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The retina visual cycle is driven by cis retinol oxidation in the outer segments of cones

Published online by Cambridge University Press:  09 February 2017

SHINYA SATO
Affiliation:
Department of Ophthalmology and Visual Sciences, Washington University School of Medicine, Saint Louis, Missouri 63110
RIKARD FREDERIKSEN
Affiliation:
Department of Physiology and Biophysics, Boston University School of Medicine, Boston, MA 02118
M. CARTER CORNWALL
Affiliation:
Department of Physiology and Biophysics, Boston University School of Medicine, Boston, MA 02118
VLADIMIR J. KEFALOV*
Affiliation:
Department of Ophthalmology and Visual Sciences, Washington University School of Medicine, Saint Louis, Missouri 63110
*
*Address correspondence to: Vladimir J. Kefalov, Ph.D, Department of Ophthalmology and Visual Sciences, Washington University in Saint Louis, 660 S. Euclid Avenue, Saint Louis, MO 63110. E-mail: kefalov@wustl.edu
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Abstract

Vertebrate rod and cone photoreceptors require continuous supply of chromophore for regenerating their visual pigments after photoactivation. Cones, which mediate our daytime vision, demand a particularly rapid supply of 11-cis retinal chromophore in order to maintain their function in bright light. An important contribution to this process is thought to be the chromophore precursor 11-cis retinol, which is supplied to cones from Müller cells in the retina and subsequently oxidized to 11-cis retinal as part of the retina visual cycle. However, the molecular identity of the cis retinol oxidase in cones remains unclear. Here, as a first step in characterizing this enzymatic reaction, we sought to determine the subcellular localization of this activity in salamander red cones. We found that the onset of dark adaptation of isolated salamander red cones was substantially faster when exposing directly their outer vs. their inner segment to 9-cis retinol, an analogue of 11-cis retinol. In contrast, this difference was not observed when treating the outer vs. inner segment with 9-cis retinal, a chromophore analogue which can directly support pigment regeneration. These results suggest, surprisingly, that the cis-retinol oxidation occurs in the outer segments of cone photoreceptors. Confirming this notion, pigment regeneration with exogenously added 9-cis retinol was directly observed in the truncated outer segments of cones, but not in rods. We conclude that the enzymatic machinery required for the oxidation of recycled cis retinol as part of the retina visual cycle is present in the outer segments of cones.

Type
Brief Communication
Copyright
Copyright © Cambridge University Press 2017 

Introduction

The vertebrate visual pigment, the light receptor molecule of rod and cone photoreceptor cells, is composed of a protein moiety, opsin, and chromophore, typically 11-cis retinal. Upon absorbing light, 11-cis retinal is photoisomerized to its all-trans form to activate the pigment before eventually dissociating from opsin [reviewed in (Ebrey & Koutalos, Reference Ebrey and Koutalos2001; Imamoto & Shichida, Reference Imamoto and Shichida2014)]. The continuous function of photoreceptor cells requires regeneration of their visual pigments with newly synthesized 11-cis retinal. In vertebrate eyes, there are two metabolic pathways for 11-cis retinal synthesis: the retinal pigment epithelium (RPE) visual cycle and the retina visual cycle (Wang & Kefalov, Reference Wang and Kefalov2011; Saari, Reference Saari2012; Tang et al., Reference Tang, Kono, Koutalos, Ablonczy and Crouch2013; Wright et al., Reference Wright, Redmond and Nickerson2015). The RPE visual cycle is the canonical pathway in which 11-cis retinal is synthesized in the RPE cells and supplied to both rods and cones. The retina visual cycle, on the other hand, is a recently discovered pathway in which 11-cis retinol is synthesized in Müller cells, supplied to cones, and then oxidized there to 11-cis retinal. This cis retinol oxidation activity is cone-specific (Jones et al., Reference Jones, Crouch, Wiggert, Cornwall and Chader1989; Miyazono et al., Reference Miyazono, Shimauchi-Matsukawa, Tachibanaki and Kawamura2008; Ala-Laurila et al., Reference Ala-Laurila, Cornwall, Crouch and Kono2009; Sato & Kefalov, Reference Sato and Kefalov2016). As a result, the retina visual cycle can supply chromophore exclusively to cones, enhancing in that way their fast dark adaptation and their function in bright light (Mata et al., Reference Mata, Radu, Clemmons and Travis2002; Kolesnikov et al., Reference Kolesnikov, Tang, Parker, Crouch and Kefalov2011; Wang et al., Reference Wang, Nymark, Frederiksen, Estevez, Shen, Corbo, Cornwall and Kefalov2014). However, little is known about the molecular mechanisms of the retina visual cycle. Although recent studies have identified several putative components of the pathway for 11-cis retinoid synthesis in Müller cells (Kaylor et al., Reference Kaylor, Yuan, Cook, Sarfare, Makshanoff, Miu, Kim, Kim, Habib, Roybal, Xu, Nusinowitz and Travis2013; Kaylor et al., Reference Kaylor, Cook, Makshanoff, Bischoff, Yong and Travis2014; Xue et al., Reference Xue, Shen, Jui, Rupp, Byrne, Hattar, Flannery, Corbo and Kefalov2015), the enzyme(s) responsible for the cis retinol oxidation in cones is still unknown.

