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A Critical Role of CaBP4 in the Cone Synapse

¹From the Departments of Ophthalmology, ³Pharmacology, and ⁴Chemistry, University of Washington, Seattle, Washington; and the ²Departments of Ophthalmology and Molecular Cardiology, Tufts–New England Med Center, Boston, Massachusetts.

	Abstract

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PURPOSE. CaBP4, a photoreceptor-specific protein of the rods and cones, is essential for the development and maintenance of the mouse photoreceptor synapse. In this study, double CaBP4/rod -transducin knockout (Cabp4^–/–Gnat1^–/–) mice lacking the rod-mediated component of electrophysiologic responses were generated and analyzed to investigate the role of CaBP4 in cones.

METHODS. The retinal morphology and physiologic function of 2-month-old Cabp4^–/–Gnat1^–/– mice were analyzed using immunocytochemistry, electron microscopy, and single-flash and flicker electroretinography (ERG).

RESULTS. The thickness of the outer plexiform layer and the number of photoreceptor terminals in Cabp4^–/–Gnat1^–/– mice were reduced to levels similar to those of Cabp4^–/– mice. Single-flash and flicker ERG showed that the amplitude and sensitivity of the b-wave in the Cabp4^–/–Gnat1^–/– mice were severely attenuated compared with those in wild-type and Gnat1^–/– mice.

CONCLUSIONS. Results indicate that the cone synaptic function in Cabp4^–/–Gnat1^–/– mice was severely disrupted, whereas the morphologic defects observed in Cabp4^–/–Gnat1^–/– mice were similar to those of single Cabp4^–/– knockout mice. This and a previous study reveal that CaBP4 is critical for signal transmission from rods and cones to second-order neurons.

In the mouse eye, CaBP4 is localized at the photoreceptor synaptic terminals in rods and cones. CaBP4 is essential for the development and maintenance of the photoreceptor synapse, likely through functional modulation of the photoreceptor Ca²⁺ channels, 1F L-type voltage-dependent calcium channels (Ca_v1.4), and neurotransmitter release.² Photoreceptor synapses in CaBP4-deficient (Cabp4^–/–) mice are severely disrupted anatomically and functionally. ERG measurements and single-cell recordings show a disruption in the transmission from photoreceptors to bipolar cells in Cabp4^–/– mice, whereas rod phototransduction is only modestly affected.

Mutations in the CACNA1F gene (Ca_v1.4 gene) are responsible for incomplete congenital stationary night blindness (CSNB2).⁹ Interestingly, the phenotypes of these patients and of mice deficient for the ß2 subunit of the Ca_v1.4 channel¹⁰ are similar to those of Cabp4^–/– mice. In a previous study, we demonstrated that the signal transfer from rods to rod bipolar cells is altered in Cabp4^–/– mice by measuring light responses of rod bipolar cells.² Ca_v1.4 channel expression has been clearly shown in rods but not yet in cones. Thus cone function response cannot be either clearly inferred from our initial ERG experiments or ascribed to CaBP4–Ca_v1.4 channel interaction. Furthermore, 30-Hz flicker ERG responses of CSNB2 patients carrying CACNA1F gene mutations suggest markedly depressed cone functions,¹¹ though these patients have normal color vision.¹²

It is important to evaluate the function of CaBP4 in cones to understand its role in the development and maintenance of the photoreceptor synapse between cone and bipolar cells and its contribution to the cone phenotype of CSNB2 patients. For this purpose, mice lacking functional rod transducin (Gnat1^–/–) were crossbred with Cabp4^–/– mice to generate Cabp4^–/–Gnat1^–/– mice. The Gnat1^–/– mouse is a useful model to evaluate pure cone function under all light conditions and has been characterized extensively by Calvert et al.¹¹ We have analyzed and compared the retinal morphology and light responses of wild-type, CaBP4, rod -transducin, and CaBP4/rod -transducin knockout mice with single-flash and flicker ERG to evaluate the cone function of each genotype more precisely.

