan Pani, Dean P. Staus, Robert J. Lefkowitz

2020Journal of Biological Chemistry50 citationsDOIOpen Access PDF

Abstract

and establish the conformational basis of the activation. Whereas free βarr1 had no effect on Src activity, βarr1 in complex with M2 muscarinic or β2-adrenergic receptors reconstituted in lipid nanodiscs activate Src by reducing the lag phase in Src autophosphorylation. Interestingly, receptor-βarr1 complexes formed with a βarr1 mutant, in which the finger-loop, required to interact with the receptor core, has been deleted, fully retain the ability to activate Src. Similarly, βarr1 in complex with only a phosphorylated C-terminal tail of the vasopressin 2 receptor activates Src as efficiently as GPCR-βarr complexes. In contrast, βarr1 and chimeric M2 receptor with nonphosphorylated C-terminal tail failed to activate Src. Taken together, these data demonstrate that the phosphorylated GPCR tail interaction with βarr1 is necessary and sufficient to empower it to allosterically activate Src. Our findings may have implications for understanding more broadly the mechanisms of allosteric activation of downstream targets by βarrs.

Topics & Concepts

G protein-coupled receptorProto-oncogene tyrosine-protein kinase SrcAllosteric regulationAutophosphorylationCell biologyBiologyReceptorSignal transducing adaptor proteinPhosphorylationChemistrySignal transductionBiochemistryProtein kinase AReceptor Mechanisms and SignalingNeuropeptides and Animal PhysiologyProtein Kinase Regulation and GTPase Signaling
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