Abstract

Without argument, the most important goal of gene therapy is to fix the somatic endogenous gene in a gene defect. This goal circumvents most major problems associated with current strategies of gene therapy mediated by viruses or proviruses, antisense oligonucleotides, or ribozymes. Our intent is to repair a gene much like the normal cellular process of nucleotide excision repair or mismatch repair, which occurs as a perfectly normal everyday occurrence in human cellular physiology.
Our aims are to employ the normal DNA repair enzymes of the eye and to supply a suitable repair substrate to the nucleus of the cell. Having provided this substrate, we will rely on the normal DNA repair enzymes of the cell to recognize a single nucleotide mismatch between the substrate and the endogenous gene and replace the defective base with the wildtype nucleotide. This process is now known as genoplasty. Our principal model systems will be the commonly available animal models of human oculocutaneous tyrosinase-negative albinism, white mice and New Zealand white rabbits. Using genoplasty, we plan to repair precisely known lesions in the tyrosinase gene somatically in RPE cells. Thus, this research will have high impact on the future directions of gene therapy in the eye. It is novel, no one else is doing this in the eye, and it is innovative because it uses the endogenous gene and normal DNA repair enzymes to allow the cell to fix itself. Our guiding hypothesis is that genoplasty works by mass action. The more substrate put into the cell, the more likely that gene repair will occur. We further hypothesize that virtually every cell has the right DNA repair enzymes and ancillary proteins. Thus, to achieve gene repair, all we need to do is get an adequate amount of substrate into the nucleus, and nature will take its course.
Our aims are: 1) to develop better assays for detecting gene repair of the tyrosinase gene in somatic RPE cells, 2) to achieve high levels of transfection and nuclear localization in ocular tissues, and 3) to design better substrates.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Small Research Grants (R03)
Project #
5R03EY013986-02
Application #
6623038
Study Section
Special Emphasis Panel (ZEY1-VSN (01))
Program Officer
Chin, Hemin R
Project Start
2002-04-01
Project End
2005-02-28
Budget Start
2003-03-01
Budget End
2004-02-29
Support Year
2
Fiscal Year
2003
Total Cost
$152,000
Indirect Cost

  Institution

Name
Emory University
Department
Ophthalmology
Type
Schools of Medicine
DUNS #
066469933
City
Atlanta
State
GA
Country
United States
Zip Code
30322

  Publications

Wu, Ji-Hong; Zhang, Sheng-Hai; Nickerson, John M et al. (2015) Cumulative mtDNA damage and mutations contribute to the progressive loss of RGCs in a rat model of glaucoma. Neurobiol Dis 74:167-179
Andrieu-Soler, Charlotte; Halhal, Mounia; Boatright, Jeffrey H et al. (2007) Single-stranded oligonucleotide-mediated in vivo gene repair in the rd1 retina. Mol Vis 13:692-706
Nickerson, John M; Frey, Ruth A; Ciavatta, Vincent T et al. (2006) Interphotoreceptor retinoid-binding protein gene structure in tetrapods and teleost fish. Mol Vis 12:1565-85
Andrieu-Soler, Charlotte; Casas, Mariana; Faussat, Anne-Marie et al. (2005) Stable transmission of targeted gene modification using single-stranded oligonucleotides with flanking LNAs. Nucleic Acids Res 33:3733-42
Ciavatta, Vincent T; Padove, Staci A; Boatright, Jeffrey H et al. (2005) Mouse retina has oligonucleotide-induced gene repair activity. Invest Ophthalmol Vis Sci 46:2291-9
Shuler Jr, R Keith; Dioguardi, Phyllis K; Henjy, Charles et al. (2004) Scleral permeability of a small, single-stranded oligonucleotide. J Ocul Pharmacol Ther 20:159-68
Rengarajan, Kalpana; Cristol, Stphen M; Mehta, Milan et al. (2002) Quantifying DNA concentrations using fluorometry: a comparison of fluorophores. Mol Vis 8:416-21