Cataract is a leading cause of blindness throughout the world, yet the
fundamental biochemical causes are unknown. A rodent model of the biochemical
processes is selenite cataract. This cataract shows some of the features of human
cataracts such as increased lens calcium, proteolysis of proteins, and
insolubilization leading to lens opacity. The goals of the current experiments were:
(1) To measure changes in transcript levels for calpains and caspase 3 and
oxidation of epithelial proteins in selenite cataract. (2) To elucidate changes in
calpain 10 and its interaction with other calpains in selenite cataract. (3) To
investigate changes in stability of ��B1-crystallin caused by deamidation and
truncation. These data would provide roles for apoptosis, protein insolubilization,
proteolysis and deamidation observed in cataract.
To induce cataract, 12-day old rats were injected with an overdose of Na���SeO���.
Epithelium was analyzed by competitive RT-PCR, zymography, and thiol-blotting.
Calpains were detected by western-blotting. For ��B1-crystallin stability studies,
recombinant ��B1-crystallins were denatured by urea or heat. Urea stability was
measured by circular dichroism and fluorescence spectrometry, and heat stability
was measured by light scattering at 405 nm.
During selenite cataract formation, calpains in epithelium were activated
resulting in increased proteolysis of crystallins, but mRNA levels for calpains did
not show appreciable changes. Oxidation of sulthydryls in epithelial proteins was
minimal during cataract formation. These results suggested that calpain-induced
proteolysis in the epithelium contribute to selenite cataract. In selenite cataract,
calpain 10 proteins disappeared, which appeared to be due to degradation by
calpain 2 and Lp82 calpain.
Deamidated ��B1-crystallin was less stable in urea and heat, compared to wildtype.
When the terminal extensions were removed, ��B1-crystallin was as stable as
wild-type. However, without the extensions, truncated ��B1-crystallin caused
accelerated precipitation in a complex with ��A-crystallin, suggesting that the
extensions may contribute to proper association with other crystallins and to
stability of the soluble complexes.
In summary, proteolysis of proteins by calpains was more pronounced than
protein oxidation in lens epithelium of selenite cataract. Deamidation and
truncation caused instability of ��B1-crystallin and abnormal association with ��A-crystallin.
Thus, proteolysis and deamidation may increase susceptibility of lenses
to cataract. / Graduation date: 2003
| Identifer | oai:union.ndltd.org:ORGSU/oai:ir.library.oregonstate.edu:1957/32630 |
| Date | 04 September 2002 |
| Creators | Kim, Yung Hae |
| Contributors | Shearer, Thomas R. |
| Source Sets | Oregon State University |
| Language | en_US |
| Detected Language | English |
| Type | Thesis/Dissertation |
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