Abstract

Three highly expressed proteins involved in light signaling in retinal rod photoreceptors, transducin, recoverin and arrestin, localize to different photoreceptor compartments depending on the conditions of ambient illumination. This transport is important for adjusting photoreceptor light sensitivity. Moreover, it plays a role in protecting rod photoreceptors from damage caused by continual stimulation from light levels we experience every day, and from aberrant photoreceptor activity that may underlie many congenital retinal degenerative diseases. Yet the mechanisms by which these proteins are localized to photoreceptor compartments, by which they are transported among compartments and by which changes in ambient light levels initiate this re-localization are not known. ? ? We have developed new methods using multiphoton microscopy to directly examine local, compartment-specific behavior of the proteins and local changes in signaling molecules within living, functioning photoreceptors. Using these new methods we will examine the: ? ? Aim 1: Mechanisms underlying protein localization to rod photoreceptor compartments. ? Aim 2: Mode of signal-dependant protein transport between rod compartments. ? Aim 3: Signals that initiate protein transport. ? ? Experiments in aims 1 and 2 will quantitatively examine the local and long distance mobilities of the proteins fused with a variant of the green fluorescent protein, photoactivatable GFP, to identify the mechanisms of localization and modes of transport. We will then take what we have learned from these studies and construct a quantitative model to test if the mobility parameters are sufficient to explain the patterns of protein localization and light-driven transport. Experiments in aim 3 are designed to identify the signals that tell the proteins to move using newly developed, expressible signal transduction sensors. ? ? Understanding the mechanisms of light-induced protein transport could reveal experimental strategies for testing adaptive or protective roles of transport directly and may lead to strategies for therapeutic intervention to slow or reverse photoreceptor degeneration in congenital disease. The proposed work fits into the National Plan for Eye and Vision Research under the Retinal Disease Program. ? ? ?

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Research Project (R01)
Project #
5R01EY018421-02
Application #
7486809
Study Section
Biology and Diseases of the Posterior Eye Study Section (BDPE)
Program Officer
Mariani, Andrew P
Project Start
2007-09-01
Project End
2012-08-31
Budget Start
2008-09-01
Budget End
2009-08-31
Support Year
2
Fiscal Year
2008
Total Cost
$346,185
Indirect Cost

  Institution

Name
Upstate Medical University
Department
Ophthalmology
Type
Schools of Medicine
DUNS #
058889106
City
Syracuse
State
NY
Country
United States
Zip Code
13210

  Publications

Lee, Sungsu; Tan, Han Yen; Geneva, Ivayla I et al. (2018) Actin filaments partition primary cilia membranes into distinct fluid corrals. J Cell Biol 217:2831-2849
Laprell, Laura; Tochitsky, Ivan; Kaur, Kuldeep et al. (2017) Photopharmacological control of bipolar cells restores visual function in blind mice. J Clin Invest 127:2598-2611
Geneva, Ivayla I; Tan, Han Yen; Calvert, Peter D (2017) Untangling ciliary access and enrichment of two rhodopsin-like receptors using quantitative fluorescence microscopy reveals cell-specific sorting pathways. Mol Biol Cell 28:554-566
Najafi, Mehdi; Calvert, Peter D (2015) Measurements of rhodopsin diffusion within signaling membrane microcompartments in live photoreceptors. Methods Mol Biol 1271:309-23
Haeri, Mohammad; Calvert, Peter D; Solessio, Eduardo et al. (2013) Regulation of rhodopsin-eGFP distribution in transgenic xenopus rod outer segments by light. PLoS One 8:e80059
Najafi, Mehdi; Calvert, Peter D (2012) Transport and localization of signaling proteins in ciliated cells. Vision Res 75:11-8
Najafi, Mehdi; Haeri, Mohammad; Knox, Barry E et al. (2012) Impact of signaling microcompartment geometry on GPCR dynamics in live retinal photoreceptors. J Gen Physiol 140:249-66
Najafi, Mehdi; Maza, Nycole A; Calvert, Peter D (2012) Steric volume exclusion sets soluble protein concentrations in photoreceptor sensory cilia. Proc Natl Acad Sci U S A 109:203-8
Calvert, Peter D; Schiesser, William E; Pugh Jr, Edward N (2010) Diffusion of a soluble protein, photoactivatable GFP, through a sensory cilium. J Gen Physiol 135:173-96