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The Journal of Neuroscience, July 9, 2003, 23(14):6152-6160
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GRK1-Dependent Phosphorylation of S and M Opsins and Their Binding to Cone Arrestin during Cone Phototransduction in the Mouse Retina
Xuemei Zhu,1 Bruce Brown,1 Aimin Li,1 Alan J. Mears,2,3 Anand Swaroop,2,3 andCheryl M. Craft1 1The Mary D. Allen Laboratory for Vision Research, Doheny Eye Institute, Department of Cell and Neurobiology, the Keck School of Medicine of the University of Southern California, Los Angeles, California 90089-9112, and Departments of 2Ophthalmology and Visual Sciences and 3Human Genetics, University of Michigan, Ann Arbor, Michigan 48105
Abstract
Top
Abstract
Introduction
The shutoff mechanisms of the rod visual transduction cascade involve G-protein-coupled receptor (GPCR) kinase 1 (GRK1) phosphorylation of light-activated rhodopsin (R*) followed by rod arrestin binding. Deactivation of the cone phototransduction cascade in the mammalian retina is delineated poorly. In this study we sought to explore the potential mechanisms underlying the quenching of the phototransduction cascade in cone photoreceptors by using mouse models lacking rods and/or GRK1. Using the "pure-cone" retinas of the neural retina leucine zipper (Nrl) knock-out (KO, -/-) mice (Mears et al., 2001), we have demonstrated the light-dependent, multi-site phosphorylation of both S and M cone opsins by in situ phosphorylation and isoelectric focusing. Immunoprecipitation with affinity-purified polyclonal antibodies against either mouse cone arrestin (mCAR) or mouse S and M cone opsins revealed specific binding of mCAR to light-activated, phosphorylated cone opsins. To elucidate the potential role of GRK1 in cone opsin phosphorylation, we created Nrl and Grk1 double knock-out (Nrl-/-Grk1-/-) mice by crossing the Nrl-/- mice with Grk1-/- mice (Chen et al., 1999
Key words: cone opsin; phosphorylation; cone arrestin; phototransduction; coimmunoprecipitation; mouse retina
Introduction
Phototransduction mechanisms are well documented in rod photoreceptors and now are regarded as a classic model system of G-protein-coupled receptor (GPCR) signaling (Baylor, 1996In rod photoreceptors the timely deactivation of photoactivated rhodopsin (R*) by GPCR kinase 1 (GRK1)-mediated R* phosphorylation followed by rod arrestin binding is critical for effective rod vision (Wilden et al., 1986a
In this study we provide direct biochemical evidence of cone opsin phosphorylation and CAR binding to phosphorylated cone opsins during phototransduction, using the neural retina leucine zipper (Nrl) knock-out (KO, -/-) mice (Mears et al., 2001
Using the pure-cone retinas of the Nrl-/- mice, we demonstrate that both S and M cone opsins are phosphorylated after light exposure and that CAR selectively binds to light-activated, phosphorylated cone opsins. We also created Nrl and Grk1 double KO (Nrl-/-Grk1-/-) mice by crossing the Nrl-/- with the Grk1-/- mice (Chen et al., 1999
Materials and Methods
Animals. C57BL/6J mice were purchased originally from the Jackson Laboratories (Bar Harbor, ME). The Nrl -/- (Mears et al., 2001Antisera generation. Rabbit antisera against the peptides of mouse S opsin (residues 1–11, MSGEDDFYLFQ) and M opsin (residues 3–16, QRLTGEQTLDHYED) were made for our research project by Zymed Laboratories (South San Francisco, CA) and affinity-purified against the peptides with the SulfoLink kit (Pierce, Rockford, IL) as previously described (Zhu and Craft, 2000
Immunoblot analysis. Total retinal homogenates from normal C57 mice were used for immunoblot analysis with either anti-S or anti-M opsin antibody and HRP-conjugated anti-rabbit secondary antibody and were visualized by an enhanced chemiluminescence (ECL) kit (Amersham Biosciences, Arlington Heights, IL) (Craft et al., 1998
Immunohistochemistry. The protocol for immunohistochemistry on mouse retinal sections has been published previously (Zhu et al., 2002b
For immunofluorescent triple labeling, the retinal sections were incubated with sequential primary antibodies, including a rabbit polyclonal [anti-M opsin, anti-S opsin, or anti-mCAR LUMIJ (Zhu et al., 2002b
For retinal whole mounts a lens-attached retina was dissected from the sclera, choroid, and pigment epithelium and was fixed in 4% paraformaldehyde in PBS overnight on a rotator at 4°C. Tissues then were washed three times and subjected to double-immunofluorescent staining. After blocking, the retinas were incubated with the first primary antibody (either an anti-S opsin or anti-M opsin polyclonal antibody) at 1:1000 dilution and then reacted with a fluorescein anti-rabbit IgG. Because the second primary antibody was also from rabbit, a microwave method (Tornehave et al., 2000
