Abstract

Protein-protein and protein-small molecule interactions at membrane surfaces underly most signal transduction pathways and many regulatory networks. The interfacial nature of these interactions presents many challenges to understanding them in terms of molecular structures and mechanisms. One of the most informative model systems for developing this understanding is the phototransduction pathway of retinal rod outer segments, in which a light signal, photon capture by the G-protein coupled receptor (GPCR), rhodopsin, is converted into a highly amplified electrical signal, hyperpolarization of the transmembrane voltage. This proposal aims to continue work aimed at understanding the structural and mechanistic bases of two key steps: activation of the heterotrimeric G protein, transducin, by photoactivated rhodopsin (R*), through accelerated exchange of GTP for GDP on the G protein subunit (G), and activation of a cGMP-specific phosphodiesterase, PD6, by G-GTP. These reactions happen on a sub-second time scale at the surface of disk membranes, and depend critically on the environment provided by the membrane lipids, so that they must be studied in that context. The proposed work is technically innovative in that cutting-edge approaches will be developed and used to determine structures that have proven intractable to conventional crystallographic approaches, and to determine the kinetics of individual steps in the G protein activation reaction. It is conceptually innovative in that it will determine for the first time the rate-limiting step in activation of a G protein, and he first structures of a G protein regulated effectors in the presence and absence of the activated G protein. There are two specific aims: 1. to refine the structures of holo-PDE6 and its complexes with transducin and a prenyl-binding protein using cryo-electron microcopy, cryo-electron tomography, and electron crystallography, combined with fitting of high resolution structures of fragments. 2. To determine the rate- limiting step in G protein activation. The startling finding i the previous funding period that the surface density of the phototransduction G protein, transducin, can be reduced by two-thirds without effect on phototransduction kinetics, eliminates binding of G protein to photoactivated rhodopsin, R*, as a candidate for the rate-limiting step in G protein activation, and leaves open the question of which step is limiting. We will use innovative approaches including flash-activation coupled with a scintillation proximity assay and time resolved fluorescence to determine the kinetics of each sub-reaction in the activation process.

Public Health Relevance

Understanding the details of phototransduction can aid in understanding blinding diseases caused by disruption of this pathway. More broadly it can guide our understanding of many other G protein-coupled pathways, which are the targets of most drugs currently in use, and which regulate nearly all important physiological processes in the central nervous system and throughout the body. PUBLIC HEALTH RELEVANCE: This proposal seeks to understand the molecular details of the first steps of vision, which can aid in understanding blinding diseases caused by disruption of this pathway. More broadly it can guide our understanding of many other G protein-coupled pathways, which are the targets of most drugs currently in use, and which regulate nearly all important physiological processes in the central nervous system and throughout the body, and so this understanding can help in design of new therapeutic approaches to a host of maladies.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Research Project (R01)
Project #
4R01EY007981-27
Application #
9020234
Study Section
Biology of the Visual System Study Section (BVS)
Program Officer
Neuhold, Lisa
Project Start
1989-08-01
Project End
2017-02-28
Budget Start
2016-03-01
Budget End
2017-02-28
Support Year
27
Fiscal Year
2016
Total Cost
Indirect Cost

  Institution

Name
Baylor College of Medicine
Department
Biochemistry
Type
Schools of Medicine
DUNS #
051113330
City
Houston
State
TX
Country
United States
Zip Code
77030

  Publications

Agosto, Melina A; Anastassov, Ivan A; Robichaux, Michael A et al. (2018) A Large Endoplasmic Reticulum-Resident Pool of TRPM1 in Retinal ON-Bipolar Cells. eNeuro 5:
Agosto, Melina A; Anastassov, Ivan A; Wensel, Theodore G (2018) Differential epitope masking reveals synapse-specific complexes of TRPM1. Vis Neurosci 35:E001
Dharmat, Rachayata; Eblimit, Aiden; Robichaux, Michael A et al. (2018) SPATA7 maintains a novel photoreceptor-specific zone in the distal connecting cilium. J Cell Biol 217:2851-2865
Tse, Dennis Y; Kim, Seong Jae; Chung, Inyoung et al. (2017) The ocular toxicity and pharmacokinetics of simvastatin following intravitreal injection in mice. Int J Ophthalmol 10:1361-1369
He, Feng; Agosto, Melina A; Anastassov, Ivan A et al. (2016) Phosphatidylinositol-3-phosphate is light-regulated and essential for survival in retinal rods. Sci Rep 6:26978
Zhao, Li; Chen, Yiyun; Bajaj, Amol Onkar et al. (2016) Integrative subcellular proteomic analysis allows accurate prediction of human disease-causing genes. Genome Res 26:660-9
Sung, Yun-Min; Wilkins, Angela D; Rodriguez, Gustavo J et al. (2016) Intramolecular allosteric communication in dopamine D2 receptor revealed by evolutionary amino acid covariation. Proc Natl Acad Sci U S A 113:3539-44
Wensel, Theodore G; Zhang, Zhixian; Anastassov, Ivan A et al. (2016) Structural and molecular bases of rod photoreceptor morphogenesis and disease. Prog Retin Eye Res 55:32-51
Roman-Sanchez, Ramon; Wensel, Theodore G; Wilson, John H (2016) Nonsense mutations in the rhodopsin gene that give rise to mild phenotypes trigger mRNA degradation in human cells by nonsense-mediated decay. Exp Eye Res 145:444-449
Wensel, Theodore G; Gilliam, Jared C (2015) Three-dimensional architecture of murine rod cilium revealed by cryo-EM. Methods Mol Biol 1271:267-92

Showing the most recent 10 out of 44 publications