	Materials and Methods

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Generation and Genotyping of Cabp4^–/– Gnat1^–/– Knockout Mice
The mice were housed in the Department of Comparative Medicine at the University of Washington and were treated according to the ARVO Statement for the Use of Animals in Ophthalmic and Vision Research. The double-knockout mice were generated by breeding Cabp4^–/– mice² and Gnat1^–/– mice.¹¹ The genotype of the mutant mice was confirmed by PCR. To identify the wild-type allele, the primer pair FH589 (5'-GTACACATGTAGATGCAGGAG-3', hybridizing in intron 4 of mouse Gnat1) and FH588 (5'-CACCAGCACCATGTCGTAAG-3', located in exon 6 of mouse Gnat1) was used to give a PCR product of 500 bp. The targeted CaBP4 allele was identified with primers K183 (5'-CTTGGCGAATATCATGGTGG-3', located in the neo-cassette) and FH588 and gave a PCR product of approximately 600 bp. The PCRs were cycled at 94°C for 5 minutes, followed by 35 cycles at 94°C for 30 seconds, 60°C for 30 seconds, and 72°C for 1.5 minutes, followed by a final extension at 72°C for 7 minutes. Cabp4^–/–, Gnat1^–/–, and Cabp4^–/–Gnat1^–/– mice were in a mixed C57BL/6, 129SvEv, and BALB/c background. The wild-type mice were C57Bl/6.

Antibodies
Monoclonal mouse anti-PSD95 (clone K28/43) was purchased from Upstate Biotechnology (Lake Placid, NY.). Mouse monoclonal anti-Bassoon was purchased from Stressgen (Victoria, BC, Canada). Rabbit anti–protein kinase C - (sc-208) and anti–rod -transducin (sc-389) were purchased from Santa Cruz Biotechnology, Inc. (Santa Cruz, CA). Labeled peanut agglutinin (PNA) and conjugated goat anti–mouse IgG were purchased from Molecular Probes, Inc. (Alexa 488; Eugene, OR). Cy3-conjugated goat anti–rabbit IgG and anti–mouse IgG were purchased from Jackson ImmunoResearch Laboratories, Inc. (West Grove, PA). The generation of rabbit polyclonal anti-CaBP4 was described previously.²

Immunocytochemistry
Mouse eyecups were fixed in 4% paraformaldehyde in 0.1 M phosphate buffer (PB; 100 mM sodium phosphate, pH 7.4) for 4 hours. After fixation, the tissues were infiltrated with graded sucrose solutions (5%, 10%, 15%, and 20% sucrose in PB), and then embedded in 33% OCT compound (Miles, Elkhart, IN) diluted with 20% sucrose in PB. Eye tissues were cut in 10-µm sections. To block non-specific labeling, retinal sections were incubated with 3% normal goat serum in PBST buffer (136 mM NaCl, 11.4 mM sodium phosphate, 0.1% Triton X-100, pH 7.4) for 20 minutes at room temperature. Sections were incubated overnight at 4°C in diluted primary antibodies. Sections were washed with PBST. For single staining, sections were incubated with Cy3-conjugated goat anti–rabbit IgG. For double staining, a mixture of Cy3-conjugated goat anti–rabbit IgG and conjugated goat anti-mouse IgG (Alexa 488; Molecular Probes) was reacted with sections. For double staining including PNA, sections were incubated with PNA and Cy3-conjugated goat anti-rabbit IgG (Alexa 488; Molecular Probes). Sections were stained with Hoechst 33342 dye (Molecular Probes) to reveal the nuclei. Then, sections were rinsed in PBST and mounted with antifade reagent (Prolong; Molecular Probes) to retard photobleaching. For experiments using retinal whole-mounts, the retinas were dissected as described previously.¹² The retinas were incubated with 5% normal goat serum in PBST buffer (136 mM NaCl, 11.4 mM sodium phosphate, 0.1% Triton X-100, pH 7.4) overnight at 4°C and then again overnight at 4°C with anti-bassoon antibody (1:500). After three washes for 15 minutes in PBST, Cy-3–conjugated goat anti-mouse (1:100) or PNA (1:50; Alexa 488; Molecular Probes) was added to the retina overnight at 4°C. Retinal whole-mounts were mounted with the photoreceptor side up.