Two hypotheses about this cone-specific reaction have been recently proposed. One suggestion is that the oxidation of cis retinol is carried out in the outer segments of cones by retinol dehydrogenase 8 (RDH8). This idea is based on the observation that deletion of RDH8 blocks the cis retinol-dependent sensitivity recovery in mouse M-cones (Kolesnikov et al., Reference Kolesnikov, Maeda, Tang, Imanishi, Palczewski and Kefalov2015). However, RDH8 is expressed in the outer segments of both rods and cones (Maeda et al., Reference Maeda, Maeda, Imanishi, Kuksa, Alekseev, Bronson, Zhang, Zhu, Sun, Saperstein, Rieke, Baehr and Palczewski2005; Miyazono et al., Reference Miyazono, Shimauchi-Matsukawa, Tachibanaki and Kawamura2008) and is thought to be primarily a reductase of all-trans retinal rather than an oxidase of cis retinol (Rattner et al., Reference Rattner, Smallwood and Nathans2000). The alternative hypothesis is that the oxidation of cis retinol takes place in cone inner segments and is carried out by RDH13-like (RDH13L) and its homologs (Sato et al., Reference Sato, Miyazono, Tachibanaki and Kawamura2015). RDH13L is a cone-specific enzyme identified from purified carp cone inner segment membranes. It oxidizes cis retinol with concomitant reduction of NADP+ or hydrophobic aldehydes. However, RDH13L is found only in fish and is, therefore, not a component of the mammalian retina visual cycle. Although it’s functional homolog, RDH14 (Sato et al., Reference Sato, Miyazono, Tachibanaki and Kawamura2015), is suggested to be expressed in mouse cones (Kanan et al., Reference Kanan, Kasus-Jacobi, Moiseyev, Sawyer, Ma and Al-Ubaidi2008), its role in the cone-specific oxidation of cis retinol has not been examined.

Here, as a way of addressing this issue, we sought to identify the cellular compartment of salamander red cones where cis retinol oxidation takes place. The salamander retina has a high percentage of cones (∼40%) (Sherry et al., Reference Sherry, Bui and Degrip1998) and its photoreceptors are >5 times larger in width than those of the mouse retina [see for instance (Koutalos & Cornwall, Reference Koutalos and Cornwall2010)]. These features allowed us targeted application of cis retinal or cis retinol selectively to the inner or outer segment of individual cones in an effort to determine the subcellular localization of the cis retinol oxidation activity in cones.

Materials and methods

Single-cell suction recordings

All experiments were performed in accordance with protocols approved by the Washington University Animal Studies Committee and the Institutional Animal Care and Use Committee of Boston University School of Medicine, following the Guide for the Care and Use of Laboratory Animals and the Animal Welfare Act. Larval tiger salamanders (Ambystoma tigrinum, Charles D. Sullivan Co. Inc., Nashville, TN) were maintained on a 12-h day–night cycle and were dark-adapted overnight before use. Single-cell recordings from salamander cones were carried out as previously described (Kefalov et al., Reference Kefalov, Crouch and Cornwall2001). For the cone dark-adaptation experiments, the inner or outer segment of a red cone was first drawn in the suction pipette and after measuring its dark current and sensitivity, the cell was exposed to brief bright 505 nm light estimated to bleach >99% of its visual pigment. Bleaching light duration was determined from the relation F = 1 − exp(−IPt), where F is the fraction of pigment to be bleached (>0.99), t is the duration of light exposure (>18 s), I is the light intensity (1.2 × 108 photons·μm-2·sec-1), and P is the photosensitivity of salamander red cones at 505 nm (2.3 × 10−9 µm2), estimated from the action spectrum of salamander red cones (Makino & Dodd, Reference Makino and Dodd1996; Sato & Kefalov, Reference Sato and Kefalov2016) and the reported photosensitivity value at the wavelength of peak absorbance (6.0 × 10−9 µm2) (Jones et al., Reference Jones, Fein, MacNichol and Cornwall1993). Following the bleach, the cell was incubated in darkness for 20 min to allow the photoactivated visual pigments to decay to free opsin. The bleach-adapted cell was then treated with 800 µl of 125 µM retinoid solution which was added to the recording chamber. The retinoid solution was prepared as follows: 300 µg of dry retinoid (9-cis retinol: Santa Cruz Biotechnology, Inc., Santa Cruz, CA; 9-cis retinal: Sigma-Aldrich, Inc., Saint Louis, MO) was dissolved into 11 µl ethanol and kept on ice until used. Just before adding to the recording chamber, 1 µl of the ethanolic retinoid solution was mixed with 100 µl of Ringer’s solution first and then additional 700 µl of Ringer’s solution was added gradually to obtain 125 µM retinoid solution. The retinoid solution thus prepared was added into the recording chamber containing ∼2 ml of perfusion solution (i.e., final concentration: ∼40 µM) using a pipette with a wide-bore tip. To optimize the delivery of retinoids to the cone held in the suction electrode, the solution in the chamber was stirred by flushing some of it in and out of the pipette 3 times. As the solution was applied to the bath, only the segment of the cell exposed to it and not drawn in the suction electrode was treated with the retinoid (Jin et al., Reference Jin, Jones and Cornwall1994). To monitor the recovery of cone sensitivity following the application of the retinoid, dim flash responses (with amplitudes below 30% of the maximum recorded from each cone) were recorded every 1 min for 9-cis retinal-treated cones or every 2 min for 9-cis retinol-treated cones, up to 20 min after the addition of retinoid solution. Flash sensitivities were determined as the ratio of dim flash response amplitude and flash intensity. Electrophysiology data were analyzed using pClamp 9 (Molecular Devices, LLC, Sunnyvale, CA) and Origin 7.5 (OriginLab, Northampton, MA).

