The objective of our research is to examine the molecular basis of photoreception and transduction in photoreceptor cells. In this five year plan, we propose experiments addressing the following two specific aims: 1. In vitro expression and mutagenesis of recombinant DNA fragments encoding the molecular photoreceptor rhodopsin will be applied to examine its structure and activity. Expression in both E. coli and mammalian cells is proposed. Rhodopsin and the corresponding mutant receptors will be examined for properties of structural folding, regulation of absorption wavelength, and functional interactions of the cytoplasmic domains with components of the cGMP cascade, e.g. G-protein, opsin kinase, and 48K-protein. 2. Techniques for isolation and characterization of two photoreceptor plasma membrane macromolecules, the Na+/Ca++ exchanger and the cGMP/light-dependent ion channel, that control cell signaling are outlined. We propose to identify and characterize the genes and mRNA encoding each of the molecules, to identify the predicted protein structure from genetic information obtained, and eventually to use in vitro expression and mutagenesis to study their structure and functional activities. Our long term research objective is to develop recombinant DNA techniques to supplement traditional biochemical isolation/characterization methods for study of proteins functional in visual transduction. As noted in aim 2, such techniques would enable us to study proteins that are important for visual function but present in only few copies per cell. In addition, we wish to initiate studies that will enable us to study the expression of genes encoding visual transduction proteins in the retina. These studies contribute basic information about macromolecules in photoreceptors that are somehow affected by genetic defects in retinitis pigmentosa or retinoblastomas.

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Research Project (R01)
Project #
5R01EY004801-10
Application #
3259336
Study Section
Visual Sciences B Study Section (VISB)
Project Start
1988-01-01
Project End
1991-06-30
Budget Start
1990-07-01
Budget End
1991-06-30
Support Year
10
Fiscal Year
1990
Total Cost
Indirect Cost
Name
University of Chicago
Department
Type
Schools of Medicine
DUNS #
225410919
City
Chicago
State
IL
Country
United States
Zip Code
60637
Applebury, M L; Farhangfar, F; Glosmann, M et al. (2007) Transient expression of thyroid hormone nuclear receptor TRbeta2 sets S opsin patterning during cone photoreceptor genesis. Dev Dyn 236:1203-12
Fasick, Jeffry I; Applebury, Meredithe L; Oprian, Daniel D (2002) Spectral tuning in the mammalian short-wavelength sensitive cone pigments. Biochemistry 41:6860-5
Applebury, M L; Antoch, M P; Baxter, L C et al. (2000) The murine cone photoreceptor: a single cone type expresses both S and M opsins with retinal spatial patterning. Neuron 27:513-23
Wilson, C J; Copeland, R A (1997) Spectroscopic characterization of arrestin interactions with competitive ligands: study of heparin and phytic acid binding. J Protein Chem 16:755-63
Wagner, E; McCaffery, P; Mey, J et al. (1997) Retinoic aid increases arrestin mRNA levels in the mouse retina. FASEB J 11:271-5
Aparicio, J G; Applebury, M L (1995) The bovine photoreceptor outer segment guanylate cyclase: purification, kinetic properties, and molecular size. Protein Expr Purif 6:501-11
Wood, R L; Park, K H; Gierow, J P et al. (1994) Immunogold localization of prolactin in acinar cells of lacrimal gland. Adv Exp Med Biol 350:75-7
Pierce, M E; Sheshberadaran, H; Zhang, Z et al. (1993) Circadian regulation of iodopsin gene expression in embryonic photoreceptors in retinal cell culture. Neuron 10:579-84
Lem, J; Applebury, M L; Falk, J D et al. (1991) Tissue-specific and developmental regulation of rod opsin chimeric genes in transgenic mice. Neuron 6:201-10
Leser, G P; Nicoll, D A; Applebury, M L (1991) Distinctive properties of the purified Na-Ca exchanger from rod outer segments. Ann N Y Acad Sci 639:222-33

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