Abstract

A major determinant of the transparency of the lens is the molecular organization of the crystallins. While most of the primary sequences of the crystallins in the beta family are known, the precise tertiary and quaternary structure remains to be determine. Little is known about the crystallin-crystallin interactions of the different beta polypeptides or how these interactions change during normal maturation and aging. One of the most striking observations in the aging human lens is the large amounts of deamidated crystallins. The overall goal of this application is to determine how deamidation affect normal cystallin- crystallin interaction. The hypothesis being tested is that deamidation plays a dual role in the overall lifetime of the lens. During lens maturation, deamidation allows increased pacing of crystallins. However, excessive deamidation causes further collapse and insolubilization of crystallin aggregates in cataract. To test this hypothesize the PI proposes to: 1) Characterize the normal structure of beta crystallins in the human lens with particular reference to those influences by deamidation. 2) Determine the effect of specific sites of deamidation on the secondary structure of beta subunits and on crystallin-crystallin interactions by using site-directed mutagenesis. 3) Determine if deamidation increases or decreases susceptibility of proteins to other post-translational modifications. The modifications to be tested are truncation, oxidation, and disulfide bond formation. These studies are important because they will help to elucidate the role of deamidation in crystallin interaction in the human lens. Site-directed mutagenesis will delineate the role of specific sites of deamidation which the investigator has identified to occur in vivo. A variety of techniques including electron spin resonance spectroscopy (ESR) will be used. ESR is advantageous because it is able to examine all regions within a protein, requires only small amounts of sample, and can be used to identify interactions occurring in solution.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
First Independent Research Support & Transition (FIRST) Awards (R29)
Project #
1R29EY012239-01
Application #
2676482
Study Section
Visual Sciences A Study Section (VISA)
Project Start
1998-08-01
Project End
2003-07-31
Budget Start
1998-08-01
Budget End
1999-07-31
Support Year
1
Fiscal Year
1998
Total Cost
Indirect Cost

  Institution

Name
Oregon Health and Science University
Department
Dentistry
Type
Schools of Dentistry
DUNS #
009584210
City
Portland
State
OR
Country
United States
Zip Code
97239

  Publications

Lampi, Kirsten J; Murray, Matthew R; Peterson, Matthew P et al. (2016) Differences in solution dynamics between lens ?-crystallin homodimers and heterodimers probed by hydrogen-deuterium exchange and deamidation. Biochim Biophys Acta 1860:304-14
Lampi, Kirsten J; Fox, Cade B; David, Larry L (2012) Changes in solvent accessibility of wild-type and deamidated ýýB2-crystallin following complex formation with ýýA-crystallin. Exp Eye Res 104:48-58
Mellies, Jay L; Benison, Gregory; McNitt, William et al. (2011) Ler of pathogenic Escherichia coli forms toroidal protein-DNA complexes. Microbiology 157:1123-33
Takata, Takumi; Smith, Joshua P; Arbogast, Brian et al. (2010) Solvent accessibility of betaB2-crystallin and local structural changes due to deamidation at the dimer interface. Exp Eye Res 91:336-46
Michiel, Magalie; Duprat, Elodie; Skouri-Panet, Feriel et al. (2010) Aggregation of deamidated human betaB2-crystallin and incomplete rescue by alpha-crystallin chaperone. Exp Eye Res 90:688-98
Dudek, Edward J; Lampi, Kirsten J; Lampi, Jason A et al. (2010) Ubiquitin proteasome pathway-mediated degradation of proteins: effects due to site-specific substrate deamidation. Invest Ophthalmol Vis Sci 51:4164-73