Abstract

EXCEED THE SPACE PROVIDED. Research will continue on the long-term goal of elucidating the molecular architecture of a-crystallin, the major protein component of the mammalian lens, and defining the mechanism of its chaperone function. The specific goals for the next funding period are to undertake a detailed thermodynamic analysis of the interactions between c_-crystallins and 13- crystallins, to investigate post-translational modifications that modulate these interactions, and to define the global structural and dynamic features of the native _-crystallin oligomer. The proposed research will definitively test the paradigm that a-crystallins maintain lens transparency through the recognition and binding of unfolding lens proteins. The results will bridge the knowledge gap between the rapidly developing understanding of the temporal trajectories of individual protein components and the consequences on their molecular interactions. The achievements of the previous funding period, including the determination of the folding pattern of the a-crystallin domain and the development of a mechanistic model of aA-crystallin chaperone function provide the bases for the proposed studies.
Four specific aims are designed to address two fundamental questions: i) What is the energy threshold required to trigger the binding of 13-crystallin to ct-crystallin and is this threshold crossed in age-related modifications? 2) How is this interaction modulated by the co-oligomerization of a-crystallin subunits and by phosphorylation of aB-crystallin? For this purpose, site-directed mutants of selected 13-crystallins will be constructed and characterized with respect to their stability and binding affinity to a-crystallin. Structural analysis will be performed using newly developed Electron Paramagnetic Resonance distance measurement methods on the 50A scale. Phosphorylation-mimic substitutions will be introduced in ctB-crystallin and their effects on the structure, dynamics and binding to 13-crystallins investigated. A unique combination of molecular biology and biophysical methods will be used to address a problem of central importance to the understanding of the molecular basis of lens transparency. To the extent that modifications of 13- crystallins play a role in age-related opacity, the proposed studies are of fundamental biomedical importance. More generally, a growing number of pathologies have been traced to protein aggregation and failures of the chaperone machinery. The anticipated results will elucidate common molecular events associated with these diseases. PERFORMANCE SITE ========================================Section End===========================================

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Research Project (R01)
Project #
5R01EY012018-08
Application #
6843132
Study Section
Visual Sciences A Study Section (VISA)
Program Officer
Liberman, Ellen S
Project Start
1998-02-01
Project End
2008-01-31
Budget Start
2005-02-01
Budget End
2006-01-31
Support Year
8
Fiscal Year
2005
Total Cost
$339,750
Indirect Cost

  Institution

Name
Vanderbilt University Medical Center
Department
Physiology
Type
Schools of Medicine
DUNS #
004413456
City
Nashville
State
TN
Country
United States
Zip Code
37212

  Publications

Mishra, Sanjay; Chandler, Shane A; Williams, Dewight et al. (2018) Engineering of a Polydisperse Small Heat-Shock Protein Reveals Conserved Motifs of Oligomer Plasticity. Structure 26:1116-1126.e4
Mishra, Sanjay; Wu, Shu-Yu; Fuller, Alexandra W et al. (2018) Loss of ?B-crystallin function in zebrafish reveals critical roles in the development of the lens and stress resistance of the heart. J Biol Chem 293:740-753
Wu, Shu-Yu; Zou, Ping; Fuller, Alexandra W et al. (2016) Expression of Cataract-linked ?-Crystallin Variants in Zebrafish Reveals a Proteostasis Network That Senses Protein Stability. J Biol Chem 291:25387-25397
Koteiche, Hanane A; Claxton, Derek P; Mishra, Sanjay et al. (2015) Species-Specific Structural and Functional Divergence of ?-Crystallins: Zebrafish ?Ba- and Rodent ?A(ins)-Crystallin Encode Activated Chaperones. Biochemistry 54:5949-58
Anderson, David M G; Floyd, Kyle A; Barnes, Stephen et al. (2015) A method to prevent protein delocalization in imaging mass spectrometry of non-adherent tissues: application to small vertebrate lens imaging. Anal Bioanal Chem 407:2311-20
Zou, Ping; Wu, Shu-Yu; Koteiche, Hanane A et al. (2015) A conserved role of ?A-crystallin in the development of the zebrafish embryonic lens. Exp Eye Res 138:104-13
Shi, Jian; Koteiche, Hanane A; McDonald, Ezelle T et al. (2013) Cryoelectron microscopy analysis of small heat shock protein 16.5 (Hsp16.5) complexes with T4 lysozyme reveals the structural basis of multimode binding. J Biol Chem 288:4819-30
Yirdaw, Robel B; McHaourab, Hassane S (2012) Direct observation of T4 lysozyme hinge-bending motion by fluorescence correlation spectroscopy. Biophys J 103:1525-36
Mishra, Sanjay; Stein, Richard A; McHaourab, Hassane S (2012) Cataract-linked ýýD-crystallin mutants have weak affinity to lens chaperones ýý-crystallins. FEBS Lett 586:330-6
McHaourab, Hassane S; Lin, Yi-Lun; Spiller, Benjamin W (2012) Crystal structure of an activated variant of small heat shock protein Hsp16.5. Biochemistry 51:5105-12

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