Eva Pebay‐Peyroula scite author profile

ATP, the principal energy currency of the cell, fuels most biosynthetic reactions in the cytoplasm by its hydrolysis into ADP and inorganic phosphate. Because resynthesis of ATP occurs in the mitochondrial matrix, ATP is exported into the cytoplasm while ADP is imported into the matrix. The exchange is accomplished by a single protein, the ADP/ATP carrier. Here we have solved the bovine carrier structure at a resolution of 2.2 A by X-ray crystallography in complex with an inhibitor, carboxyatractyloside. Six alpha-helices form a compact transmembrane domain, which, at the surface towards the space between inner and outer mitochondrial membranes, reveals a deep depression. At its bottom, a hexapeptide carrying the signature of nucleotide carriers (RRRMMM) is located. Our structure, together with earlier biochemical results, suggests that transport substrates bind to the bottom of the cavity and that translocation results from a transient transition from a 'pit' to a 'channel' conformation.

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X-ray Structure of Bacteriorhodopsin at 2.5 Angstroms from Microcrystals Grown in Lipidic Cubic Phases

Pebay‐Peyroula

Rummel

Rosenbusch

et al. 1997

Science

875

670

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Lipidic cubic phases provide a continuous three-dimensional bilayer matrix that facilitates nucleation and growth of bacteriorhodopsin microcrystals. The crystals diffract x-rays isotropically to 2.0 angstroms. The structure of this light-driven proton pump was solved at a resolution of 2.5 angstroms by molecular replacement, using previous results from electron crystallographic studies as a model. The earlier structure was generally confirmed, but several differences were found, including loop conformations and side chain residues. Eight water molecules are now identified experimentally in the proton pathway. These findings reveal the constituents of the proton translocation pathway in the ground state.

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Protein, lipid and water organization in bacteriorhodopsin crystals: a molecular view of the purple membrane at 1.9 Å resolution

et al. 1999

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X-ray structure of sensory rhodopsin II at 2.1-Å resolution

Royant

Nollert

Edman

et al. 2001

Proc. Natl. Acad. Sci. U.S.A.

276

324

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Sensory rhodopsins (SRs) belong to a subfamily of heptahelical transmembrane proteins containing a retinal chromophore. These photoreceptors mediate the cascade of vision in animal eyes and phototaxis in archaebacteria and unicellular flagellated algae. Signal transduction by these photoreceptors occurs by means of transducer proteins. The two archaebacterial sensory rhodopsins SRI and SRII are coupled to the membrane-bound HtrI and HtrII transducer proteins. Activation of these proteins initiates phosphorylation cascades that modulate the flagellar motors, resulting in either attractant (SRI) or repellent (SRII) phototaxis. In addition, transducer-free SRI and SRII were shown to operate as proton pumps, analogous to bacteriorhodopsin. Here, we present the x-ray structure of SRII from Natronobacterium pharaonis (pSRII) at 2.1-Å resolution, revealing a unique molecular architecture of the retinal-binding pocket. In particular, the structure of pSRII exhibits a largely unbent conformation of the retinal (as compared with bacteriorhodopsin and halorhodopsin), a hydroxyl group of Thr-204 in the vicinity of the Schiff base, and an outward orientation of the guanidinium group of Arg-72. Furthermore, the structure reveals a putative chloride ion that is coupled to the Schiff base by means of a hydrogen-bond network and a unique, positively charged surface patch for a probable interaction with HtrII. The high-resolution structure of pSRII provides a structural basis to elucidate the mechanisms of phototransduction and color tuning.A rchaeal rhodopsins are photoactive heptahelical transmembrane proteins containing a retinal chromophore that is bound to a Lys in helix G. Despite their common structural fold, their functions are distinctly different: bacteriorhodopsin (BR) and halorhodopsin (HR) are light-driven ion pumps transporting protons and chloride ions, respectively. The two archaebacterial sensory rhodopsins (SRs) SRI and SRII are blue-and greensensitive photosensors that transduce light signals into attractant and repellent migratory responses, respectively (1, 2). Signal transduction by these photoreceptors occurs by means of the membrane-bound HtrI and HtrII transducer proteins, whose activation initiates phosphorylation cascades that modulate the flagellar motors (3). In addition, analogous to BR, both SRI and SRII can operate as proton pumps when not bound to their respective transducers (2), suggesting that key elements of the mechanism of energy transduction in BR have been conserved in SRs. In particular, activation of these photoreceptors and also of visual rhodopsins from animal eyes induces tilting of helices on the cytoplasmic side (4). The mechanism by which this structural change in SRII is translated into proton pumping or signaling is not understood yet. Moreover, the physical mechanism of the spectral shift of SRII, which absorbs maximally near 500 nm (as compared with other archaeal rhodopsins whose absorption maxima are Ͼ560 nm) has not been defined. A comprehensive understanding of the mechanis...

