Phospho-regulated tethering of focal adhesion kinase to vinculin links force transduction to focal adhesion signaling

被引:0
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作者
Karen Diaz-Palacios [1 ]
Pilar López Navajas [1 ]
Bárbara Rodrigo Martín [1 ]
Ruth Matesanz [1 ]
Juan R. Luque-Ortega [3 ]
Asier Echarri [2 ]
Daniel Lietha [1 ]
机构
[1] Molecular and Cellular Biosciences,
[2] Margarita Salas Center for Biological Research (CIB),undefined
[3] Spanish National Research Council (CSIC),undefined
[4] Biomedicine,undefined
[5] Margarita Salas Center for Biological Research (CIB),undefined
[6] Spanish National Research Council (CSIC),undefined
[7] Molecular Interactions Facility,undefined
[8] Margarita Salas Center for Biological Research (CIB),undefined
[9] Spanish National Research Council (CSIC),undefined
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D O I
10.1186/s12964-025-02201-3
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摘要
Focal Adhesion Kinase (FAK) is a key signaling molecule in focal adhesions (FAs) orchestrating the formation, maturation and turnover of the FA complex. A controlled FA lifecycle is essential for various cellular processes requiring mesenchymal cell migration and is harnessed by advanced cancers to initiate cancer invasion and metastasis. The mechanical force for migration is transmitted from actin stress fibers to FAs via specialized force transduction components in FAs. These forces are known to activate FA signaling, suggesting a communication between FA force transduction and FA signaling components, yet how this occurs mechanistically is unknown. Here we demonstrate that paxillin can act as an adaptor protein to connect FAK with the force transduction component vinculin. Our data show that this connection forms inefficient in the basal state but suggest Y925 phosphorylation in FAK as a key mechanism for optimal formation of the FAK:paxillin:vinculin linkage. This is achieved by switching binding of the paxillin LD2 motif from FAK to vinculin while keeping paxillin LD4 tethered to FAK. We further provide the first high-resolution crystal structure of LD2 bound to the vinculin tail domain, which importantly shows that vinculin can simultaneously link to actin. This therefore ensures an intact force transduction role of vinculin while tethered via paxillin to the signaling apparatus in FAs. With this data, all interactions of the force transmitting tether to FAK are structurally defined and we provide an atomic model for FAK force activation. In summary, we propose a phospho-regulated connection between signaling and force transduction components in FAs allowing for force induced activation of FA signaling.
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