Detection of soluble and membrane-bound mCAR. WT and Grk1 -/- mice were killed either mid-day under room light (after light exposure for at least 2 hr) or dark-adapted overnight and killed in the dark under infrared (IR) light. Both retinas from the same mouse were homogenized gently (not sonicated) in 125 µl of 50 mM sodium phosphate buffer, pH 6.8, either under room light or under IR light. Retinal homogenates were centrifuged at 13,000 rpm in a refrigerated microfuge either in the light or in the dark for 10 min at 4°C. The supernatants were removed immediately, the pellets were resuspended and homogenized in 125 µl of buffer, and all samples were treated with SDS sample buffer either in the light or dark. An equal volume of proteins was resolved on replicate 11.5% SDS-PAGE gels and transferred to polyvinylidene difluoride (PVDF) membranes (Immobilon, Millipore, Bedford, MA), which were incubated in either a polyclonal mCAR (LUMIJ) (Zhu et al., 2002b
In situ phosphorylation of opsins in mouse retinas. Adult WT, Nrl -/-, and Nrl -/-Grk1 -/- mice were dark-adapted overnight and killed in the dark. The retinas were dissected under IR light; each was put into 0.5 ml of phosphate-free Krebs' buffer [consisting of (in mM): 100 HEPES, pH 7.4, 10 glucose, 120 NaCl, 5 KCl, 1 MgSO4, 1 CaCl2] containing 0.6 mCi (1.25 mCi/ml) 32P orthophosphate and was incubated for 30 min at RT in the dark. The buffer was changed to nonradioactive Krebs', and one retina of each strain was homogenized in SDS sample buffer in the dark while the other retina was exposed to direct bright sunlight, which is
8000 foot candle (fc), for 10 min before homogenization. The proteins were resolved on an 11.5% SDS-PAGE gel and transferred to a PVDF membrane. The membrane was exposed first to a Storm PhosphorImager screen (Molecular Dynamics) to observe opsin phosphorylation, followed by incubation in antibodies to mouse M opsin, S opsin, or rhodopsin (1D4) to observe the quantity and location of each opsin relative to the radioactive phosphate (32P).
Separation of phosphorylated opsin species by isoelectric focusing. Two Nrl -/- (20–23 weeks old) and two age-matched WT mice were dark-adapted overnight. The mice were killed, and the retinas were dissected under IR light. Two retinas from each strain were exposed on ice to direct bright sunlight (
Immunoprecipitation. Four adult Nrl -/- or Nrl -/-Grk1 -/- mice were dark-adapted overnight and killed; the retinas were dissected under IR light. The eight retinas were put into two tubes (4 retinas each) labeled dark and light, each containing 0.5 ml of phosphate-free Krebs' buffer containing 0.6 mCi 32P orthophosphate, and were incubated at RT for 30 min. The retinas were washed and put in 1 ml of Krebs' buffer lacking the 32P orthophosphate. The light tube was uncapped and exposed to direct bright sunlight (
Immunoprecipitation (IP) was performed with the Protein A-Agarose IP kit (KPL, Gaithersburg, MD). Four hundred microliters of the retinal supernatants (dark or light) were mixed with 400 µl of a 50% suspension of protein A-agarose in lysis buffer with no protease inhibitors or okadaic acid and rotated at 4°C for 1 hr to preclear the samples (remove proteins from the lysates that bind nonspecifically to the resin). The samples were centrifuged at 14,000 x g for 20 sec, and the agarose pellet was discarded. The precleared dark or light supernatant (150 µl) was mixed with 5 µg of affinity-purified polyclonal antibodies against mCAR, S opsin, M opsin, or CRX (control) and was incubated with end-over-end mixing overnight at 4°C. Fifty microliters of a 50% suspension of protein A-agarose in lysis buffer with no protease inhibitors or okadaic acid were added, and the tubes were rotated in the dark for 1.5 hr at 4°C. The immunoprecipitates were collected by centrifugation at 14,000 x g for 20 sec, washed one time with 0.5 ml of ice-cold lysis buffer, solubilized in 60 µl of SDS-PAGE sample buffer, electrophoresed on an 11.5% SDS-PAGE gel, and transferred to an Immobilon membrane. The membrane was exposed to a Storm PhosphorImager screen (Molecular Dynamics) to detect radioactive proteins before being subjected to immunoblot analysis with anti-mCAR (LUMIJ), S, or M opsin antibodies.
