Abstract

Optical clarity is a prerequisite for normal lens function. In broad terms this proposal addresses the question of how the biological functional integrity of the lens contributes to the physical requirements necessary for sustained transparency. The opaque lens, resulting from enhanced light scattering, is the medical condition of cataract. We propose to continue liquids and solids NMR studies of lens tissue and its purified crystallins which are aimed at the elucidation of the motional dynamics characteristics of both large and small molecules (and the affecting factors), such that lens protein organization and interaction can be inferred. Our intent is to forge a link to transparency. Because of lens heterogeneity some of the proposed NMR experiments will be performed on a spatially localized basis. 13C and 31P off-resonance rotating frame spin lattice relaxation experiments and the solid state NMR techniques of dipolar decoupling and cross polarization will be employed to assess the motional characteristics of lens proteins and phosphorus metabolites. The multiquantum spectral behavior of 23Na+ and 39K+ will be used to report on the surrounding macromolecular organization. Pulse gradient spin echo NMR experiments will permit elucidation of translational diffusion as well as the occurrence of restricted diffusion of lens water and selected phosphorus metabolites. Proton microimaging experiments will enable the acquisition of spatially localized lens water diffusion data. Particular emphasis will be directed to the elucidation of the organizational differences between the lens cortex and nucleus. Initial experiments will be performed with bovine lens homogenates, the intact lens, and purified alpha, beta, and gamma-crystallins. The potential interplay of metabolism with lens protein organization and interaction will be explored. The ancillary technique of resolution enhanced FTIR spectroscopy will be utilized in the proposed studies as a probe of protein structure. Bovine, rabbit, and human lens tissue will be utilized. Age will be a variable. Both the clear and cataractous lens will be studied. These studies will be extended to the X-ray, galactose, high Ca++, Tris, EGTA, and oubain induced experimental cataracts in the above animal models. The results of the proposed studies may provide the basic knowledge necessary to establish rationale for the identification f lenses with pre- cataractous changes. The ability to do so will permit an opportunity to initiate medical anticataract therapy and monitor efficacy of treatment.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Research Project (R01)
Project #
5R01EY004033-13
Application #
2158969
Study Section
Biophysical Chemistry Study Section (BBCB)
Project Start
1982-03-01
Project End
1996-02-29
Budget Start
1994-03-01
Budget End
1996-02-29
Support Year
13
Fiscal Year
1994
Total Cost
Indirect Cost

  Institution

Name
University of California Santa Cruz
Department
Chemistry
Type
Schools of Arts and Sciences
DUNS #
City
Santa Cruz
State
CA
Country
United States
Zip Code
95064

  Publications

Luo, Y; Rydzewski, J; de Graaf, R A et al. (1999) In vivo observation of lactate methyl proton magnetization transfer in rat C6 glioma. Magn Reson Med 41:676-85
Kuwata, K; Liu, H; Schleich, T et al. (1997) Rotational correlation times of internuclear vectors in a DNA duplex with G-A mismatch determined in aqueous solution by complete relaxation matrix analysis of off-resonance ROESY (O-ROESY) spectra. J Magn Reson 128:70-81
Rydzewski, J M; Schleich, T (1996) Deuterium off-resonance rotating frame spin-lattice relaxation of macromolecular bound ligands. Biophys J 70:1472-84
Willis, J A; Schleich, T (1996) Oxidative-stress induced protein glutathione mixed-disulfide formation in the ocular lens. Biochim Biophys Acta 1313:20-8
Willis, J A; Schleich, T (1995) 13C-NMR spectroscopic studies of 2-mercaptoethanol-stimulated glutathione synthesis in the intact ocular lens. Biochim Biophys Acta 1265:1-7
Stevens, A; Wang, S X; Caines, G H et al. (1995) 13C-NMR off-resonance rotating frame spin-lattice relaxation studies of bovine lens gamma-crystallin self association: effect of 'macromolecular crowding'. Biochim Biophys Acta 1246:82-90
Kuwata, K; Brooks, D; Yang, H et al. (1994) Relaxation-matrix formalism for rotating-frame spin-lattice proton NMR relaxation and magnetization transfer in the presence of an off-resonance irradiation field. J Magn Reson B 104:11-25
Yang, H; Schleich, T (1994) Modified Jeener solid-echo pulse sequences for the measurement of the proton dipolar spin-lattice relaxation time (T1D) of tissue solid-like macromolecular components. J Magn Reson B 105:205-10
Rydzewski, J M; Schleich, T (1994) Off-resonance rotating-frame spin-lattice relaxation of quadrupolar (spin-1) nuclei. J Magn Reson B 105:129-36
Yang, H; Schleich, T (1994) T1 discrimination contributions to proton magnetization transfer in heterogeneous biological systems. Magn Reson Med 32:16-22

Showing the most recent 10 out of 31 publications