How myosin VI traps its off-state, is activated and dimerizes

Author:

Canon Louise,Kikuti CarlosORCID,Planelles-Herrero Vicente J.ORCID,Lin Tianming,Mayeux Franck,Sirkia Helena,Lee Young il,Heidsieck Leila,Velikovsky Léonid,David Amandine,Liu Xiaoyan,Moussaoui Dihia,Forest Emma,Höök Peter,Petersen Karl J.,Morgan Tomos E.,Di Cicco Aurélie,Sirés-Campos JuliaORCID,Derivery EmmanuelORCID,Lévy DanielORCID,Delevoye CédricORCID,Sweeney H. Lee,Houdusse AnneORCID

Abstract

AbstractMyosin VI (Myo6) is the only minus-end directed nanomotor on actin, allowing it to uniquely contribute to numerous cellular functions. As for other nanomotors, the proper functioning of Myo6 relies on precise spatiotemporal control of motor activity via a poorly defined off-state and interactions with partners. Our structural, functional, and cellular studies reveal key features of myosin regulation and indicate that not all partners can activate Myo6. TOM1 and Dab2 cannot bind the off-state, while GIPC1 binds Myo6, releases its auto-inhibition and triggers proximal dimerization. Myo6 partners thus differentially recruit Myo6. We solved a crystal structure of the proximal dimerization domain, and show that its disruption compromises endocytosis in HeLa cells, emphasizing the importance of Myo6 dimerization. Finally, we show that the L926Q deafness mutation disrupts Myo6 auto-inhibition and indirectly impairs proximal dimerization. Our study thus demonstrates the importance of partners in the control of Myo6 auto-inhibition, localization, and activation.

Funder

Foundation for the National Institutes of Health

Agence Nationale de la Recherche

Ligue Contre le Cancer

Publisher

Springer Science and Business Media LLC

Subject

General Physics and Astronomy,General Biochemistry, Genetics and Molecular Biology,General Chemistry,Multidisciplinary

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