Structure of the α-actinin-vinculin head domain complex determined by cryo-electron microscopy

Deborah F. Kelly; Dianne W. Taylor; Constantina Bakolitsa; Andrey A. Bobkov; Laurie Bankston; Robert C. Liddington; Kenneth A. Taylor

doi:10.1016/j.jmb.2005.12.076

Structure of the α-actinin-vinculin head domain complex determined by cryo-electron microscopy

Deborah F. Kelly, Dianne W. Taylor, Constantina Bakolitsa, Andrey A. Bobkov, Laurie Bankston, Robert C. Liddington, Kenneth A. Taylor

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Abstract

The vinculin binding site on α-actinin was determined by cryo-electron microscopy of 2D arrays formed on phospholipid monolayers doped with a nickel chelating lipid. Chicken smooth muscle α-actinin was cocrystallized with the β1-integrin cytoplasmic domain and a vinculin fragment containing residues 1-258 (vinculin_D1). Vinculin _D1 was located at a single site on α-actinin with 60-70% occupancy. In these arrays, α-actinin lacks molecular 2-fold symmetry and the two ends of the molecule, which contain the calmodulin-like and actin binding domains, are held in distinctly different environments. The vinculin_D1 difference density has a shape very suggestive of the atomic structure. The atomic model of the complex juxtaposes the α-actinin binding site on vinculin_D1 with the N-terminal lobe of the calmodulin-like domain on α-actinin. The results show that the interaction between two species with weak affinity can be visualized in a membrane-like environment.

Original language	English (US)
Pages (from-to)	562-573
Number of pages	12
Journal	Journal of Molecular Biology
Volume	357
Issue number	2
DOIs	https://doi.org/10.1016/j.jmb.2005.12.076
State	Published - Mar 24 2006

All Science Journal Classification (ASJC) codes

Structural Biology
Molecular Biology

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title = "Structure of the α-actinin-vinculin head domain complex determined by cryo-electron microscopy",

abstract = "The vinculin binding site on α-actinin was determined by cryo-electron microscopy of 2D arrays formed on phospholipid monolayers doped with a nickel chelating lipid. Chicken smooth muscle α-actinin was cocrystallized with the β1-integrin cytoplasmic domain and a vinculin fragment containing residues 1-258 (vinculinD1). Vinculin D1 was located at a single site on α-actinin with 60-70% occupancy. In these arrays, α-actinin lacks molecular 2-fold symmetry and the two ends of the molecule, which contain the calmodulin-like and actin binding domains, are held in distinctly different environments. The vinculinD1 difference density has a shape very suggestive of the atomic structure. The atomic model of the complex juxtaposes the α-actinin binding site on vinculinD1 with the N-terminal lobe of the calmodulin-like domain on α-actinin. The results show that the interaction between two species with weak affinity can be visualized in a membrane-like environment.",

author = "Kelly, {Deborah F.} and Taylor, {Dianne W.} and Constantina Bakolitsa and Bobkov, {Andrey A.} and Laurie Bankston and Liddington, {Robert C.} and Taylor, {Kenneth A.}",

note = "Funding Information: We thank Mr Greg Cadwell for cloning and protein purification and Professor David R. Critchley (University of Leicester, UK) for the talin VBS3, α-actinin-1 and vinculin D1 constructs and his comments on an earlier version of the manuscript. This research was supported by NIH Grant GM64346 to the Cell Migration Consortium.",

year = "2006",

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doi = "10.1016/j.jmb.2005.12.076",

language = "English (US)",

volume = "357",

pages = "562--573",

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T1 - Structure of the α-actinin-vinculin head domain complex determined by cryo-electron microscopy

AU - Kelly, Deborah F.

AU - Taylor, Dianne W.

AU - Bakolitsa, Constantina

AU - Bobkov, Andrey A.

AU - Bankston, Laurie

AU - Liddington, Robert C.

AU - Taylor, Kenneth A.

N1 - Funding Information: We thank Mr Greg Cadwell for cloning and protein purification and Professor David R. Critchley (University of Leicester, UK) for the talin VBS3, α-actinin-1 and vinculin D1 constructs and his comments on an earlier version of the manuscript. This research was supported by NIH Grant GM64346 to the Cell Migration Consortium.

PY - 2006/3/24

Y1 - 2006/3/24

N2 - The vinculin binding site on α-actinin was determined by cryo-electron microscopy of 2D arrays formed on phospholipid monolayers doped with a nickel chelating lipid. Chicken smooth muscle α-actinin was cocrystallized with the β1-integrin cytoplasmic domain and a vinculin fragment containing residues 1-258 (vinculinD1). Vinculin D1 was located at a single site on α-actinin with 60-70% occupancy. In these arrays, α-actinin lacks molecular 2-fold symmetry and the two ends of the molecule, which contain the calmodulin-like and actin binding domains, are held in distinctly different environments. The vinculinD1 difference density has a shape very suggestive of the atomic structure. The atomic model of the complex juxtaposes the α-actinin binding site on vinculinD1 with the N-terminal lobe of the calmodulin-like domain on α-actinin. The results show that the interaction between two species with weak affinity can be visualized in a membrane-like environment.

AB - The vinculin binding site on α-actinin was determined by cryo-electron microscopy of 2D arrays formed on phospholipid monolayers doped with a nickel chelating lipid. Chicken smooth muscle α-actinin was cocrystallized with the β1-integrin cytoplasmic domain and a vinculin fragment containing residues 1-258 (vinculinD1). Vinculin D1 was located at a single site on α-actinin with 60-70% occupancy. In these arrays, α-actinin lacks molecular 2-fold symmetry and the two ends of the molecule, which contain the calmodulin-like and actin binding domains, are held in distinctly different environments. The vinculinD1 difference density has a shape very suggestive of the atomic structure. The atomic model of the complex juxtaposes the α-actinin binding site on vinculinD1 with the N-terminal lobe of the calmodulin-like domain on α-actinin. The results show that the interaction between two species with weak affinity can be visualized in a membrane-like environment.

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Structure of the α-actinin-vinculin head domain complex determined by cryo-electron microscopy

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