Abstract

The overall goal of this project is to employ an innovative mass spectrometric technique to detect and characterize modifications to the chirality of individual amino acids within peptides and proteins. Chirality, or the handedness of a molecule, is a crucial attribute that influences both structure and function. Changes in chirality are very difficult to detect;however, a new method dependent on site specific radical migration is extremely sensitive to structure and can detect changes in chirality. The underlying motivation for performing this research is to investigate potential causes of cataract disease and to understand how protein modifications influence aging in general. Changes in chirality have been examined in primarily a generic sense in eye lens proteins previously, and these changes have been noted to increase for cataractous lenses. Site-specific examination of changes in chirality has not been carried out previously because no suitable tool was available for performing the task. The outcome of this project will be detailed information that elucidates how chiral inversion contributes to cataract formation and to aging in general, which is necessary to guide the development of potential preventative treatments.

Public Health Relevance

This research will examine molecular modifications that occur due to aging and are relevant to the formation of cataract, which is the world's leading cause of blindness. A more detailed understanding of these modifications is necessary to guide the development of potential therapies.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
1R01GM107099-01A1
Application #
8760787
Study Section
Enabling Bioanalytical and Imaging Technologies Study Section (EBIT)
Program Officer
Edmonds, Charles G
Project Start
2014-08-01
Project End
2018-07-31
Budget Start
2014-08-01
Budget End
2015-07-31
Support Year
1
Fiscal Year
2014
Total Cost
$256,139
Indirect Cost
$66,139

  Institution

Name
University of California Riverside
Department
Chemistry
Type
Schools of Earth Sciences/Natur
DUNS #
627797426
City
Riverside
State
CA
Country
United States
Zip Code
92521

  Publications

Talbert, Lance E; Julian, Ryan R (2018) Directed-Backbone Dissociation Following Bond-Specific Carbon-Sulfur UVPD at 213 nm. J Am Soc Mass Spectrom 29:1760-1767
Lyon, Yana A; Riggs, Dylan; Fornelli, Luca et al. (2018) The Ups and Downs of Repeated Cleavage and Internal Fragment Production in Top-Down Proteomics. J Am Soc Mass Spectrom 29:150-157
Bonner, James; Talbert, Lance E; Akkawi, Nicholas et al. (2018) Simplified identification of disulfide, trisulfide, and thioether pairs with 213 nm UVPD. Analyst 143:5176-5184
Lyon, Yana A; Sabbah, Georgette M; Julian, Ryan R (2018) Differences in ?-Crystallin isomerization reveal the activity of protein isoaspartyl methyltransferase (PIMT) in the nucleus and cortex of human lenses. Exp Eye Res 171:131-141
Lyon, Yana A; Sabbah, Georgette M; Julian, Ryan R (2017) Identification of Sequence Similarities among Isomerization Hotspots in Crystallin Proteins. J Proteome Res 16:1797-1805
R Julian, Ryan (2017) The Mechanism Behind Top-Down UVPD Experiments: Making Sense of Apparent Contradictions. J Am Soc Mass Spectrom 28:1823-1826
Lyon, Yana A; Beran, Gregory; Julian, Ryan R (2017) Leveraging Electron Transfer Dissociation for Site Selective Radical Generation: Applications for Peptide Epimer Analysis. J Am Soc Mass Spectrom 28:1365-1373
Riggs, Dylan L; Gomez, Sonia V; Julian, Ryan R (2017) Sequence and Solution Effects on the Prevalence of d-Isomers Produced by Deamidation. ACS Chem Biol 12:2875-2882
Bonner, James; Lyon, Yana A; Nellessen, Christopher et al. (2017) Photoelectron Transfer Dissociation Reveals Surprising Favorability of Zwitterionic States in Large Gaseous Peptides and Proteins. J Am Chem Soc 139:10286-10293