TY - JOUR KW - Animals KW - Arrestin KW - Binding Sites KW - Mice KW - Mice, Inbred C57BL KW - Mice, Knockout KW - Phosphorylation KW - Receptors, G-Protein-Coupled KW - Retinal Rod Photoreceptor Cells KW - Rhodopsin KW - Serine KW - Threonine AU - Anthony Azevedo AU - Thuy Doan AU - Hormoz Moaven AU - Iza Sokal AU - Faiza Baameur AU - Sergey Vishnivetskiy AU - Kristoff Homan AU - John Tesmer AU - Vsevolod Gurevich V AU - Jeannie Chen AU - Fred Rieke AB -

Rod photoreceptors generate measurable responses to single-photon activation of individual molecules of the G protein-coupled receptor (GPCR), rhodopsin. Timely rhodopsin desensitization depends on phosphorylation and arrestin binding, which quenches G protein activation. Rhodopsin phosphorylation has been measured biochemically at C-terminal serine residues, suggesting that these residues are critical for producing fast, low-noise responses. The role of native threonine residues is unclear. We compared single-photon responses from rhodopsin lacking native serine or threonine phosphorylation sites. Contrary to expectation, serine-only rhodopsin generated prolonged step-like single-photon responses that terminated abruptly and randomly, whereas threonine-only rhodopsin generated responses that were only modestly slower than normal. We show that the step-like responses of serine-only rhodopsin reflect slow and stochastic arrestin binding. Thus, threonine sites play a privileged role in promoting timely arrestin binding and rhodopsin desensitization. Similar coordination of phosphorylation and arrestin binding may more generally permit tight control of the duration of GPCR activity.

BT - Elife DA - 2015 Apr 24 DO - 10.7554/eLife.05981 J2 - Elife LA - eng N2 -

Rod photoreceptors generate measurable responses to single-photon activation of individual molecules of the G protein-coupled receptor (GPCR), rhodopsin. Timely rhodopsin desensitization depends on phosphorylation and arrestin binding, which quenches G protein activation. Rhodopsin phosphorylation has been measured biochemically at C-terminal serine residues, suggesting that these residues are critical for producing fast, low-noise responses. The role of native threonine residues is unclear. We compared single-photon responses from rhodopsin lacking native serine or threonine phosphorylation sites. Contrary to expectation, serine-only rhodopsin generated prolonged step-like single-photon responses that terminated abruptly and randomly, whereas threonine-only rhodopsin generated responses that were only modestly slower than normal. We show that the step-like responses of serine-only rhodopsin reflect slow and stochastic arrestin binding. Thus, threonine sites play a privileged role in promoting timely arrestin binding and rhodopsin desensitization. Similar coordination of phosphorylation and arrestin binding may more generally permit tight control of the duration of GPCR activity.

PY - 2015 T2 - Elife TI - C-terminal threonines and serines play distinct roles in the desensitization of rhodopsin, a G protein-coupled receptor. VL - 4 SN - 2050-084X ER -