Microspectrophotometry measurements

The microspectrophotometry measurements were performed on a previously described instrument (Frederiksen et al., Reference Frederiksen, Boyer, Nickle, Chakrabarti, Koutalos, Crouch, Oprian and Cornwall2012). At the beginning of an MSP experiment, a dark-adapted retina was chopped and triturated. Solution containing isolated intact cells and outer segments was placed on a quartz cover-slip window located in the bottom of a 2 mm-deep Plexiglass recording chamber. The tissue was allowed to settle and adhere to the quartz window for up to 10 min to minimize movement of the cells, after which the tissue in the chamber was superfused at a rate of 4 ml/min with Ringer’s solution identical to that used in the electrophysiological experiments. At this time, an isolated intact photoreceptor cell or outer segments were identified from their projected image on the screen of the infrared video system. A baseline absorbance spectrum was measured in an area adjacent to the selected outer segment. Following this measurement, the outer segment was oriented in the beam path with the polarization of the incident measuring beam parallel to the plane of the disks (rods) or invaginations (cones), and absorbance spectra in this area were measured in steps of 2 nm step width. Generally, ten complete sample scans and ten baseline scans were averaged to increase the signal-to-noise ratio of a measured spectrum. The absorbance spectrum was calculated using Beers’ Law according to the relation; OD = log10(I o/I t), where OD is optical density or absorbance, I o is the light transmitted through a cell-free space adjacent to the outer segment, and I t is the light transmitted through the outer segment.

Dark-adapted spectra of the visual pigment were measured in this way from rod and cone outer segments. Once the dark-adapted spectral absorbance was established, the pigment was bleached (>99%) using a calibrated (505 nm; 1.3 × 107 photons·μm-2·sec-1) LED light source. Bleaching photoproducts were monitored periodically and were allowed to decay to undetectable levels. This period was 10 min for cone outer segments, and about 60 min for rods. Following this, we measured the bleached absorbance spectrum. Next, we treated the preparation with 1 ml of 40 µM 9-cis retinol for 10 min. Spectral absorbance was measured and the pigment regeneration was monitored until no further change in spectral absorbance could be detected. Then the regenerated pigment (cones) was bleached once more to confirm that it was photosensitive. If no pigment was regenerated (rods) the preparation was treated with 1 ml of 40 µM 11-cis retinal for 10 min and allowed to regenerate visual pigment.

Statistics

A two-tailed unpaired Student’s t-test was used to test for the significance of difference in the mean values of two sample groups. P-values of <0.05 were considered to be statistically significant.

Results

Location of the cis retinol oxidation reaction in salamander red cones

In the living retina, fresh 11-cis retinol is provided by the Müller cells to cones, and ultimately used for pigment regeneration in the cone outer segments. However, as Müller cell processes do not make direct contact with the cone outer segments (Sarantis & Mobbs, Reference Sarantis and Mobbs1992; Garlipp & Gonzalez-Fernandez, Reference Garlipp and Gonzalez-Fernandez2013), their 11-cis retinol is most likely delivered to the cone inner segments (Insinna et al., Reference Insinna, Daniele, Davis, Larsen, Kuemmel, Wang, Nikonov, Knox and Pugh2012). It is currently unclear whether the subsequent oxidation of 11-cis retinol to 11-cis retinal takes place in the inner or outer segments of cones. To determine the location of cis retinol oxidation in cones, we compared the time course of sensitivity recovery of fully bleached (>99% of visual pigment) isolated salamander red cones in a suction electrode when their outer vs. inner segment was exposed to 9-cis retinol, a commercially available more stable analogue of 11-cis retinol. As the suction electrode fits tightly around the photoreceptor cell, chromophore movement from the bath into the electrode was restricted so that only the part of the cell outside the electrode was exposed to it (Jin et al., Reference Jin, Jones and Cornwall1994). Thus, we reasoned that exposing directly the part of the cell where oxidation takes place to 9-cis retinol would result in faster pigment regeneration compared to the reverse cell configuration. Isolated salamander red cones were drawn into the suction pipette from the outer segment to the mid-point of the inner segment (outer segment-in configuration; Fig. 1A) or from the cell body to the base of the outer segment (outer segment-out configuration; Fig. 2A). Cone pigments were fully bleached (>99%) by 505 nm light and then the cells were kept in darkness for 20 min until their sensitivity reached a steady state. At this point, 9-cis retinal or 9-cis retinol was added to the bath of the recording chamber and the change in cone sensitivity was monitored for the next 10 min for 9-cis retinal or 20 min for 9-cis retinol. Although the relation between the fraction of bleached pigment and sensitivity is nonlinear (Jones et al., Reference Jones, Fein, MacNichol and Cornwall1993; Kefalov et al., Reference Kefalov, Estevez, Kono, Goletz, Crouch, Cornwall and Yau2005), physiological measurements of cone sensitivity provide a reliable method for monitoring the onset and kinetics of cone pigment regeneration. Thus, we used the kinetics of cone dark adaptation to estimate the rate of pigment regeneration in the outer segment, and the initial delay in this process to estimate the time required for the production/delivery of 9-cis retinal to the outer segment.