Results
Membrane association of mCAR in a light-dependent and GRK1-dependent manner
To explore whether CAR contributes to quenching light-activated cone opsins in the mammalian retina, we analyzed the redistribution of mCAR to retinal membranes in response to light. The distribution of mCAR and mouse SAG (mSAG) was analyzed by immunoblot analysis of membrane and soluble proteins of retinal homogenates from either light- or dark-adapted mice. Figure 1 shows that 50% of the mCAR protein is in the membrane fraction (pellet) in the dark-adapted retina, whereas 81% is in the membrane fraction in the light-adapted retina (Fig. 1A), similar to the distribution of mSAG, which is mostly in the soluble fraction in the dark-adapted retina but redistributes to the membranes when exposed to light (Fig. 1C). These results are consistent with our previous observation that a portion of the mCAR immunoreactivity translocates to the cone outer segments in a light-dependent manner (Zhu et al., 2002b
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Figure 1. Light- and GRK1-dependent membrane association of mCAR. Adult WT or Grk1 -/- mice were killed either at mid-day in the light or dark-adapted overnight and killed in the dark under IR light. The retinas were dissected under room light from light-adapted mice (L) or under IR light from dark-adapted mice (D) and were homogenized. The supernatants (Sup; soluble fraction) and pellets (membrane fraction) were separated by centrifugation, and the pellets were resuspended in the same volume of buffer. Equal volumes of proteins were resolved on replicate 11.5% SDS-PAGE gels and transferred to PVDF membranes, which were detected with the mCAR (LUMIJ) or rod arrestin (mSAG, C10C10) antibodies with an ECL kit. In each panel a representative immunoblot and a histogram representing quantitative data (mean ± SEM) from at least three immunoblots are shown.
Generation and characterization of anti-mouse S and M opsin antibodies
To facilitate our cone opsin phosphorylation studies, we generated rabbit polyclonal antibodies against peptides derived from mouse S and M opsin peptide sequences and affinity-purified them against their respective peptide. Immunoblot analysis of retinal homogenates from normal C57BL/6J mice with the two affinity-purified antibodies identified a single band of the predicted molecular weight of the respective opsin, i.e., 37.5 kDa for S opsin and 39 kDa for M opsin (Fig. 2A,B). Minor bands were seen after a longer film exposure time (data not shown). To verify the specificity of the antibodies, we did a peptide-blocking experiment by incubating the primary antibody with 100 times excess (mol peptide/mol specific antibody) of the specific peptide used to generate the antibody and found that only the major band was blocked completely by the peptide (data not shown). When the primary antibody was omitted and only the secondary antibody was incubated with the blot, all of the minor bands were observed, but the major one was missing (data not shown), suggesting that the minor bands were caused by cross-reaction with the secondary antibody.
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Figure 2. Characterization of anti-mouse S opsin (A) and M opsin (B) antibodies by Western blotting and immunohistochemistry. Western blot analysis was performed with normal adult C57BL/6J mouse whole retinal homogenate, and immunohistochemistry was done on C57BL/6J mouse retinal frozen sections. Cone photoreceptor cells were labeled with biotinylated peanut agglutinin and visualized with Texas Red-avidin D in red (b,e). S and M opsins were labeled with anti-S and anti-M opsin polyclonal antibodies, respectively, and visualized with fluorescein label in green (a, d). Dual immunofluorescence labeling verified both S and M opsin immunoreactivities localized to cone cells (c, f). OS, Outer segments; IS, inner segments; ONL, outer nuclear layer. Scale bar, 20 µm.
Immunohistochemistry that used mouse retinal sections revealed specificity of both antibodies for cone photoreceptor outer segments (Fig. 2A,B). The cone outer segment staining was blocked completely by the specific peptide used to generate the antibody (data not shown).
Both GRK1 and mCAR are expressed in both S and M cone photoreceptors
Previous studies have shown the expression of both GRK1 (Lyubarsky et al., 2000
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Figure 3. Localization of GRK1 in both S and M cone photoreceptors of the normal mouse retina. Adult C57 mouse retinal frozen sections were triple labeled fluorescently with the GRK1-specific monoclonal antibody D11 (A, E, I), the fluorescent nuclear dye PI (red in C, G, K), and the polyclonal anti-S opsin (B), anti-M opsin (F), or anti-mCAR (LUMIJ, J). Overlay of A and B with PI staining (C) or E and F with PI staining (G) reveals colocalization of GRK1 with both S opsins (C) and M opsins (G) in the cone outer segments, and overlay of I and J with PI staining (K) shows colocalization of GRK1 with mCAR also in the cone outer segments. A phase-contrast image (D, H, L) also is shown for each section. Note that the staining of GRK1 and S and M opsins is restricted to the outer segments (OS), whereas the staining of mCAR is diffused throughout the cone photoreceptors but condensed in the cone outer segments and the synaptic terminals. IS, Inner segments; ONL, outer nuclear layer; OPL, outer plexiform layer. Scale bar, 20 µm.
