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An improved open-channel structure of MscL determined from FRET confocal microscopy and simulation
Authors:Ben Corry  Annette C Hurst  Prithwish Pal  Takeshi Nomura  Paul Rigby  Boris Martinac
Institution:1.School of Biomedical, Biomolecular and Chemical Sciences, and 2.Centre for Microscopy Characterisation and Analysis, The University of Western Australia, Crawley WA 6009, Australia;3.School of Biomedical Sciences, The University of Queensland, Brisbane QLD 4072, Australia;4.Victor Chang Cardiac Research Institute, Darlinghurst NSW 2010, Australia;5.St. Vincent’s Clinical School, The University of New South Wales, Sydney NSW 2052, Australia
Abstract:Mechanosensitive channels act as molecular transducers of mechanical force exerted on the membrane of living cells by opening in response to membrane bilayer deformations occurring in physiological processes such as touch, hearing, blood pressure regulation, and osmoregulation. Here, we determine the likely structure of the open state of the mechanosensitive channel of large conductance using a combination of patch clamp, fluorescence resonance energy transfer (FRET) spectroscopy, data from previous electron paramagnetic resonance experiments, and molecular and Brownian dynamics simulations. We show that structural rearrangements of the protein can be measured in similar conditions as patch clamp recordings while controlling the state of the pore in its natural lipid environment by modifying the lateral pressure distribution via the lipid bilayer. Transition to the open state is less dramatic than previously proposed, while the N terminus remains anchored at the surface of the membrane where it can either guide the tilt of or directly translate membrane tension to the conformation of the pore-lining helix. Combining FRET data obtained in physiological conditions with simulations is likely to be of great value for studying conformational changes in a range of multimeric membrane proteins.
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