Fig. 1. Kinetics of red cone sensitivity recovery when exposing the inner segment to exogenous 9-cis chromophore. (A) Image of a red cone in the outer segment-in configuration under microscope with infrared illumination. (B) Dim flash responses from bleached red cones at indicated times after treatment with 9-cis retinal (black traces) and 9-cis retinol (red traces). Response amplitudes are normalized to the flash intensity (i.e. response per photon) to allow direct comparison of sensitivity. (C) Sensitivity recovery time course of bleached red cones in the outer segment-in (OS-in) configuration incubated with 9-cis retinal (filled black squares; n = 10) or 9-cis retinol (filled red circles; n = 8). Data are shown as mean ± SEM.

Fig. 2. Kinetics of red cone sensitivity recovery when exposing the outer segment to exogenous 9-cis chromophore. (A) Image of a red cone in the outer segment-out configuration under microscope with infrared illumination. (B) Sensitivity recovery time course of bleached red cones in the outer segment-out (OS-out) configuration incubated with 9-cis retinal (open black squares; n = 7) or 9-cis retinol (open red circles; n = 8). Data are shown as mean ± SEM.

We began by treating the inner segments of bleached red cones with 9-cis retinal in order to determine the kinetics of delivery of this retinoid to the outer segment and the subsequent rate of cone pigment regeneration in a configuration similar to that in vivo, with the retinoid delivered from the Müller cells. As 9-cis retinal can be used directly for pigment regeneration, the dark adaptation of cones in this case was rate-limited by its delivery to the outer segment. For outer segment-in cones (Fig. 1A), sensitivity recovery began shortly upon exposure to 9-cis retinal (Fig. 1B, black traces). The recovery onset was delayed by ∼1 min (Fig. 1C, black filled squares), possibly reflecting the time required for 9-cis retinal taken up by the inner segment from the bath to reach the outer segment of the cell, sheltered inside the suction electrode. The subsequent dark adaptation of the cones proceeded rapidly and was largely completed within 5–6 min.

We next treat the inner segments of bleached cones with 9-cis retinol, a functional analogue to the 11-cis retinol produced by Müller cells in the retina (Sato & Kefalov, Reference Sato and Kefalov2016). In comparison with 9-cis retinal, use of 9-cis retinol requires the additional step of oxidation before it could be used for pigment regeneration. Thus, the overall time course of cone dark adaptation in this case was determined by two processes: production of 9-cis retinal and its delivery to the outer segment. As expected, the administration of 9-cis retinol to the inner segments resulted in gradual recovery of cone sensitivity, indicating that cones could oxidize 9-cis retinol and use it for pigment regeneration. However, this recovery was delayed by ∼6 min (Fig. 1B, red traces; Fig. 1C, filled red circles) from the time of retinoid application. This delay in the onset of cone recovery with 9-cis retinol was substantially larger than the ∼1 min delay observed for 9-cis retinal in the same configuration. The slight transient decrease in sensitivity upon the application of 9-cis retinol was likely due to toxicity of its high concentration in the bath when the perfusion was stopped during retinoid application. Indeed, this decrease was not observed when the 9-cis retinol solution was diluted 10-fold and the perfusion was not halted during its application, thus rapidly removing excess retinoid from the recording chamber (data not shown). The kinetics of the 9-cis retinol-driven recovery were also >3-fold slower than the recovery driven by 9-cis retinal so that cone dark adaptation was still incomplete 20 min after treatment. Thus, when the retinoid was applied to the cone inner segment, the recovery driven by 9-cis retinol was delayed by several min and proceeded >3-fold slower than the recovery driven by 9-cis retinal. This could reflect the different traffic rates of 9-cis retinal and 9-cis retinol through the cone inner segment, or could be caused by the extra oxidation step of 9-cis retinol to 9-cis retinal. However, based only on the results above, we could not determine which of these two factors causes the delay or the slower recovery of cones when their inner segments were treated with 9-cis retinol vs. 9-cis retinal.

To address this question and distinguish between these two possibilities, we treated directly the outer segments of bleached cones with 9-cis retinal and 9-cis retinol by using the outer segment-out configuration (Fig. 2A). When applied directly to the outer segment, 9-cis retinal could be immediately taken up by the cone and began driving pigment regeneration and dark adaptation within seconds (Fig. 2B; black open squares). Direct comparison of cones treated with 9-cis retinal in the outer segment-in (Fig. 3A, open squares) and outer segment-out (Fig. 3A, filled squares) configurations demonstrated that their kinetics of dark adaptation were comparable. The only difference was the ∼1 min delay in cone recovery when the chromophore was applied to the inner segment of the cones, compared to its direct application to the outer segment. This delay when 9-cis retinal is applied to the cone inner segment is comparable to that previously observed with 11-cis retinal (Jin et al., Reference Jin, Jones and Cornwall1994) and likely reflects the time required for the retinoid to reach the outer segment. Notably, the ensuing 9-cis retinal-driven pigment regeneration in our experiments was independent of the site of retinoid application and completed within 5–6 min.