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Figure 4. Localization of mCAR in both S and M cone photoreceptors of the normal mouse retina. Adult C57 mouse retinal whole mounts were double labeled immunofluorescently with either anti-S (A) or anti-M opsin antibody (D) and the anti-mCAR antibody LUMIJ (B, E). Overlay of A and B (C) or D and E (F) reveals colocalization of mCAR with both S and M opsins in the cone outer segments.
In the Nrl-/- mouse retina (Fig. 5) GRK1 is colocalized with either S or M opsin to the short outer segments of all photoreceptors, whereas mCAR is expressed throughout the whole photoreceptor layer, with the most intense staining in the outer segments and the synaptic terminals. mCAR also is colocalized with both S and M opsins in the outer segments of the Nrl-/- retinas.
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Figure 5. GRK1 and mCAR both are expressed in all photoreceptors of the Nrl -/- mouse retina. Adult Nrl-/- mouse retinal frozen sections were double labeled fluorescently with D11 (A) + anti-S opsin (B), D11 (E) + anti-M opsin (F), LUMIJ (I) + anti-S opsin (J), and LUMIJ (M) + anti-M opsin (N). Overlay of A and B (C) or E and F (G) reveals colocalization of GRK1 with both S opsins (C) and M opsins (G) in the shortouter segments, and overlay of I and J (K) or M and N (O) shows colocalization of mCAR with both S and M opsins also in the outer segments. Note that the staining of GRK1 and S and M opsins is restricted to the outer segment layer (OS), whereas the staining of mCAR is diffused throughout the photoreceptors but condensed in the outer segments and the synaptic terminals. A phase-contrast image (D, H, L, P) is shown for each section. IS, Inner segments; ONL, outer nuclear layer; OPL, outer plexiform layer. Scale bar, 20 µm.
Light- and GRK1-dependent phosphorylation of cone opsins
To determine cone opsin phosphorylation after light exposure, we examined the light-dependent incorporation of 32P orthophosphate into the pure-cone retinas of the Nrl-/- mice. Exposure of isolated intact retinas from Nrl-/- mice to bright sunlight (
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Figure 6. In situ light-dependent phosphorylation of opsins ex vivo. A, In situ phosphorylation of opsins. WT, Nrl -/-, and Nrl -/-Grk1 -/- mice were dark-adapted overnight and killed. The retinas were dissected under IR light and incubated in phosphate-free Krebs' buffer containing 1.25 mCi/ml 32P orthophosphate for 30 min at RT in the dark. One retina of each strain was homogenized in SDS sample buffer in the dark (D) while the other retina was exposed to bright sunlight (L) for 10 min before homogenization. The proteins were resolved on an 11.5% SDS-PAGE gel and transferred to a PVDF membrane. Opsin phosphorylation was detected by autoradiography on a PhosphorImager screen. B, Immunoblot analysis of the same membrane in A, using polyclonal antibodies to mouse S or M opsin or the rhodopsin monoclonal antibody 1D4, sequentially, to observe the quantity and location of the opsins relative to the radioactive phosphate (32P) identified in A. Note the slightly higher molecular weight of the phosphorylated as compared with the unphosphorylated species of S and M opsin and rhodopsin.
To investigate the role of GRK1 in cone opsin phosphorylation, as indicated by the analysis of the Grk1-/- mice (Lyubarsky et al., 2000
Phosphorylation of cone opsins at multiple sites
Recent evidence shows that multiple phosphorylation of rhodopsin at the C terminus is necessary for rapid and reproducible deactivation of rhodopsin (Mendez et al., 2000
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Figure 7. Multiple phosphorylation of S and M opsins ex vivo. A, Alignment of C-terminal sequences for mouse rhodopsin and S and M opsins. The conserved amino acids among all three opsins are indicated with an asterisk. Potential phosphorylation sites (serine and threonine residues) are underlined. B, Separation of S and M opsin and rhodopsin and their phosphorylated species by isoelectric focusing (IEF). Retinas from Nrl -/- (S and M opsins) and WT mice (rhodopsin) were dissected under infrared light, exposed to direct bright sunlight (
Coimmunoprecipitation of mCAR with light-activated, phosphorylated cone opsins
To examine whether mCAR interacts with light-activated, phosphorylated cone opsins, we performed IP on Nrl-/- mouse retinal proteins with either the mCAR antibody or cone opsin antibodies as well as the CRX antibody, which is also an affinity-purified rabbit polyclonal antibody (Zhu and Craft, 2000-mCAR) and the anti-cone opsin antibodies (
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Figure 8. Coimmunoprecipitation of mCAR with light-activated, phosphorylated cone opsins. A, Coimmunoprecipitation of mCAR with phosphorylated S and M opsins from light-exposed Nrl -/- mouse retinas. Nrl -/- mouse retinas were dissected under IR light from dark-adapted mice and incubated in phosphate-free Krebs' buffer containing 1.25 mCi/ml 32P orthophosphate for 30 min. Four retinas were exposed to bright sunlight (
In the Nrl-/-Grk1-/- mouse retina (Fig. 8B), where no cone opsin phosphorylation occurred after light activation (Fig. 6A), no 32P-labeled proteins were precipitated by any of the antibodies. The mCAR antibody did not pull down either cone opsin, nor did the cone opsin antibodies pull down mCAR either in the light-exposed or dark-adapted retina, although each antibody pulled down equal amounts of its corresponding protein from both the light-exposed and dark-adapted retinas (Fig. 8B). These results further confirm that the phosphorylated protein bands in the 32P incorporation experiments (Fig. 6A) and in the coimmunoprecipitation experiments with the Nrl-/- mice (Fig. 8A) are GRK1-phosphorylated cone opsins and that the binding of mCAR to cone opsins is phosphorylation-dependent, similar to rod arrestin binding to phosphorylated R*.