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High-resolution X-ray structure of an early intermediate in the bacteriorhodopsin photocycle

Edman

Nollert

Royant

et al. 1999

Nature

317

308

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Bacteriorhodopsin is the simplest known photon-driven proton pump and as such provides a model for the study of a basic function in bioenergetics. Its seven transmembrane helices encompass a proton translocation pathway containing the chromophore, a retinal molecule covalently bound to lysine 216 through a protonated Schiff base, and a series of proton donors and acceptors. Photoisomerization of the all-trans retinal to the 13-cis configuration initiates the vectorial translocation of a proton from the Schiff base, the primary proton donor, to the extracellular side, followed by reprotonation of the Schiff base from the cytoplasm. Here we describe the high-resolution X-ray structure of an early intermediate in the photocycle of bacteriorhodopsin, which is formed directly after photoexcitation. A key water molecule is dislocated, allowing the primary proton acceptor, Asp 85, to move. Movement of the main-chain Lys 216 locally disrupts the hydrogen-bonding network of helix G, facilitating structural changes later in the photocycle.

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NADPH oxidase activator p67phox behaves in solution as a multidomain protein with semi-flexible linkers

Durand

Vivès

Cannella

et al. 2010

Journal of Structural Biology

287

292

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Helix deformation is coupled to vectorial proton transport in the photocycle of bacteriorhodopsin

Royant

Edman

Ursby

et al. 2000

Nature

232

261

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A wide variety of mechanisms are used to generate a proton-motive potential across cell membranes, a function lying at the heart of bioenergetics. Bacteriorhodopsin, the simplest known proton pump, provides a paradigm for understanding this process. Here we report, at 2.1 A resolution, the structural changes in bacteriorhodopsin immediately preceding the primary proton transfer event in its photocycle. The early structural rearrangements propagate from the protein's core towards the extracellular surface, disrupting the network of hydrogen-bonded water molecules that stabilizes helix C in the ground state. Concomitantly, a bend of this helix enables the negatively charged primary proton acceptor, Asp 85, to approach closer to the positively charged primary proton donor, the Schiff base. The primary proton transfer event would then neutralize these two groups, cancelling their electrostatic attraction and facilitating a relaxation of helix C to a less strained geometry. Reprotonation of the Schiff base by Asp 85 would thereby be impeded, ensuring vectorial proton transport. Structural rearrangements also occur near the protein's surface, aiding proton release to the extracellular medium.

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Structural basis for lipid‐mediated interactions between mitochondrial ADP/ATP carrier monomers

Nury¹,

Dahout-Gonzalez²,

Trezeguet³

et al. 2005

FEBS Letters

182

203

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The oligomerization state of the ADP/ATP carrier is an important issue in understanding the mechanism underlying nucleotide exchange across the inner mitochondrial membrane. The first high resolution structure obtained in the presence of carboxyatractyloside revealed a large cavity formed within a monomer in which the inhibitor is strongly bound. Whereas the protein-protein interactions implicated in the first crystal form are not biologically relevant, the new crystal form described herein, highlights favorable protein-protein interactions. The interactions are mediated by endogenous cardiolipins, which are tightly bound to the protein, two cardiolipins being sandwiched between the monomers on the matrix side. The putative dimerization interface evidenced here is consistent with other structural, biochemical or functional data published so far.

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