Sections were analyzed under a confocal microscope (Zeiss LSM510; Carl Zeiss, New York, NY.). Immunofluorescent images were obtained with a 40x/1.3 NA objective lens (Plan-Neofluar; Carl Zeiss). Projections of confocal images were made using LSM510 software 3.0 (Carl Zeiss).

Transmission Electron Microscopy
Mouse eyecups were primarily fixed by immersion in 2.5% glutaraldehyde, 1.6% paraformaldehyde in pH 7.4, 0.08 M piperazine diethanesulfonic acid (PIPES) buffer containing 2% sucrose, initially at room temperature for approximately 1 hour, then at 4°C for the remainder of a 24-hour period. The eyecups were then washed with pH 7.35, 0.13 M phosphate buffer, and secondarily fixed with 1% OsO₄ in pH 7.4, 0.1 M phosphate buffer for 1 hour at room temperature. After another wash with 0.13 M phosphate buffer, the eyecups were dehydrated through a methanol series and transitioned to epoxy embedding medium with propylene oxide. The eyecups were infiltrated (Eponate 812; Ted Pella, Inc., Redding, CA) and embedded for sectioning in Eponate 812 by hardening at 70°C for 24 hours before ultramicrotomy. Ultrathin sections (60–70 nm) were cut with a diamond knife and mounted on 50-mesh grids coated with a film (Pioloform; Ted Pella). The sections were then stained with aqueous-saturated uranium acetate and Reynold’s formula lead citrate before survey and micrography (CM10 electron microscope; Philips, Eindhoven, The Netherlands). A montage of individual images was created in Adobe Photoshop. Photoreceptor terminals and synaptic ribbons were counted from working prints of sections obtained from 3 eyes. Sections were analyzed from end to end.

Electroretinograms
Before recording, mice were dark adapted overnight. Under safety light, mice were anesthetized by intraperitoneal injection using 20 µL/g body weight of 6 mg/mL ketamine and 0.44 mg/mL xylazine diluted in 10 mM sodium phosphate (pH 7.2) containing 100 mM NaCl. Pupils were dilated with 1% tropicamide. A contact lens electrode was placed on the eye, and a reference electrode and a ground electrode were placed in the ear and on the tail. Electroretinograms were recorded with the universal testing and electrophysiologic system (UTAS E-3000; LKC Technologies, Inc., Gaithersburg, MD). Light intensity was calibrated by the manufacturer and was computer controlled. Mice were placed in a Ganzfeld chamber, and scotopic and photopic responses to flash stimuli were obtained from both eyes simultaneously.

Single-Flash Recording.
Flash stimuli had a range of intensities (–3.7 to 2.8 log cd · s · m^–2), and white light flash duration was adjusted according to intensity (20 µs-1 ms). Three to five recordings were made at >10-second intervals, and for higher intensity, intervals were 10 minutes long or as indicated. There were no significant differences between the first and the fifth flashes. Photopic responses were examined after bleaching at 1.4 log cd · m^–2 for 15 minutes. Four to eight 2-month-old animals were typically used for the recording of each point in all conditions.

Flicker-Flash Recording.
The recordings were performed following the same procedure as for single-flash recording. Flicker stimuli had a range of intensities (–3.7 to 1.4 log cd · s · m^–2) with various frequencies (5–30 Hz). Statistical analysis was carried out using one-way ANOVA.

