The trabecular meshwork of the eye is the principal site of outflow resistance to the aqueous humor. Our long-term goal is to develop selective gene transfer systems to assist cells in reducing resistance to aqueous humor outflow and thereby stopping visual field loss. We looked at the effects of transforming growth factor beta (TGF- beta) on the trabecular meshwork since the level of this cytokine increases in the aqueous humor with glaucoma. Using gene array analysis we were able to see alterations in gene expression of components related to the extracellular matrix when (TGF-beta) was added to the culture media of human trabecular meshwork cells. We verified the results of the gene arrays with real time polymerase chain reactions and with relative quantitative polymerase chain reactions. In addition, analysis of the proteome of the cells treated with TGF-beta was done. Several of the genes that were altered as a result of the TGF treatment had changes in the protein content within the cells. In addition, we noted changes in several cytoskeletal proteins. These changes suggested that in addition to the extracellular components whose gene expression had changed as a result of the TGF-beta treatment, alteration in the cytoskeleton of the trabecular meshwork was influenced at the protein level. Both of these finding are consistent with work that has been published with trabecular meshwork in perfusion culture and are consistent with changes observed in glaucoma. Thus, several of the alteration in the trabecular meshwork thought to be related to glaucoma may in fact be related to the increase in TGF-beta in aqueous humor. We are also studying the protein myocilin. Mutations in this protein have been shown to be associated with some forms of glaucoma. We over-expressed normal myocilin in mouse eyes to determine if the intraocular pressure was altered. Although the amount of myocilin in the mouse eye was approximately 4.7 fold more than in human aqueous humor, or about 2ng/ul, no increase in intraocular pressure was observed. These results indicate that over-expression of human myocilin by itself is not the cause of the increased resistance to outflow seen in primary open angle glaucoma. In addition, we expressed mutated myocilin to determine how this protein might be altering trabecular meshwork cells and thereby causing glaucoma. In vivo, in our transgenic mice, the mutated myocilin remained in the endoplasmic reticulum and the build-up of this mutated protein is probably responsible for the alteration and death of the trabecular meshwork cells in this form of glaucoma. We are currently working on ways to silence mutated myocilin. Silencing this protein should ultimately help the cells in regaining normal function and thereby cause an increase in outflow. This would have the effect of reducing the damage to the retinal ganglion cells. Initial work was done on parameters that influence silencing and several factors were shown to be significantly correlated to silencing by siRNAs. One of these factors is the effect of secondary or local structure on silencing. Since temperature can influence energy and this change can affect local structure, we investigated the influence of temperature on silencing of myocilin with various siRNAs. We found several of these siRNAs were affected by temperature with some assisted at lower temperatures and other being ineffective at lower temperatures. Temperature is an important consideration since the temperature of the anterior chamber of the eye is several degrees lower than body temperature.

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Intramural Research (Z01)
Project #
1Z01EY000303-11
Application #
7139184
Study Section
(LMOD)
Project Start
Project End
Budget Start
Budget End
Support Year
11
Fiscal Year
2005
Total Cost
Indirect Cost
Name
U.S. National Eye Institute
Department
Type
DUNS #
City
State
Country
United States
Zip Code
Russell, Paul; Walsh, Erin; Chen, WeiPing et al. (2006) The effect of temperature on gene silencing by siRNAs: implications for silencing in the anterior chamber of the eye. Exp Eye Res 82:1011-6
Sinha, Debasish; Hose, Stacey; Zhang, Cheng et al. (2005) A spontaneous mutation affects programmed cell death during development of the rat eye. Exp Eye Res 80:323-35
Zillig, Markus; Wurm, Antje; Grehn, Franz J et al. (2005) Overexpression and properties of wild-type and Tyr437His mutated myocilin in the eyes of transgenic mice. Invest Ophthalmol Vis Sci 46:223-34
Zhao, Xiujun; Ramsey, Keri E; Stephan, Dietrich A et al. (2004) Gene and protein expression changes in human trabecular meshwork cells treated with transforming growth factor-beta. Invest Ophthalmol Vis Sci 45:4023-34
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Rhee, Douglas J; Tamm, Ernst R; Russell, Paul (2003) Donor corneoscleral buttons: a new source of trabecular meshwork for research. Exp Eye Res 77:749-56
van den IJssel, Paul; Wheelock, Robert; Prescott, Alan et al. (2003) Nuclear speckle localisation of the small heat shock protein alpha B-crystallin and its inhibition by the R120G cardiomyopathy-linked mutation. Exp Cell Res 287:249-61
Zigler Jr, J Samuel; Qin, Chuan; Kamiya, Toshikazu et al. (2003) Tempol-H inhibits opacification of lenses in organ culture. Free Radic Biol Med 35:1194-202
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Takase, Hiroshi; Sugita, Sunao; Rhee, Douglas J et al. (2002) The presence of macrophage migration inhibitory factor in human trabecular meshwork and its upregulatory effects on the T helper 1 cytokine. Invest Ophthalmol Vis Sci 43:2691-6

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