Abstract

Vitamin A (retinal) and coenzyme Q (ubiquinone) are small hydrophobic isoprenoids whose photochemical and redox properties have been exploited by membrane proteins. The proposed research focuses on the mechanism of light transduction by the retinal chromophore in the visual pigment rhodopsin and proton translocation by quinone molecules in mitochondrial and photosynthetic membranes. These studies take advantage of magic angle spinning NMR approaches for obtaining high-resolution structural data of membrane proteins in bilayer environments. Chemical shift measurements of the protein-bound retinal chromophore are proposed for determining the structure of the retinal binding site in rhodopsin and its photointermediates. Rotational resonance NMR measurements are proposed for determining C+C-C+C torsion angles along the retinal chain. Together, these studies address the mechanism for energy storage in the rhodopsin - >bathorhodopsin reaction, and the mechanism for proton transfer in the metarhodopsin I -> metarhodopsin II reaction. The proton transfer reaction is the key step in triggering the binding of the G-protein transducin. Similar measurements on the red, green and blue cone proteins will establish the mechanism of color regulation in visual pigments. NMR studies are proposed for determining the location and orientation of free ubiquinone and ubiquinol in membrane bilayers. NMR measurements of 13C-labeled quinone molecules in oriented membrane bilayers are planned that take advantage of the orientation dependence of the chemical shift and dipole-dipole interactions. NMR measurements of 2H-labeled quinones are proposed that take advantage of the sensitivity to motion of the 2H lineshape to characterize quinone dynamics. Comparative studies of quinones with different chain lengths (3-10 isoprene units) are aimed at addressing the role of chain length in determining quinone location and dynamics. Together, these studies address how quinones facilitate the transport of protons between protein components in energy transducing membranes. Finally, rotational-echo double resonance NMR measurements are planned for determining which residues form the quinone binding sites in the cytochrome bC1 complex. The rotational-echo experiment yields high- resolution distance constraints between 13C--labeled quinones and 15N- labeled protein groups with approximately 5 A. Such structural data is essential for establishing the key residues responsible for catalyzing the quinone redox chemistry.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
2R01GM041412-06A2
Application #
2180862
Study Section
Molecular and Cellular Biophysics Study Section (BBCA)
Project Start
1988-12-01
Project End
1999-03-31
Budget Start
1995-04-01
Budget End
1996-03-31
Support Year
6
Fiscal Year
1995
Total Cost
Indirect Cost

  Institution

Name
Yale University
Department
Biochemistry
Type
Schools of Medicine
DUNS #
082359691
City
New Haven
State
CT
Country
United States
Zip Code
06520

  Publications

Sanchez-Reyes, Omar B; Cooke, Aidan L G; Tranter, Dale B et al. (2017) G Protein-Coupled Receptors Contain Two Conserved Packing Clusters. Biophys J 112:2315-2326
Kimata, Naoki; Pope, Andreyah; Eilers, Markus et al. (2016) Retinal orientation and interactions in rhodopsin reveal a two-stage trigger mechanism for activation. Nat Commun 7:12683
Kimata, Naoki; Pope, Andreyah; Sanchez-Reyes, Omar B et al. (2016) Free backbone carbonyls mediate rhodopsin activation. Nat Struct Mol Biol 23:738-43
Opefi, Chikwado A; Tranter, Dale; Smith, Steven O et al. (2015) Construction of stable mammalian cell lines for inducible expression of G protein-coupled receptors. Methods Enzymol 556:283-305
Kimata, Naoki; Reeves, Philip J; Smith, Steven O (2015) Uncovering the triggers for GPCR activation using solid-state NMR spectroscopy. J Magn Reson 253:111-8
Kimata, Naoki; Pope, Andreyah; Rashid, Dawood et al. (2015) Sequential structural changes in rhodopsin occurring upon photoactivation. Methods Mol Biol 1271:159-71
Pope, Andreyah; Eilers, Markus; Reeves, Philip J et al. (2014) Amino acid conservation and interactions in rhodopsin: probing receptor activation by NMR spectroscopy. Biochim Biophys Acta 1837:683-93
Goncalves, Joseph; Eilers, Markus; South, Kieron et al. (2013) Magic angle spinning nuclear magnetic resonance spectroscopy of G protein-coupled receptors. Methods Enzymol 522:365-89
Xu, Bing; Chakraborty, Raja; Eilers, Markus et al. (2013) High-level expression, purification and characterization of a constitutively active thromboxane A2 receptor polymorphic variant. PLoS One 8:e76481
Opefi, Chikwado A; South, Kieron; Reynolds, Christopher A et al. (2013) Retinitis pigmentosa mutants provide insight into the role of the N-terminal cap in rhodopsin folding, structure, and function. J Biol Chem 288:33912-26

Showing the most recent 10 out of 53 publications