	Results

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Morphologic Changes of the Retina
The morphology and the expression of relevant proteins were first analyzed in 2-month-old mice with antibodies directed against CaBP4 and rod -transducin proteins. As expected, no CaBP4 proteins were detected in the Cabp4^–/– and Cabp4^–/– Gnat1^–/– retinas, and no -transducin proteins were observed in the Gnat1^–/– and Cabp4^–/– Gnat1^–/– mice (Fig. 1) . The localization of CaBP4 in Gnat1^–/– and transducin in Cabp4^–/– was similar to that in the wild-type mice. The thickness of all nuclear layers except the outer plexiform layer was unaltered in all knockout mice compared with the wild-type mice. To determine whether the cones were preserved in all knockout mice, we labeled the cones with fluorescein-labeled PNA. There was no difference in either the pattern of PNA staining or the number of cone photoreceptors in wild-type and all knockout mice (Figs. 2A 2B 2C 2D) . The inset points out the localization of CaBP4 in cones also labeled with PNA (Fig. 2A) . CaBP4 staining was observed at the cone synaptic pedicles alongside the PNA-labeled synaptic membranes. CaBP4 staining was also observed in the rod spherules not labeled with PNA. To analyze the morphology of the synapse, an antibody against the presynaptic protein PSD95 was used to label the photoreceptor presynapse. The anti–protein kinase C alpha (PKC) antibody was used to visualize the neuronal processes of rod bipolar cells. Gnat1^–/– and wild-type mice showed comparable pericellular staining with anti-PKC and developed dendrites (Figs. 2E 2G) . Inflated photoreceptor synaptic terminals were observed with anti-PSD95 in Gnat1^–/– and wild-type mice. Photoreceptor terminals were condensed in Cabp4^–/– and Cabp4^–/– Gnat1^–/– mice, and the dendrites of their rod bipolar cells were short and underdeveloped (Figs. 2F 2H) compared with those of Gnat1^–/– and wild-type mice.

View larger version (75K): [in this window] [in a new window]   FIGURE 1. Immunofluorescence staining of 2-month-old wild-type and knockout mice retina with antibodies recognizing CaBP4 and rod -transducin. (A–D) Immunolocalization of CaBP4 (red). Labeling is observed in the outer plexiform layer. Some labeling is also observed in the inner segment. As expected, no CaBP4 immunoreactivity is detected in the retinas of Cabp4–/– and Cabp4–/– Gnat1–/– mice. (E–H) Immunolocalization of rod -transducin (red). Immunofluorescence is observed in the outer segment. No immunoreactivity is detected in the retina of Gnat–1– and Cabp4–/– Gnat1–/– mice. (A–H) Nuclei are visualized by staining with Hoechst 33,342 dye. Scale bars, 20 µm.

View larger version (98K): [in this window] [in a new window]   FIGURE 2. Morphologic changes in the retinas of 2-month-old mice. (A–D) Immunolocalization of PKC (red) and staining of cone photoreceptor with PNA (green). No difference was observed in the PNA staining pattern of cone photoreceptors between wild-type and single- and double-knockout mice. In wild-type mice, CaBP4 (red) is expressed in cones also labeled with PNA (green) (A, inset). CaBP4 staining is observed at the cone synaptic pedicles alongside the PNA-labeled synaptic membranes. CaBP4 staining is also observed in the rod spherules not labeled with PNA. (E–H) Synaptic changes in the OPL visualized by immunolocalization of PKC (red) and PSD95 (green). Visualization of photoreceptor presynapses using anti-PSD95 antibody and of neuronal processes of rod bipolar cells using anti-PKC. In wild-type and Gnat1–/– mice, the photoreceptor terminals are inflated, whereas those in Cabp4–/– and Cabp4–/– Gnat1–/– mice are disorganized and condensed. (A–H) Nuclei are visualized by staining with Hoechst 33,342 dye. Scale bars, (A–D) 20 µm; (A, inset) 2 µm; (E–H) 5 µm.

View larger version (85K): [in this window] [in a new window]   FIGURE 3. PNA labeling of cones in retinal whole-mounts of 2-month-old mice. (A) Staining of cone outer segments in the four quadrants of flat-mounted retina labeled with PNA from wild-type and all knockout mice. D, dorsal; V, ventral; N, nasal, T, temporal. Scale bars, 20 µm. (B) Double labeling with anti-bassoon (red) and PNA (green) across the outer plexiform layer in the temporal quadrant of the flat-mounted retina. Horseshoe-shaped structures are observed in wild-type and Gnat1–/– mice, but mostly punctate staining is observed in Cabp4–/– and Cabp4–/– Gnat1–/– mice. In wild-type and Gnat1–/– mice, the PNA-labeled cone pedicles are round, but the cone pedicles of Cabp4–/– and Cabp4–/– Gnat1–/– mice are more disorganized and appear spread out in a diamond-shaped structure. Scale bar, 5 µm.

