| Literature DB >> 24513194 |
Isabel Llorente-Garcia1, Tchern Lenn2, Heiko Erhardt3, Oliver L Harriman4, Lu-Ning Liu5, Alex Robson4, Sheng-Wen Chiu4, Sarah Matthews4, Nicky J Willis5, Christopher D Bray5, Sang-Hyuk Lee6, Jae Yen Shin6, Carlos Bustamante6, Jan Liphardt6, Thorsten Friedrich3, Conrad W Mullineaux5, Mark C Leake7.
Abstract
Chemiosmotic energy coupling through oxidative phosphorylation (OXPHOS) is crucial to life, requiring coordinated enzymes whose membrane organization and dynamics are poorly understood. We quantitatively explore localization, stoichiometry, and dynamics of key OXPHOS complexes, functionally fluorescent protein-tagged, in Escherichia coli using low-angle fluorescence and superresolution microscopy, applying single-molecule analysis and novel nanoscale co-localization measurements. Mobile 100-200nm membrane domains containing tens to hundreds of complexes are indicated. Central to our results is that domains of different functional OXPHOS complexes do not co-localize, but ubiquinone diffusion in the membrane is rapid and long-range, consistent with a mobile carrier shuttling electrons between islands of different complexes. Our results categorically demonstrate that electron transport and proton circuitry in this model bacterium are spatially delocalized over the cell membrane, in stark contrast to mitochondrial bioenergetic supercomplexes. Different organisms use radically different strategies for OXPHOS membrane organization, likely depending on the stability of their environment.Entities:
Keywords: Co-localization analysis; Cytoplasmic membrane; Fluorescence microscopy; Fluorescent protein; Oxidative phosphorylation; Single-molecule biophysics
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Year: 2014 PMID: 24513194 DOI: 10.1016/j.bbabio.2014.01.020
Source DB: PubMed Journal: Biochim Biophys Acta ISSN: 0006-3002