Fig. 3. Comparison of the kinetics of bleached red cone recovery in outer segment-in vs. outer segment-out configurations (data replotted from Fig. 1C and 2B). (A) Sensitivity recovery time course of bleached red cones incubated with 9-cis retinal in the OS-out (filled black squares) or OS-in (open black squares) configuration. (B) Sensitivity recovery time course of bleached red cones incubated with 9-cis retinol in the OS-out (filled red circles) or OS-in (open red circles) configuration.

Having established the time course of dark adaptation driven by exogenous cis retinal in the two cell configurations, we next compared the kinetics of cone dark adaptation with cis retinol. Pigment regeneration in this case requires the additional step of oxidation to cis retinal before pigment regeneration. To investigate the subcellular localization and the kinetics of cis retinol oxidation in cones, we compared the kinetics of 9-cis retinol-driven cone dark adaptation in the outer-segment-in configuration with that of bleached cones in the outer segment-out configuration. Notably, similar to the treatment with 9-cis retinal in this configuration, and unlike the treatment with 9-cis retinol in the reverse configuration, the recovery of cone sensitivity in this case began immediately after the application of the retinoid (Fig. 2B, red open circles). Thus, cones could rapidly and efficiently utilize 9-cis retinol for robust pigment regeneration when the retinoid was applied directly to their outer segments. The kinetics of the 9-cis retinol-driven recovery of sensitivity were slower than those of the 9-cis retinal-driven recovery in this configuration (Fig. 2B), but comparable to those of the 9-cis retinol-driven recovery in the outer segment-in configuration (Fig. 3B). In both recording configurations, the kinetics of recovery with 9-cis retinol was ∼3-fold slower than that with 9-cis retinal (Figs. 1C and 2B). Together, these results suggest that the delay in cone recovery when 9-cis retinol is applied to the inner segment is most likely due to the slow transport of this retinoid to the outer segment. The immediate onset of cone recovery when 9-cis retinol is applied directly to the outer segment is consistent with the notion that its oxidation to 9-cis retinal occurs in the outer segment itself rather than in the inner segment. The ∼3-fold slower dark adaptation with 9-cis retinol over 9-cis retinal likely reflects the relatively slow oxidation of cis retinol to cis retinal in the outer segments of cones.

cis Retinol oxidation in the truncated cone outer segment

Our physiological data is consistent with the presence of cis retinol oxidation activity in cone outer segments. However, the spatial isolation between the outer and inner segments by our suction electrode was likely not ideal. Thus, the possibility still existed that in the outer segment-out configuration, 9-cis retinol from the bath could reach the tip of the inner segment and get oxidized there instead of in the outer segment. A second complication of the interpretation of our recordings arose from the slight decrease of cone sensitivity in the outer segment-in configuration upon the application of 9-cis retinol (Fig. 1C). This transient sensitivity suppression, which was not observed in the outer segment-out configuration, could also have masked any early onset of cone recovery mediated by oxidation in the inner segment. To rule out these possibilities, we tested directly the ability of truncated salamander cone outer segments to oxidize 9-cis retinol and use it for pigment regeneration. As suction recordings from truncated cone outer segments are quite challenging, we used microspectrophotometry (MSP) to measure directly pigment regeneration in 9-cis retinol-treated cone outer segments broken off from the rest of the cell. Truncated outer segments from dark-adapted red cones were identified by their shape and their characteristic absorption spectrum (Fig. 4A) with a peak at 610 ± 4 nm (mean ± s.d., n = 4), reflecting the mix of 11-cis A1 and 11-cis A2 chromophore in the retina of larval tiger salamanders (Makino et al., Reference Makino, Groesbeek, Lugtenburg and Baylor1999). The outer segments were then bleached by bright light, which, as expected, resulted in the ablation of the pigment peak in the absorption spectrum (Fig. 4B). Critically, treatment of such bleached truncated cone outer segments with 9-cis retinol resulted in robust 9-cis pigment regeneration as demonstrated by the reappearance of a blue-shifted pigment spectrum (Fig. 4C) with a peak at 544 ± 9 nm (mean ± s.d., n = 4). This peak wavelength is comparable to the reported value for the 9-cis pigment in salamander red cones (542 nm) (Makino et al., Reference Makino, Groesbeek, Lugtenburg and Baylor1999). The absorption peak disappeared after an additional bright light illumination, confirming that it originated from bleachable pigment and not from nonspecific retinoid products. This result clearly demonstrates that 9-cis retinol can be oxidized in the truncated cone outer segment and used for 9-cis pigment formation. As a control, the same experiments were done with intact salamander red rods (Fig. 4E) following a bleach (Fig. 4F). In this case, pigment regeneration was not observed after 9-cis retinol treatment (Fig. 4G). However, subsequent treatment with 11-cis retinal produced robust pigment regeneration (Fig. 4H). The inability of salamander rods to utilize 9-cis retinol for pigment regeneration is consistent with our recent finding that 9-cis retinol oxidation activity is cone-specific (Sato & Kefalov, Reference Sato and Kefalov2016). Importantly, the lack of regeneration in rods under these conditions also ruled out contamination with 9-cis retinal in our 9-cis retinol preparation. Together, these MSP results substantiate our findings from single-cell recordings above and clearly demonstrate that the oxidation of 9-cis retinol takes place in cone outer segments and can drive robust cone pigment regeneration.