View larger version (196K): [in this window] [in a new window]   FIGURE 4. Ultrastructure of photoreceptors of 2-month-old mice analyzed by transmission electron microscopy. (A–D) Cross-sections through the photoreceptors. The outer plexiform layer is thinner in Cabp4–/– and Cabp4–/– Gnat1–/– mice than in wild-type mice. OS, outer segment; IS, inner segment; ONL, outer nuclear layer; OPL, outer plexiform layer. (E–H) Cross-sections through the OS. OS ultrastructure was comparable in retinas of knockout and wild-type mice (i.e., they were straight, parallel cylinders). (I–L) Cross-sections through the OPL. The OPL is delineated by black lines. Photoreceptor terminals that constitute the OPL in the wild-type and Gnat1–/– mice were thinned in Cabp4–/– and Cabp4–/– Gnat1–/– mice. Scale bars, (A--D) 10 µm; (E--L) 2.5 µm.

Analysis of Cone Function Using Electroretinogram Recordings
Electroretinograms of wild-type, Cabp4^–/–, Gnat1^–/–, and Cabp4^–/– Gnat1^–/– mice were recorded under scotopic and photopic conditions.

Scotopic Conditions.
As expected from previous studies, no a-wave originating from rods was detected in 2-month-old Gnat1^–/– mice.¹⁴ Their b-wave resulting from cone-mediated responses showed reduced amplitude and was only detectable from –1.0 log cd · s · m^–2 (Figs. 5A 5B) . In Cabp4^–/– mice, the amplitude of the a-wave was half the amplitude of that of wild-type mice, and the b-wave was even more severely affected (Figs. 5A 5B) . Both waves became detectable at intensities higher than –2.0 log cd · s · m^–2. In the Cabp4^–/– Gnat1^–/– double-knockout mice, the a-wave and b-wave were almost absent, suggesting that there were no rod- and almost no cone-driven responses in scotopic conditions. These data also suggested that the b-wave observed in Cabp4^–/– mice under these conditions originated mostly from rod responses.

View larger version (18K): [in this window] [in a new window]   FIGURE 5. Single-flash ERG responses of increasing intensity for 2-month-old wild-type, Gnat1–/–, Cabp4–/–, and Gnat1–/–Cabp4–/– mice. Serial responses to increasing flash stimuli were obtained for wild-type, Gnat1–/–, Cabp4–/–, and Gnat1–/– Cabp4–/– mice for selected intensities under scotopic conditions (A) and photopic conditions (C) and were plotted as a function of a-wave and b-wave versus light intensity under scotopic conditions (B) and photopic conditions (D). In scotopic conditions, the a-wave amplitudes of Gnat1–/– Cabp4–/– mice were significantly reduced compared with those of wild-type and Cabp4–/– mice (P < 0.0001), but they were not significantly reduced compared with those of Gnat1–/– (P > 0.1). The b-wave amplitudes of Gnat1–/– Cabp4–/– mice in scotopic conditions were attenuated significantly compared with those of mice of all other genetic backgrounds (P < 0.001). In photopic conditions, the a-wave amplitudes of Gnat1–/–, Cabp4–/–, and Gnat1–/– Cabp4–/– mice were moderately reduced compared with those of wild-type mice (P < 0.1), whereas no significant differences were observed among those of Gnat1–/–, Cabp4–/–, and Gnat1–/– Cabp4–/– mice (P > 0.1). The b-wave amplitudes of Cabp4–/– and Cabp4–/– Gnat1–/– mice were significantly attenuated (P < 0.001) compared with those of wild-type and Gnat1–/– mice, whereas no significant difference was observed between those of Cabp4–/– and Gnat1–/– Cabp4–/– mice. (B, D) SE bars are shown.