Discussion
In the vertebrate retina two distinct cell populations of photoreceptors, rods and cones, coexist. Rods are specialized for dim light vision, whereas cones provide high-acuity color vision. Although cones comprise only 5% of photoreceptors in the human retina, they are far more important than rods for vision in daylight. Even at night our world is flooded with enough artificial light so that our cones can function, and we can see clearly in color. Despite its importance in vision the cone phototransduction cascade and its underlying molecular mechanisms are poorly understood. In this study we aimed to explore the potential involvement of opsin phosphorylation and CAR binding in the cone phototransduction cascade, using mouse models lacking rods and/or GRK1.Cone opsin phosphorylation in the mammalian retina
Two critical events, receptor phosphorylation and arrestin binding, participate in the deactivation of GPCRs (Freedman and Lefkowitz, 1996Cone opsins from the all-cone retina of lizard, from the cone-dominant retina of chicken, and from the rod-dominant retina of carp are phosphorylated in vitro either by the endogenous kinase or by bovine GRK1 (Walter et al., 1986
GRK1 is responsible for light-dependent cone opsin phosphorylation in the mouse retina
Seven distinct mammalian GRKs, each differing in tissue distribution and in regulatory properties, have been identified to date. Among these enzymes GRK1 is involved in phototransduction. Proof that GRK1 phosphorylation of R* is required for normal inactivation of R* in vivo has come from single-cell recordings of photoresponses in rods expressing mutant rhodopsin lacking the C terminus (Chen et al., 1995GRK1 is localized in both rod and cone photoreceptors in many species, including the rod-dominant human, monkey, and mouse (Zhao et al., 1998
In contrast to the Grk1-/- mouse phenotype, human patients with Grk1 null mutation have either normal or slightly abnormal photopic vision (Cideciyan et al., 1998
The role of GRK1 in rods is to inactivate R* that, in concert with regeneration, leads to the recovery of sensitivity (Cideciyan et al., 1998
CAR is involved in the cone phototransduction cascade
Members of the arrestin family are involved in GPCR desensitization, internalization, and GPCR-mediated activation of MAPK pathways. In the rod photoreceptor the rod arrestin binding after receptor phosphorylation is necessary to complete the quench of the light-activated phototransduction cascade (Wilden et al., 1986bTo elucidate further the function of CAR, we are creating mCAR KO mice. Characterization of the morphological, biochemical, and electrophysiological phenotypes of these mice will clarify the physiological role of CAR in the shutoff of cone phototransduction as well as verify its other functions in both the retina and the pineal gland.
Footnotes
Received Jan. 16, 2003; revised May. 20, 2003; accepted May. 23, 2003.These studies were supported, in part, by National Institutes of Health/National Eye Institute Grants EY00395 (R.N.L. and C.M.C.) and EY11115 (A.S.), grants from Core Vision Research Center (EY03040 to Doheny Eye Institute and EY07003 to University of Michigan), the Smith Endowment for Neurogenetic Research, the Foundation Fighting Blindness, and Research to Prevent Blindness. Postdoctoral support was provided by generous contributions from the Tony Gray Foundation and Dorie and Fred Miller. C.M.C. is the Mary D. Allen Chair for Vision Research, Doheny Eye Institute. We thank Dr. Ching-Kang Chen for providing the Grk1-/- mice for our studies. We also thank Drs. Jeannie Chen, Anna Mendez, and Angela Roca for helpful suggestions on the phosphorylation experiments and for critical reading of this manuscript.
This manuscript is dedicated to Mary D. Allen for her generous support of our program in vision research and Dr. Richard N. Lolley, our lifetime collaborator.
