Research will be conducted to understand how G proteins are activated in the cytoplasm of the cell by a protein factor called Ric-8A. Heterotrimeric G proteins modulate cell metabolism, secretion, electrical conductivity, gene transcription, cell division and cellular motility, and therefore are essential to life in the doman of eukaryotes to which humans belong. Misregulation of G proteins is associated with cancer and a range of other diseases of relevance to general medicine. While most processes controlled by heterotrimeric G proteins occur at cell membranes, recent research has shown that G alpha subunits (G?) also control certain events in cell cytoplasm. Important among these is asymmetric cell division, which is essential for embryonic development. Ric-8A is critical regulator of G? in this process. Ric-8A is a Guanine nucleotide Exchange Factor (GEF) that catalyzes the exchange of guanosine diphosphate (GDP) for guanosine triphosphate (GTP) at the active site of G?. This reaction transitions G? to the so-called activated state. In preliminary studies, the Principal Investigator's laboratory demonstrated that Ric-8A induces and stabilizes G?i1 (a Gi-class G? subunit) in a structurally heterogeneous or molten globule-like state. The nucleotide-free Ric-8A:G?i1 intermediate is stable in the absence of GTP. The hypothesis to be tested is that Ric-8A catalyzes nucleotide exchange by altering the global and local structure of G?i1, and by increasing flexibility and inducing dynamic behavior. The overall goal of the project is to characterize the trajectory of the exchange reaction from binding of Ric-8A to G?i1.GDP, to the formation of the nucleotide-free Ric-8A:G?i1 complex. The first two aims of the proposal address, respectively, the structure and the dynamic behavior of the Ric- 8A:G?i1 complex.
The first aim i s to use Double Electron-Electron Resonance (DEER) spectroscopy to observe large-scale changes in the structures of G?i1 and Ric-8A upon formation of the G?i1:Ric-8A complex. Hydrogen-Deuterium eXchange, followed by proteolysis and Mass Spectrometry (HDXMS) will be employed to observe structural changes at a level of detail that approaches single amino acid residues. In the second aim, Forster Resonance Energy Transfer (smFRET) studies of individual molecules, either freely diffusing or immobilized on a solid matrix, will be conducted to determine whether formation of the G?i1:Ric-8A complex is accompanied by changes in the dynamic behavior of either protein.
The third aim of the proposal is to understand the mechanism by which Ric-8A alters the structure of G?i1 in the transition from the GDP- bound state to the nucleotide-free state. A combination of DEER and HDXMS methods will be used to study this transition. Site Directed Spin Labeling and Electron Paramagnetic Resonance Spectroscopy, together with mutational scanning experiments, will be used to identify Ric-8A residues that are critical to G?i1-binding and GEF activity, and the sites at which Ric-8A makes contact with G?i1.

Public Health Relevance

Normal human development requires that events during embryogenesis are tightly controlled, and that physiological processes throughout the body are properly regulated. Molecules called G proteins control both. This research will discover, at the molecular level, how G proteins are themselves regulated by a recently characterized protein molecule called Ric-8. This work will generate fundamental knowledge that will aid in understanding a regulatory process that is essential to life and that is disrupted in many diseases.

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
4R01GM105993-04
Application #
9021667
Study Section
Molecular and Integrative Signal Transduction Study Section (MIST)
Program Officer
Flicker, Paula F
Project Start
2013-04-01
Project End
2017-02-28
Budget Start
2016-03-01
Budget End
2017-02-28
Support Year
4
Fiscal Year
2016
Total Cost
$418,946
Indirect Cost
$124,518
Name
University of Montana
Department
Type
Organized Research Units
DUNS #
010379790
City
Missoula
State
MT
Country
United States
Zip Code
59812
Black, Labe A; Thomas, Celestine J; Nix, Gwendolyn N et al. (2016) Nanosecond Dynamics of G?i1 Bound to Nucleotides or Ric-8A, a G? Chaperone with GEF Activity. Biophys J 111:722-731
Kant, Ravi; Zeng, Baisen; Thomas, Celestine J et al. (2016) Ric-8A, a G protein chaperone with nucleotide exchange activity induces long-range secondary structure changes in G?. Elife 5:
Sprang, Stephen R (2016) Invited review: Activation of G proteins by GTP and the mechanism of G?-catalyzed GTP hydrolysis. Biopolymers 105:449-62
Van Eps, Ned; Thomas, Celestine J; Hubbell, Wayne L et al. (2015) The guanine nucleotide exchange factor Ric-8A induces domain separation and Ras domain plasticity in G?i1. Proc Natl Acad Sci U S A 112:1404-9
Sprang, Stephen R (2013) An acid test for g proteins. Mol Cell 51:405-6
Chan, Puiyee; Thomas, Celestine J; Sprang, Stephen R et al. (2013) Molecular chaperoning function of Ric-8 is to fold nascent heterotrimeric G protein ? subunits. Proc Natl Acad Sci U S A 110:3794-9