Abstract

The aim of cataract research is to prevent or delay human cataract formation. Cataract is the world's leading cause of blindness. Impaired epithelial function invariably leads to a loss of transparency. A therapy aimed at delaying or preventing human cataracts needs to be evaluated on human lens epithelial cells (HLECs). Due to the scarcity of viable human lenses, numerous investigators have tried to culture HLECs. However, normal, HLECs complete 2-4 passages in culture and undergo senescence. HLECs have properties different from those of the lower species. For example, lens epithelial lines can be established from lower species using standard techniques; this is not true of HLECs. Metabolic fluxes in various species are also different relative to the polyol pathway. Aldose reductase activity is high in the dog and rat lens, very low in the human lens and absent in the mouse. Although viral transformation of HLECs permits growth, virally transformed cells have properties that are different from their non-transformed counterparts. Experiments are needed to determine the properties of normal HLECs.
Our aims are to establish a reliable supply of normal HLECs, characterize them and make them available to the eye research community. This is absolutely necessary for future studies.
The aims are to: 1. Determine if a wound-healing environment permits the long-term growth of normal HLECs from young, old and cataractous lenses. 2. Determine if the introduction of telomerase into HLECs permits establishment of lines fromlens explants, permits established lines to overcome senescence, and if the presence of telomerase maintains the diploid state and allows maintenance of in vivo characteristics. Determine the ploidy, isoenzyme phenotyping, DNA fingerprint, alphaA and alphaB crystallin expression, and growth in cells generated Aim 1 or 2. 3. Determine if there are metabolic differences between cells from young, old and cataractous lenses. 4. Identify lens-specific regulatory elements in the promoters of genes that encode gamma-glutamylcysteine synthetase (GCS).

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Research Project (R01)
Project #
5R01EY013123-03
Application #
6518691
Study Section
Visual Sciences A Study Section (VISA)
Program Officer
Liberman, Ellen S
Project Start
2000-07-01
Project End
2005-05-31
Budget Start
2002-06-01
Budget End
2005-05-31
Support Year
3
Fiscal Year
2002
Total Cost
$213,000
Indirect Cost

  Institution

Name
Oakland University
Department
Biology
Type
Schools of Arts and Sciences
DUNS #
City
Rochester
State
MI
Country
United States
Zip Code
48309

  Publications

Obrenovich, Mark E; Fan, Xingjun; Satake, Makoto et al. (2006) Relative suppression of the sodium-dependent Vitamin C transport in mouse versus human lens epithelial cells. Mol Cell Biochem 293:53-62
Marcantonio, J M; Reddan, J R (2004) TGFbeta2 influences alpha5-beta1 integrin distribution in human lens cells. Exp Eye Res 79:437-42
Wormstone, I M; Tamiya, S; Eldred, J A et al. (2004) Characterisation of TGF-beta2 signalling and function in a human lens cell line. Exp Eye Res 78:705-14
Lo, Woo-Kuen; Zhou, Cheng-Jing; Reddan, John (2004) Identification of caveolae and their signature proteins caveolin 1 and 2 in the lens. Exp Eye Res 79:487-98
Reddan, John R; Giblin, Frank J; Sevilla, Michael et al. (2003) Propyl gallate is a superoxide dismutase mimic and protects cultured lens epithelial cells from H2O2 insult. Exp Eye Res 76:49-59
Wormstone, I M; Tamiya, S; Marcantonio, J M et al. (2000) Hepatocyte growth factor function and c-Met expression in human lens epithelial cells. Invest Ophthalmol Vis Sci 41:4216-22