Flicker ERG.
Flicker ERG to stimuli varying in temporal frequency and intensity was recorded to investigate cone responses. Pure cone responses are best characterized at 20 Hz¹⁵ or are dominantly observed at high-intensity 10-Hz stimulation in scotopic conditions.¹⁶ In scotopic conditions at 10 Hz, the sensitivity and amplitude of the flicker ERG were reduced significantly for all knockout mice compared with wild-type mice. Flicker ERG amplitudes of Cabp4^–/– and Cabp4^–/– Gnat1^–/– mice were significantly less than those of Gnat1^–/– mice. At a frequency of 20 Hz, a severe reduction in the amplitude of flicker ERG was observed for Cabp4^–/– and Cabp4^–/– Gnat1^–/– mice (Fig. 6) . Surprisingly, the amplitude of Gnat1^–/– was also affected, though less than in the other knockout mice. Under photopic conditions, the sensitivity of the flicker ERG was similar for all mice. However, the amplitude of the flicker ERG was severely reduced at higher intensities (at >0.6 log cd · s · m^–2) for all knockout mice, though the reduction in Gnat1^–/– was again less severe. Together, these data demonstrate that the responses of cones and rods in CaBP4-deficient mice are significantly affected or absent in comparison with wild-type mice.

View larger version (26K): [in this window] [in a new window]   FIGURE 6. Flicker-flash ERG responses of increasing intensity with various frequencies for wild-type, Gnat1–/–, Cabp4–/–, and Gnat1–/–Cabp4–/– mice. Flicker responses to increasing flash stimuli at varying frequency were obtained for wild-type, Gnat1–/–, Cabp4–/–, and Gnat1–/– Cabp4–/– mice and plotted as flicker wave amplitude versus light intensity under scotopic conditions (left) and photopic conditions (right). In scotopic conditions with 10- and 20-Hz stimulations, amplitudes and sensitivities of responses of Gnat1–/–Cabp4–/– mice and Cabp4–/– mice were significantly attenuated compared with those of Gnat1–/– and wild-type mice (P < 0.001), whereas no significant changes were observed between Gnat1–/– Cabp4–/– mice and Cabp4–/– mice (P > 0.1). In photopic conditions with 10-Hz stimulation, Gnat1–/– Cabp4–/– mice showed significantly lower amplitudes and sensitivities than did other mice (P < 0.01). Cabp4–/– mice revealed significantly reduced amplitudes compared with wild-type mice (P < 0.0001). Small changes, and these only at higher intensities (P < 0.05 at >0.6 log cd · s · m–2), were observed in Cabp4–/– mice compared with Gnat1–/– mice. With 20-Hz stimulation, Gnat1–/– Cabp4–/– mice and Cabp4–/– mice showed significantly attenuated responses compared with Gnat1–/– and wild-type mice (P < 0.001), whereas no significant difference was observed between the attenuated responses of Gnat1–/– Cabp4–/– mice and Cabp4–/– mice (P > 0.1). SE bars are shown.

	Discussion

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In this study, to investigate the role of CaBP4 for cone vision, we crossbred Cabp4^–/– with Gnat1^–/– mice. These Cabp4^–/– Gnat1^–/– double-knockout mice allowed us to study the effect of CaBP4-deficiency without interference from rod-mediated responses. No detectable changes in retinal morphology between double-knockout mice and single-knockout mice were observed, and the cones were as well preserved in double-knockout mice as in single-knockout mice. These results indicate that the absence of photoexcitation in rods does not affect the CaBP4-deficient phenotype morphologically, confirming the suitability of this model to study the effect of CaBP4 deficiency on cone signaling function. These observations are in accordance with other findings that demonstrate that the absence of functional cones and rods does not affect the structural development of the photoreceptor synapses after eye opening.²⁰ Synaptic contacts between photoreceptor terminals, horizontal cell processes, and bipolar cell dendrites were also reported to be relatively normal in double cone cyclic nucleotide-gated cation channel /rhodopsin knockout mice up to postnatal week 4.²⁰

The absence of morphologic changes between these Cabp4^–/– and Cabp4^–/– Gnat1^–/– mice also suggests that changes in the photoreceptor terminals associated with rod-mediated light responses, including light-dependent changes of the calcium concentration at the synapse, do not contribute to the mechanisms underlying the phenotype of Cabp4^–/– mice. The light-independent phenotype corroborates the putative role of CaBP4 in photoreceptor synaptogenesis.