Correspondence should be addressed to Dr. Cheryl M. Craft, Mary D. Allen Chair for Vision Research, Doheny Eye Institute, Professor and Chair, Department of Cell and Neurobiology, The Keck School of Medicine of the University of Southern California, 1333 San Pablo Street, BMT 401, Los Angeles, CA 90033. E-mail: ccraft{at}usc.edu.
Copyright © 2003 Society for Neuroscience 0270-6474/03/236152-09$15.00/0
References
Abdulaeva G, Hargrave PA, Smith WC (1995) The sequence of arrestins from rod and cone photoreceptors in the frogs Rana catesbeiana and Rana pipiens. Localization of gene transcripts by reverse-transcription polymerase chain reaction on isolated photoreceptors. Eur J Biochem 234: 437–442.[Medline]
Arshavsky V, Antoch MP, Philippov PP (1987) On the role of transducin GTPase in the quenching of a phosphodiesterase cascade of vision. FEBS Lett 224: 19–22.[Medline]
Baylor D (1996) How photons start vision. Proc Natl Acad Sci USA 93: 560–565.
[Abstract/Free Full Text] Baylor DA, Burns ME (1998) Control of rhodopsin activity in vision. Eye 12: 521–525.
Baylor DA, Lamb TD, Yau KW (1979) The membrane current of single rod outer segments. J Physiol (Lond) 288: 589–611.
[Abstract/Free Full Text] Bessant DA, Payne AM, Mitton KP, Wang QL, Swain PK, Plant C, Bird AC, Zack DJ, Swaroop A, Bhattacharya SS (1999) A mutation in NRL is associated with autosomal dominant retinitis pigmentosa. Nat Genet 21: 355–356.[Web of Science][Medline]
Carter-Dawson LD, LaVail MM (1979) Rods and cones in the mouse retina. I. Structural analysis using light and electron microscopy. J Comp Neurol 188: 245–262.[Web of Science][Medline]
Chen CK, Burns ME, Spencer M, Niemi GA, Chen J, Hurley JB, Baylor DA, Simon MI (1999) Abnormal photoresponses and light-induced apoptosis in rods lacking rhodopsin kinase. Proc Natl Acad Sci USA 96: 3718–3722.
[Abstract/Free Full Text] Chen CK, Zhang K, Church-Kopish J, Huang W, Zhang H, Chen YJ, Frederick JM, Baehr W (2001) Characterization of human GRK7 as a potential cone opsin kinase. Mol Vis 7: 305–313.[Web of Science][Medline]
Chen J, Makino CL, Peachey NS, Baylor DA, Simon MI (1995) Mechanisms of rhodopsin inactivation in vivo as revealed by a COOH-terminal truncation mutant. Science 267: 374–377.
[Abstract/Free Full Text] Cideciyan AV, Zhao X, Nielsen L, Khani SC, Jacobson SG, Palczewski K (1998) Null mutation in the rhodopsin kinase gene slows recovery kinetics of rod and cone phototransduction in man. Proc Natl Acad Sci USA 95: 328–333.
[Abstract/Free Full Text] Cideciyan AV, Jacobson SG, Gupta N, Osawa S, Locke KG, Weiss ER, Wright AF, Birch DG, Milam AH (2003) Cone deactivation kinetics and GRK1/GRK7 expression in enhanced S cone syndrome caused by mutations in NR2E3. Invest Ophthalmol Vis Sci 44: 1268–1274.
[Abstract/Free Full Text] Craft CM, Whitmore DH (1995) The arrestin superfamily: cone arrestins are a fourth family. FEBS Lett 362: 247–255.[Web of Science][Medline]
Craft CM, Whitmore DH, Wiechmann AF (1994) Cone arrestin identified by targeting expression of a functional family. J Biol Chem [Erratum (1994) 269:17756] 269: 4613–4619.
[Abstract/Free Full Text] Craft CM, Xu J, Slepak VZ, Zhan-Poe X, Zhu X, Brown B, Lolley RN (1998) PhLPs and PhLOPs in the phosducin family of G
binding proteins. Biochemistry 37: 15758–15772.[Medline]
Fain GL, Matthews HR, Cornwall MC, Koutalos Y (2001) Adaptation in vertebrate photoreceptors. Physiol Rev 81: 117–151.
[Abstract/Free Full Text] Freedman NJ, Lefkowitz RJ (1996) Desensitization of G-protein-coupled receptors. Recent Prog Horm Res 51: 319–351.