Fig. 4. Microspectrophotometric measurement of pigment regeneration in a truncated cone outer segment and in an intact rod. (A) Absorbance spectrum of a dark-adapted cone outer segment. Fitted to the data is a visual pigment template with peak wavelength at 605 nm and an optical density of 0.039. (B) Absorbance spectrum of the same cone outer segment as in (A) recorded after >99% of the visual pigment had been bleached. (C) Absorbance spectrum of the same bleached cone outer segment as in (B) recorded after treatment with 9-cis retinol. Fitted to the data is a visual pigment template with peak wavelength at 549 nm and an optical density of 0.040. (D) Absorbance spectrum of the same regenerated cone outer segment as in (C) recorded after a second >99% bleach of its visual pigment. (E) Absorbance spectrum of the outer segment of an intact dark-adapted red rod. Fitted to the data is a visual pigment template with peak wavelength at 518 nm and an optical density of 0.14. (F) Absorbance spectrum of the same rod as in (E) recorded after >99% of the visual pigment had been bleached. (G) Absorbance spectrum of the same bleached rod as in (F) recorded after treatment with 9-cis retinol. (H) Absorbance spectrum of the same bleached rod as in (G) recorded after treatment with 11-cis retinal. Fitted to the data is a visual pigment template with peak wavelength at 500 nm and an optical density of 0.12.

Discussion

Oxidation and traffic of 9-cis retinol in cones

This study builds on two elegant previous studies that showed that cis retinol can drive cone pigment regeneration (Jones et al., Reference Jones, Crouch, Wiggert, Cornwall and Chader1989) and that the movement of retinoid from the inner to outer segment of salamander cones can be studied by restricting access with a suction electrode (Jin et al., Reference Jin, Jones and Cornwall1994). Here, we used a similar approach to determine the cone compartment where oxidation of cis retinol takes place. We found that when the cone outer segment was treated with 9-cis retinal, dark adaptation began essentially immediately (Fig. 2B). When the cone inner segment was treated with 9-cis retinal, the recovery onset was delayed by ∼1 min (Fig. 1C) reflecting the time required for the movement of 9-cis retinal to the outer segment before pigment regeneration can begin. The kinetics of the subsequent dark adaptation was identical in the two configurations (Fig. 3A). Notably, after its onset, the kinetics of cone recovery with 9-cis retinol in the two configurations were also identical (Fig. 3B) but ∼3-fold slower than the recovery kinetics with 9-cis retinal. This result suggests that the oxidation of cis retinol proceeds relatively slowly and might be rate-limiting for the regeneration of pigment via the retina visual cycle. On the other hand, after exposing the inner segment of bleached cones to 9-cis retinol, sensitivity recovery onset was delayed by ∼6 min. The absence of such delay in the outer segment-out configuration (Fig. 2B) allowed us to rule out slow 9-cis retinol oxidation as its source. Instead, this result suggested that this delay likely reflects the time required for 9-cis retinol to travel from the inner to the outer segments of cones, similar to the case of 9-cis retinal. Thus, the most likely explanation for our electrophysiological results is that 9-cis retinol is oxidized in the cone outer segment.

Notably, the delay in recovery onset observed in outer segment-in cones with 9-cis retinol (Fig. 1C) was similar to the delay observed in intact salamander retina [Fig. 5A in (Wang et al., Reference Wang, Estevez, Cornwall and Kefalov2009)]. Thus, even though isomeric differences between endogenous 11-cis retinoids and their exogenous 9-cis analogs used in this study could exist, they do not appear to affect dramatically cone dark adaptation. Together, our results suggest that in the intact eye, cis retinol is transported from the microvilli of Müller cells to cone outer segments via the inner segments and is then oxidized to the cis retinal needed for pigment regeneration. The substantially longer time for 9-cis retinol delivery from the inner to the outer segment compared to 9-cis retinal (Fig. 1C) suggests the presence of an efficient mechanism for transporting cis retinal from cone inner segment to the outer segment. Alternatively, the movement of cis retinol through the cone inner segment could somehow be obstructed. Photoreceptors are thought not to have retinoid binding proteins that regulate the transport of hydrophobic retinoids within the cytosol. Indeed, cellular retinal binding protein (Collery et al., Reference Collery, McLoughlin, Vendrell, Finnegan, Crabb, Saari and Kennedy2008) and cellular retinol binding protein (Bok et al., Reference Bok, Ong and Chytil1984) have not been detected from photoreceptors. Thus, chromophore-binding proteins are not likely to be involved in the regulation of retinoid transport through the cone inner segment. Finally, it is also worth pointing out that due to their different chemical nature, retinol is less hydrophobic than retinal, and would therefore be expected to partition and diffuse differently through the cellular membranes and cytosol of cone photoreceptors.

