| Article ID | Journal | Published Year | Pages | File Type |
|---|---|---|---|---|
| 5914478 | Journal of Structural Biology | 2012 | 9 Pages |
Abstract
Homohexameric, N-Ethylmaleimide Sensitive Factor (NSF) disassembles Soluble NSF Attachment Protein Receptor (SNARE) complexes after membrane fusion, an essential step in vesicular trafficking. NSF contains three domains (NSF-N, NSF-D1, and NSF-D2), each contributing to activity. We combined electron microscopic (EM) analysis, analytical ultracentrifugation (AU) and functional mutagenesis to visualize NSF's ATPase cycle. 3D density maps show that NSF-D2 remains stable, whereas NSF-N undergoes large conformational changes. NSF-Ns splay out perpendicular to the ADP-bound hexamer and twist upwards upon ATP binding, producing a more compact structure. These conformations were confirmed by hydrodynamic, AU measurements: NSF-ATP sediments faster with a lower frictional ratio (f/f0). Hydrodynamic analyses of NSF mutants, with specific functional defects, define the structures underlying these conformational changes. Mapping mutations onto our 3D models allows interpretation of the domain movement and suggests a mechanism for NSF binding to and disassembly of SNARE complexes.
Keywords
PDBATPase associated with diverse cellular activitiesNSFSNAREVCPAAAAAA proteinsSNAREsanalytical ultracentrifugationAnalytical centrifugationSNAPN-ethylmaleimide sensitive factorMembrane traffickingElectron microscopyValosin containing proteinProtein Data Basesoluble NSF attachment proteinSNAP Receptor
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Molecular Biology
Authors
Arne Moeller, Chunxia Zhao, Michael G. Fried, Elizabeth M. Wilson-Kubalek, Bridget Carragher, Sidney W. Whiteheart,