Fukada Y, Kokame K, Okano T, Shichida Y, Yoshizawa T, McDowell JH, Hargrave PA, Palczewski K (1990) Phosphorylation of iodopsin, chicken red-sensitive cone visual pigment. Biochemistry 29: 10102–10106.[Medline]
Hisatomi O, Imanishi Y, Satoh T, Tokunaga F (1997) Arrestins expressed in killifish photoreceptor cells. FEBS Lett 411: 12–18.[Web of Science][Medline]
Hisatomi O, Matsuda S, Satoh T, Kotaka S, Imanishi Y, Tokunaga F (1998) A novel subtype of G-protein-coupled receptor kinase, GRK7, in teleost cone photoreceptors. FEBS Lett 424: 159–164.[Web of Science][Medline]
Jeon CJ, Strettoi E, Masland RH (1998) The major cell populations of the mouse retina. J Neurosci 18: 8936–8946.
[Abstract/Free Full Text] Kennedy MJ, Lee KA, Niemi GA, Craven KB, Garwin GG, Saari JC, Hurley JB (2001) Multiple phosphorylation of rhodopsin and the in vivo chemistry underlying rod photoreceptor dark adaptation. Neuron 31: 87–101.[Web of Science][Medline]
Krupnick JG, Benovic JL (1998) The role of receptor kinases and arrestins in G-protein-coupled receptor regulation. Annu Rev Pharmacol Toxicol 38: 289–319.[Web of Science][Medline]
Krupnick JG, Gurevich VV, Benovic JL (1997) Mechanism of quenching of phototransduction. Binding competition between arrestin and transducin for phosphorhodopsin. J Biol Chem 272: 18125–18131.
[Abstract/Free Full Text] Leskov IB, Klenchin VA, Handy JW, Whitlock GG, Govardovskii VI, Bownds MD, Lamb TD, Pugh Jr EN, Arshavsky VY (2000) The gain of rod phototransduction: reconciliation of biochemical and electrophysiological measurements. Neuron 27: 525–537.[Web of Science][Medline]
Lyubarsky AL, Chen C, Simon MI, Pugh Jr EN (2000) Mice lacking G-protein receptor kinase 1 have profoundly slowed recovery of cone-driven retinal responses. J Neurosci 20: 2209–2217.
[Abstract/Free Full Text] Maeda T, Ohguro H, Sohma H, Kuroki Y, Wada H, Okisaka S, Murakami A (2000) Purification and characterization of bovine cone arrestin (cArr). FEBS Lett 470: 336–340.[Web of Science][Medline]
Mata NL, Radu RA, Clemmons RC, Travis GH (2002) Isomerization and oxidation of vitamin A in cone-dominant retinas: a novel pathway for visual-pigment regeneration in daylight. Neuron 36: 69–80.[Web of Science][Medline]
Mears AJ, Kondo M, Swain PK, Takada Y, Bush RA, Saunders TL, Sieving PA, Swaroop A (2001) Nrl is required for rod photoreceptor development. Nat Genet 29: 447–452.[Web of Science][Medline]
Mendez A, Burns ME, Roca A, Lem J, Wu LW, Simon MI, Baylor DA, Chen J (2000) Rapid and reproducible deactivation of rhodopsin requires multiple phosphorylation sites. Neuron 28: 153–164.[Web of Science][Medline]
Murakami A, Yajima T, Sakuma H, McLaren MJ, Inana G (1993) X-arrestin: a new retinal arrestin mapping to the X chromosome. FEBS Lett 334: 203–209.[Web of Science][Medline]
Perry RJ, McNaughton PA (1991) Response properties of cones from the retina of the tiger salamander. J Physiol (Lond) 433: 561–587.
[Abstract/Free Full Text] Pitcher JA, Freedman NJ, Lefkowitz RJ (1998) G-protein-coupled receptor kinases. Annu Rev Biochem 67: 653–692.[Web of Science][Medline]
Pugh Jr EN, Lamb TD (2000) Phototransduction in vertebrate rods and cones: molecular mechanisms of amplification, recovery and light adaptation. In: Handbook of biological physics, Vol 3 (Stavenga DG, DeGrip WJ, Pugh Jr EN, eds), pp 184–255. Amsterdam: Elsevier.
Rehemtulla A, Warwar R, Kumar R, Ji X, Zack DJ, Swaroop A (1996) The basic motif-leucine zipper transcription factor Nrl can positively regulate rhodopsin gene expression. Proc Natl Acad Sci USA 93: 191–195.
[Abstract/Free Full Text] Sakuma H, Inana G, Murakami A, Higashide T, McLaren MJ (1996) Immunolocalization of X-arrestin in human cone photoreceptors. FEBS Lett 382: 105–110.[Web of Science][Medline]
Schnapf JL, Nunn BJ, Meister M, Baylor DA (1990) Visual transduction in cones of the monkey Macaca fascicularis. J Physiol (Lond) 427: 681–713.
[Abstract/Free Full Text] Smith WC, Gurevich EV, Dugger DR, Vishnivetskiy SA, Shelamer CL, McDowell JH, Gurevich VV (2000) Cloning and functional characterization of salamander rod and cone arrestins. Invest Ophthalmol Vis Sci 41: 2445–2455.