cis Retinol oxidase in cone outer segment

Our MSP data (Fig. 4) clearly demonstrate the presence of cis retinol oxidase in the outer segments of cones. This result is consistent with the hypothesis that RDH8 is the enzyme responsible for this reaction. RDH8 is expressed in cone outer segments (Maeda et al., Reference Maeda, Maeda, Imanishi, Kuksa, Alekseev, Bronson, Zhang, Zhu, Sun, Saperstein, Rieke, Baehr and Palczewski2005; Miyazono et al., Reference Miyazono, Shimauchi-Matsukawa, Tachibanaki and Kawamura2008) and shows weak but detectable activity to cis retinoid (Rattner et al., Reference Rattner, Smallwood and Nathans2000). In addition, deletion of RDH8 blocks the sensitivity recovery with exogenous 9-cis retinol in mouse M-cones (Kolesnikov et al., Reference Kolesnikov, Maeda, Tang, Imanishi, Palczewski and Kefalov2015). However, RDH8 is expressed not only in cones but also in rods (Maeda et al., Reference Maeda, Maeda, Imanishi, Kuksa, Alekseev, Bronson, Zhang, Zhu, Sun, Saperstein, Rieke, Baehr and Palczewski2005; Miyazono et al., Reference Miyazono, Shimauchi-Matsukawa, Tachibanaki and Kawamura2008), a distribution inconsistent with the cone-specific oxidation of cis retinol. One possibility is that RDH8 is not itself the cis retinol dehydrogenase, but rather it supports this reaction by providing NADP+ through the reduction of all-trans retinal (Kaylor et al., Reference Kaylor, Cook, Makshanoff, Bischoff, Yong and Travis2014). Further studies will be needed to determine the exact involvement of RDH8 in the retina visual cycle.

In contrast to our finding from salamander, a recent biochemical study reported cis-retinol oxidation activity in the carp cone inner segments but not in the outer segments (Sato et al., Reference Sato, Fukagawa, Tachibanaki, Yamano, Wada and Kawamura2013; Sato et al., Reference Sato, Miyazono, Tachibanaki and Kawamura2015). RDH13L, the enzyme responsible for this inner segment activity, is localized in the inner segments of carp cones but it is not found in the amphibian genome. Notably, a functional homologue of RDH13L, RDH14, is expressed in rod and cone outer segments in bovine retina (Haeseleer et al., Reference Haeseleer, Jang, Imanishi, Driessen, Matsumura, Nelson and Palczewski2002). However, the functional role of RDH14 in the retina visual cycle, and specifically in the oxidation of 11-cis retinol, is still unknown. The conflicting results obtained from salamander cones (this study) and from carp cones (Sato et al., Reference Sato, Fukagawa, Tachibanaki, Yamano, Wada and Kawamura2013; Sato et al., Reference Sato, Miyazono, Tachibanaki and Kawamura2015) may simply reflect interspecies difference. Alternatively, co-factors or other reaction modifiers could be required for the efficient oxidation of cis retinol in cones. In that case, their availability or absence in different experimental conditions could determine the subcellular location of this reaction. Similarly, the presence or absence of cellular compartmentalization in different experimental conditions could also affect the efficiency of cis retinol oxidation. Nevertheless, the robust pigment regeneration and dark adaptation observed in our experiments with cone outer segment-delivered 9-cis retinol clearly demonstrate the presence of cis retinol dehydrogenase activity in the outer segments of cones but not rods.

Finally, it is also possible that another enzyme, different from RDH8 and RDH14, is responsible for the oxidation of cis retinol in the outer segments of cones. Notably, RPE65, the isomerohydrolase of the canonical RPE visual cycle, was recently shown to be expressed in the outer segments of cones in some mouse strains (Tang et al., Reference Tang, Wheless and Crouch2011 b) as well as in humans (Tang et al., Reference Tang, Buhusi, Ma and Crouch2011 a). It has been suggested that this protein might be involved in the cone visual cycle by acting as a retinol-binding protein (Tang et al., Reference Tang, Kono, Koutalos, Ablonczy and Crouch2013). An interesting possibility is that RPE65 might interact with the cone-specific RDH and, in that way, facilitate the oxidation of cis retinol in cones. However, the functional role of RPE65 in cones is still unclear and its possible involvement in the retina visual cycle has not been explored.

