Abstract

The primary objective of this research is to understand how motile processes in photoreceptors and RPE cells are regulated by light, circadian, and morphogenetic signals, ie. to identify all steps in the regulatory pathways which lead from the physiological signals ultimately to the appropriate effector systems (ie. microtubule- or actin-based cytoskeletons) responsible for producing movement. This work emphasizes use of teleost retinomotor movements as a model system since powerful quantitative assays are available which permit analysis of the effects of extra- and intra-cellular regulators on these movements. Information gained from these retinomotor studies will be used to further our understanding of other photoreceptor and RPE motile processes crucial to retinal function in all species, such as phagocytosis and morphogenesis. Work in the last grant period showed that the extracellular messenger dopamine mimics light onset by inducing light-adaptive retinomotor movements in photoreceptors and RPE, and that intracellular pathways involving specific interplays of Ca++, cAMP, and protein kinase C contribute to regulating the actin- and microtubule-dependent processes which produce retinomotor movements. The present application proposes the following specific approaches to further clarify the roles of these agents in regulation of photoreceptor and RPE motility: 1) To ascertain whether dopamine and light have similar effects on photoreceptor and RPE cyclic nucleotide levels by determining the effects of light, darkness, and dopamine on cAMP and cGMP levels in isolated photoreceptor fragments (rod inner-outer segments, RIS-ROS, and cone inner-outer segments, CIS-COS) and in isolated RPE cells; 2) To investigate the roles of Ca++, cAMP, and specific protein kinases in regulating retinomotor movements in rods, cones, and RPE cells by further characterization of phorbolester effects and by extending lysed cell motile model studies to rods and RPE; 3) To investigate changes in protein phosphorylation in motile RIS-ROS, CIS-COS, and RPE cells that occur in response to light, dark, dopamine, Ca++, cAMP, and protein kinase C; 4) To characterize the cytoskeletal components of RIS-ROS, CIS-COS, and RPE cells using SDS PAGE, Western Blots, and immunolocalization; 5) To use immunocytochemistry to identify changes in distribution of cytoskeletal components during morphogenesis of photoreceptors and RPE.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Method to Extend Research in Time (MERIT) Award (R37)
Project #
4R37EY003575-14
Application #
2158857
Study Section
Special Emphasis Panel (NSS)
Project Start
1980-12-01
Project End
1998-11-30
Budget Start
1993-12-01
Budget End
1994-11-30
Support Year
14
Fiscal Year
1994
Total Cost
Indirect Cost

  Institution

Name
University of California Berkeley
Department
Biochemistry
Type
Schools of Arts and Sciences
DUNS #
094878337
City
Berkeley
State
CA
Country
United States
Zip Code
94704

  Publications

Dalal, Jasbir S; Stevens Jr, Stanley M; Alvarez, Sophie et al. (2011) Mouse class III myosins: kinase activity and phosphorylation sites. J Neurochem 119:772-84
Katti, Christiana; Dalal, Jasbir S; Dosé, Andrea C et al. (2009) Cloning and distribution of myosin 3B in the mouse retina: differential distribution in cone outer segments. Exp Eye Res 89:224-37
Salles, Felipe T; Merritt Jr, Raymond C; Manor, Uri et al. (2009) Myosin IIIa boosts elongation of stereocilia by transporting espin 1 to the plus ends of actin filaments. Nat Cell Biol 11:443-50
Lin-Jones, Jennifer; Sohlberg, Lorraine; Dose, Andrea et al. (2009) Identification and localization of myosin superfamily members in fish retina and retinal pigmented epithelium. J Comp Neurol 513:209-23
Lin-Jones, Jennifer; Burnside, Beth (2007) Retina-specific protein fascin 2 is an actin cross-linker associated with actin bundles in photoreceptor inner segments and calycal processes. Invest Ophthalmol Vis Sci 48:1380-8
Lee, Edwin S; Burnside, Beth; Flannery, John G (2006) Characterization of peripherin/rds and rom-1 transport in rod photoreceptors of transgenic and knockout animals. Invest Ophthalmol Vis Sci 47:2150-60
Lin-Jones, Jennifer; Parker, Ed; Wu, Mike et al. (2004) Myosin 3A transgene expression produces abnormal actin filament bundles in transgenic Xenopus laevis rod photoreceptors. J Cell Sci 117:5825-34
Lin-Jones, Jennifer; Parker, Ed; Wu, Mike et al. (2003) Disruption of kinesin II function using a dominant negative-acting transgene in Xenopus laevis rods results in photoreceptor degeneration. Invest Ophthalmol Vis Sci 44:3614-21
Dose, Andrea C; Hillman, David W; Wong, Cynthia et al. (2003) Myo3A, one of two class III myosin genes expressed in vertebrate retina, is localized to the calycal processes of rod and cone photoreceptors and is expressed in the sacculus. Mol Biol Cell 14:1058-73
Les Erickson, F; Corsa, Amoreena C; Dose, Andrea C et al. (2003) Localization of a class III myosin to filopodia tips in transfected HeLa cells requires an actin-binding site in its tail domain. Mol Biol Cell 14:4173-80

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