Electroretinograms were recorded to investigate the effect of CaBP4 deficiency on cone function. Single-flash ERG responses of the Cabp4^–/– Gnat1^–/– mice were severely reduced in scotopic conditions, whereas there was no significant difference in photopic conditions compared with Cabp4^–/– mice. Reduced-flicker ERG demonstrates that amplitudes and sensitivities of Cabp4^–/– Gnat1^–/– mice and Cabp4^–/– mice were significantly attenuated compared with those of Gnat1^–/– mice and wild-type mice, suggesting that few neural connections between cone cells and bipolar cells are functional in Cabp4^–/– and Cabp4^–/– Gnat1^–/– mice, in agreement with the results obtained using single-flash ERG recordings. These data demonstrate that in the absence of CaBP4, the synaptic transmission of the light response from cones to second-order neurons is severely affected. Unexpectedly, flicker ERG of Gnat1^–/– mice under scotopic and photopic conditions was attenuated compared with that of wild-type mice. This difference might be attributed to the different genetic backgrounds of wild-type mice and knockout mice.

Gresh et al. ²¹ reported that a reduced amplitude of flicker ERG correlates with increasing flicker frequency more noticeably in Balb/c mice than in C57Bl/6 mice. To confirm the genetic background effects of mice for flicker ERG, double-heterozygous mice that comprise mixed C57BL/6, 129SvEv, and BALB/c backgrounds were prepared and analyzed with flicker ERG under the same conditions used in this study. However, no significant differences were observed between C57BL/6 wild-type mice and double-heterozygous mice (data not shown).

We have previously shown that CaBP4 interacts with expressed 1F (Ca_v1.4) L-type, voltage-dependent calcium channels and modulates their functional properties.² Although the molecular identity of the cone Ca²⁺ channels is not fully elucidated, some cone channels contain the Ca_v1.3 subunit.^{22 23 24} Moreover, immunostaining of additional aggregates to typical horseshoe-shaped structures with an anti-Ca_v1.4 1F antibody suggests that Ca_v1.4 1F is also present in cone terminals.²⁵ The severely reduced cone signaling in CaBP4-deficient mice indicates that CaBP4 is also critical for the release of neurotransmitter from cone synaptic terminals. These results suggest that cones express the Ca_v1.4 subunit or a subunit highly homologous to it. The gene encoding the -subunit of Ca_v1.4 appears to have diverged more recently from that of the human Ca_v1.3.²⁶ Their amino acid sequences share 70% overall similarity and 84% similarity between transmembrane segments. Furthermore, in humans, mutations in the gene encoding the Ca_v1.4 -subunit cause CSNB2. ERG responses of CSNB2 patients show reduced b-wave amplitude, but their color vision is almost, if not completely, normal, suggesting that cones express a calcium channel other than Ca_v1.4.

Ca_v1.4-deficient mice also show ERG responses with an electronegative configuration and ectopic photoreceptor synapses (Orton NC, et al. IOVS 2004;45:ARVO Abstract 2507). Cav1.4 and Cav1.3 share biophysical properties; both activate at more negative voltages and more rapidly than Cav1.2, and both inactivate more slowly than Cav1.2. However, Ca_v1.3 -deficient mice do not exhibit electroretinogram changes.²⁷ The phenotypes of CSNB2 patients and Ca_v1.4-deficient and Ca_v1.3-deficient mice can be reconciled if cones can be shown to coexpress two types of L-type voltage-dependent calcium channels. This would also be consistent with the critical role of CaBP4 in modulating rod and cone neurotransmitter release.

	Acknowledgements

 
The authors thank Daniel Possin, supported by Vision Core Grant EY01730, for his great expertise with the EM experiments and Rebecca Birdsong for her help during manuscript preparation.

	Footnotes

 
Supported by National Institutes of Health Grants EY014561 (FH), EY12008 (JL), and EY09339 (KP); a grant from the E.K. Bishop Foundation; and Vision Core Grant EY01730.

Submitted for publication April 18, 2005; revised July 1, 2005; accepted September 23, 2005.

Disclosure: T. Maeda, None; J. Lem, None; K. Palczewski, None; F. Haeseleer, None

The publication costs of this article were defrayed in part by page charge payment. This article must therefore be marked "advertisement " in accordance with 18 U.S.C. 1734 solely to indicate this fact.

Corresponding author: Françoise Haeseleer, Department of Ophthalmology, University of Washington, Box 356485, Seattle, WA 98195; fanfan{at}u.washington.edu.

	References

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