[Abstract/Free Full Text] Swain PK, Hicks D, Mears AJ, Apel IJ, Smith JE, John SK, Hendrickson A, Milam AH, Swaroop A (2001) Multiple phosphorylated isoforms of NRL are expressed in rod photoreceptors. J Biol Chem 276: 36824–36830.
[Abstract/Free Full Text] Swaroop A, Xu JZ, Pawar H, Jackson A, Skolnick C, Agarwal N (1992) A conserved retina-specific gene encodes a basic motif/leucine zipper domain. Proc Natl Acad Sci USA 89: 266–270.
[Abstract/Free Full Text] Tachibanaki S, Tsushima S, Kawamura S (2001) Low amplification and fast visual pigment phosphorylation as mechanisms characterizing cone photoresponses. Proc Natl Acad Sci USA 98: 14044–14049.
[Abstract/Free Full Text] Tornehave D, Hougaard DM, Larsson L (2000) Microwaving for double indirect immunofluorescence with primary antibodies from the same species and for staining of mouse tissues with mouse monoclonal antibodies. Histochem Cell Biol 113: 19–23.[Web of Science][Medline]
Walter AE, Shuster TA, Farber DB (1986) Light-induced phosphorylation of proteins from the all-cone retina of the lizard, Anolis carolinensis. Invest Ophthalmol Vis Sci 27: 1609–1614.
[Abstract/Free Full Text] Weiss ER, Raman D, Shirakawa S, Ducceschi MH, Bertram PT, Wong F, Kraft TW, Osawa S (1998) The cloning of GRK7, a candidate cone opsin kinase, from cone- and rod-dominant mammalian retinas. Mol Vis 4: 27.[Medline]
Weiss ER, Ducceschi MH, Horner TJ, Li A, Craft CM, Osawa S (2001) Species-specific differences in expression of G-protein-coupled receptor kinase (GRK) 7 and GRK1 in mammalian cone photoreceptor cells: implications for cone cell phototransduction. J Neurosci 21: 9175–9184.
[Abstract/Free Full Text] Wilden U (1995) Duration and amplitude of the light-induced cGMP hydrolysis in vertebrate photoreceptors are regulated by multiple phosphorylation of rhodopsin and by arrestin binding. Biochemistry 34: 1446–1454.[Medline]
Wilden U, Kuhn H (1982) Light-dependent phosphorylation of rhodopsin: number of phosphorylation sites. Biochemistry 21: 3014–3022.[Medline]
Wilden U, Hall SW, Kuhn H (1986a) Phosphodiesterase activation by photoexcited rhodopsin is quenched when rhodopsin is phosphorylated and binds the intrinsic 48-kDa protein of rod outer segments. Proc Natl Acad Sci USA 83: 1174–1178.
[Abstract/Free Full Text] Wilden U, Wust E, Weyand I, Kuhn H (1986b) Rapid affinity purification of retinal arrestin (48 kDa protein) via its light-dependent binding to phosphorylated rhodopsin. FEBS Lett 207: 292–295.[Medline]
Xu J, Dodd RL, Makino CL, Simon MI, Baylor DA, Chen J (1997) Prolonged photoresponses in transgenic mouse rods lacking arrestin. Nature 389: 505–509.[Medline]
Zhang Y, Li A, Zhu X, Wong CH, Brown B, Craft CM (2001) Cone arrestin expression and induction in retinoblastoma cells. In: Ninth international symposium on retinal degeneration (Anderson RE, LaVail MM, Hollyfield JG, eds), pp 309–317. Durango, CO: Kluwer Academic.
Zhao X, Huang J, Khani SC, Palczewski K (1998) Molecular forms of human rhodopsin kinase (GRK1). J Biol Chem 273: 5124–5131.
[Abstract/Free Full Text] Zhao X, Yokoyama K, Whitten ME, Huang J, Gelb MH, Palczewski K (1999) A novel form of rhodopsin kinase from chicken retina and pineal gland. FEBS Lett 454: 115–121.[Medline]
Zhu X, Craft CM (2000) Modulation of CRX transactivation activity by phosducin isoforms. Mol Cell Biol 20: 5216–5226.
[Abstract/Free Full Text] Zhu X, Ma B, Babu S, Murage J, Knox BE, Craft CM (2002a) Mouse cone arrestin gene characterization: promoter targets expression to cone photoreceptors. FEBS Lett 524: 116–122.[Web of Science][Medline]
Zhu X, Li A, Brown B, Weiss ER, Osawa S, Craft CM (2002b) Mouse cone arrestin expression pattern: light-induced translocation in cone photoreceptors. Mol Vis 8: 462–471.[Web of Science][Medline]
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