Abstract

This project studies the regulation of expression of genes encoding lens fiber membrane channel proteins, which are essential for maintaining the transparency and correct refractive index of the lens. We are presently focusing on the regulation of expression of the gene encoding MIP, the major intrinsic protein of the lens fiber membrane, that is specifically expressed in the ocular lens fibers and belongs to an ancient family of transmembrane channel proteins. We have continued studying the transcriptional regulation of the MIP gene. The Sp family of transcription factors is involved in the regulation of transcription of the MIP gene. Sp3 interacts with a regulatory element of the MIP promoter, required for activation in the lens. We also studied the expression of the transcription factors AP2. We found that the gene encoding the transcription factor AP2 is expressed in the lens epithelia and that a novel splice variant, which lacks part of the activation domain, is present in the lens. In collaboration with Drs. Dwight Stambolian and Jack Favor we have characterized at the molecular level the Hfi mouse genetic cataract, which localizes to the MIP gene locus. We found that a deletion in the exon2/intron3 junction of the MIP gene results in deletion of exon 2 in the resultant transcript, produced by an exon skipping mechanism. MIP knock-out mouse experiments that we are conducting in collaboration with Dr. Anthony Wynshaw-Boris, will allow us to understand the role of MIP gene expression in lens transparency.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Intramural Research (Z01)
Project #
1Z01EY000253-09
Application #
6162362
Study Section
Special Emphasis Panel (LMDB)
Project Start
Project End
Budget Start
Budget End
Support Year
9
Fiscal Year
1997
Total Cost
Indirect Cost

  Institution

Name
U.S. National Eye Institute
Department
Type
DUNS #
City
State
Country
United States
Zip Code

  Publications

Egwuagu, C E; Li, W; Yu, C-R et al. (2006) Interferon-gamma induces regression of epithelial cell carcinoma: critical roles of IRF-1 and ICSBP transcription factors. Oncogene 25:3670-9
Yang, Ying; Stopka, Tomas; Golestaneh, Nady et al. (2006) Regulation of alphaA-crystallin via Pax6, c-Maf, CREB and a broad domain of lens-specific chromatin. EMBO J 25:2107-18
Fan, Jianguo; Fariss, Robert N; Purkiss, Andrew G et al. (2005) Specific interaction between lens MIP/Aquaporin-0 and two members of the gamma-crystallin family. Mol Vis 11:76-87
Golestaneh, Nady; Fan, Jianguo; Fariss, Robert N et al. (2004) Lens major intrinsic protein (MIP)/aquaporin 0 expression in rat lens epithelia explants requires fibroblast growth factor-induced ERK and JNK signaling. J Biol Chem 279:31813-22
Ebong, Samuel; Chepelinsky, Ana B; Robinson, Michael L et al. (2004) Characterization of the roles of STAT1 and STAT3 signal transduction pathways in mammalian lens development. Mol Vis 10:122-31
Cui, Wenwu; Tomarev, Stanislav I; Piatigorsky, Joram et al. (2004) Mafs, Prox1, and Pax6 can regulate chicken betaB1-crystallin gene expression. J Biol Chem 279:11088-95
Fan, Jianguo; Donovan, Anna K; Ledee, Dolena R et al. (2004) gammaE-crystallin recruitment to the plasma membrane by specific interaction between lens MIP/aquaporin-0 and gammaE-crystallin. Invest Ophthalmol Vis Sci 45:863-71
Ebong, Samuel; Yu, Cheng-Rong; Carper, Deborah A et al. (2004) Activation of STAT signaling pathways and induction of suppressors of cytokine signaling (SOCS) proteins in mammalian lens by growth factors. Invest Ophthalmol Vis Sci 45:872-8
Drake, K Dawn; Schuette, Diana; Chepelinsky, Ana B et al. (2002) pH-Dependent channel activity of heterologously-expressed main intrinsic protein (MIP) from rat lens. FEBS Lett 512:199-204
Drake, K Dawn; Schuette, Diana; Chepelinsky, Ana B et al. (2002) Heterologous expression and topography of the main intrinsic protein (MIP) from rat lens. FEBS Lett 512:191-8

Showing the most recent 10 out of 13 publications