Co-factor driving the cis retinol oxidation in cones

Previous studies with amphibian rods (Kawamura & Murakami, Reference Kawamura and Murakami1989) and fish rods and cones (Takemoto et al., Reference Takemoto, Tachibanaki and Kawamura2009) both suggest that the inside of the truncated outer segment remains accessible to bath-applied compounds. Thus, the truncated outer segments in our experiments also likely remained open, allowing wash out of small molecules from the cytoplasm. NADP+ is thought to be a cofactor in the cone-specific cis retinol oxidation (Mata et al., Reference Mata, Radu, Clemmons and Travis2002). However, we observed 9-cis retinol-driven pigment regeneration in the truncated cone outer segment (Fig. 4) even though NADP+ was expected to be washed out rapidly. Thus, the cofactor for cis retinol oxidation in the truncated cone outer segment is not likely to be NADP+. A possible alternative co-factor is all-trans retinal, which is insoluble and shown to work as a co-factor in the cis retinol oxidation reaction by carp RDH13L and mouse RDH14 (Sato et al., Reference Sato, Miyazono, Tachibanaki and Kawamura2015). All-trans retinal is released at a high concentration (up to 3 mM) in cone outer segments following the bleaching of their visual pigments (Harosi, Reference Harosi1975). In the intact cones, all-trans retinal is then rapidly converted to all-trans retinol by NADPH-driven reduction (Ala-Laurila et al., Reference Ala-Laurila, Kolesnikov, Crouch, Tsina, Shukolyukov, Govardovskii, Koutalos, Wiggert, Estevez and Cornwall2006). However, our attempt to detect acceleration of cis retinol oxidation by all-trans retinal was not successful: addition of all-trans retinal to the 9-cis retinol treatment of either outer segment-in (Fig. 1A) or outer segment-out (Fig. 2A) bleached cones did not affect the kinetics of cone dark adaptation (data not shown). Thus, the cofactor for cis-retinol oxidation is still unclear and further experiments will be needed to clarify the molecular mechanism of this key reaction of the retina visual cycle. Our finding that the oxidation of cis retinol takes place in the outer segments of cones should inform future studies and help in the eventual identification of the enzyme responsible for this reaction.

Author contribution

SS and VJK designed the study and wrote the paper. SS and VJK designed, performed, and analyzed the experiments shown in Figs. 1, 2, and 3. RF and MCC designed, performed, and analyzed the experiments shown in Fig. 4. All authors reviewed the results and approved the final version of the manuscript.

Acknowledgments

This work was supported by National Institutes of Health (NIH) grants EY019312 and EY025696 (V.J.K.), EY001157 (M.C.C.), EY002687 to the Department of Ophthalmology and Visual Sciences at Washington University, and by Research to Prevent Blindness. We are grateful to the National Eye Institute and Rosalie Crouch from the Medical University of South Carolina for the 11-cis retinal.

References

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Figure 0

Fig. 1. Kinetics of red cone sensitivity recovery when exposing the inner segment to exogenous 9-cis chromophore. (A) Image of a red cone in the outer segment-in configuration under microscope with infrared illumination. (B) Dim flash responses from bleached red cones at indicated times after treatment with 9-cis retinal (black traces) and 9-cis retinol (red traces). Response amplitudes are normalized to the flash intensity (i.e. response per photon) to allow direct comparison of sensitivity. (C) Sensitivity recovery time course of bleached red cones in the outer segment-in (OS-in) configuration incubated with 9-cis retinal (filled black squares; n = 10) or 9-cis retinol (filled red circles; n = 8). Data are shown as mean ± SEM.

Figure 1

Fig. 2. Kinetics of red cone sensitivity recovery when exposing the outer segment to exogenous 9-cis chromophore. (A) Image of a red cone in the outer segment-out configuration under microscope with infrared illumination. (B) Sensitivity recovery time course of bleached red cones in the outer segment-out (OS-out) configuration incubated with 9-cis retinal (open black squares; n = 7) or 9-cis retinol (open red circles; n = 8). Data are shown as mean ± SEM.

Figure 2

Fig. 3. Comparison of the kinetics of bleached red cone recovery in outer segment-in vs. outer segment-out configurations (data replotted from Fig. 1C and 2B). (A) Sensitivity recovery time course of bleached red cones incubated with 9-cis retinal in the OS-out (filled black squares) or OS-in (open black squares) configuration. (B) Sensitivity recovery time course of bleached red cones incubated with 9-cis retinol in the OS-out (filled red circles) or OS-in (open red circles) configuration.

Figure 3

Fig. 4. Microspectrophotometric measurement of pigment regeneration in a truncated cone outer segment and in an intact rod. (A) Absorbance spectrum of a dark-adapted cone outer segment. Fitted to the data is a visual pigment template with peak wavelength at 605 nm and an optical density of 0.039. (B) Absorbance spectrum of the same cone outer segment as in (A) recorded after >99% of the visual pigment had been bleached. (C) Absorbance spectrum of the same bleached cone outer segment as in (B) recorded after treatment with 9-cis retinol. Fitted to the data is a visual pigment template with peak wavelength at 549 nm and an optical density of 0.040. (D) Absorbance spectrum of the same regenerated cone outer segment as in (C) recorded after a second >99% bleach of its visual pigment. (E) Absorbance spectrum of the outer segment of an intact dark-adapted red rod. Fitted to the data is a visual pigment template with peak wavelength at 518 nm and an optical density of 0.14. (F) Absorbance spectrum of the same rod as in (E) recorded after >99% of the visual pigment had been bleached. (G) Absorbance spectrum of the same bleached rod as in (F) recorded after treatment with 9-cis retinol. (H) Absorbance spectrum of the same bleached rod as in (G) recorded after treatment with 11-cis retinal. Fitted to the data is a visual pigment template with peak wavelength at 500 nm and an optical density of 0.12.