GABAC Receptors Are Localized with Microtubule-Associated Protein 1B in Mammalian Cone Photoreceptors

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The Journal of Neuroscience, September 15, 2000, 20(18):6789-6796

GABA_C Receptors Are Localized with Microtubule-Associated Protein 1B in Mammalian Cone Photoreceptors
Bikash Pattnaik, Abdeljelil Jellali, José Sahel, Henri Dreyfus, and Serge Picaud
Laboratoire de Physiopathologie Cellulaire et Moléculaire de la Rétine, Institut National de la Santé et de la Recherche Médicale EMI 99-18, University Louis Pasteur, 67091 Strasbourg Cedex, France

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Protein MAP1B was recently reported to link GABA_C receptors to the cytoskeleton at neuronal synapses. This interaction wasdemonstrated in the mammalian retina, where GABA_C receptors werethought to be exclusively expressed in bipolar cells. Our previousstudies on cultured photoreceptors suggested however the presenceof GABA_C receptors in cones. To further investigate GABA_C receptorexpression in cones, we measured GABA responses in mammalian photoreceptorsin situ, and we examined the distribution of the receptor andthat of protein MAP1B in the mammalian outer retina. Photoreceptorswere recorded from flat-mounted retinas of retinal degenerationmice at an age when the retina becomes cone-dominated after rodcell death. GABA_A and GABA_C-gated currents were produced onlyin cones but not rods. Recording freshly dissociated retinal cellsfrom wild-type C57 mice confirmed the presence of GABA_A and GABA_Creceptors in cones. Immunohistochemical labeling of mouse andrat retinal sections localized GABA_C receptors to cone terminalsthat were identified by peanut agglutinin lectin staining. Asexpected from previous studies on bipolar cells, the punctateimmunostaining was not restricted to cone terminals in the outerplexiform layer. MAP1B immunolabeling was obtained in rat andpig retinas and was similarly found in cone terminals identifiedby the peanut agglutinin lectin staining. These results providephysiological and histological evidence that cones receive a GABAfeedback in the mammalian retina and are consistent with the notionthat protein MAP1B links GABA_C receptors to the cytoskeleton atpostsynapticsites.

Key words: GABA; GABA_A receptor; GABA_C receptor; MAP1B; retina; photoreceptor; cone

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

GABA_C receptors were recently classified in the GABA_A receptor family (Barnard et al., 1998), although this concept is notwidely accepted (Bormann, 2000). GABA_C receptors gate a Cl channel similar to GABA_A receptors but exhibit a different pharmacologicalprofile (Bormann, 2000). The main difference with conventionalGABA_A receptors is their bicuculline and barbiturate resistances;specific antagonists to GABA_C receptors are also available (Ragozzinoet al., 1996). Furthermore, GABA_C receptors, in contrast to GABA_Areceptors, do not desensitize, rendering them particularly wellsuited for processing gradedpotentials.

GABA_C receptor $rho$ subunits share only 30% homology with GABA_A receptor subunits. All $rho$ subunits, except rat $rho$ 2 subunits, canform homomeric GABA-gated Cl channels, most of which are sensitive to picrotoxin. Only ratand mouse $rho$ 2 subunits are insensitive to picrotoxin and can conferthis picrotoxin insensitivity to heteromeric channels (Cuttinget al., 1991; Wang et al., 1994; Zhang et al., 1995; Shingai etal., 1996; Enz and Cutting, 1998; Greka et al., 1998). Recently,the microtubule-associated protein MAP1B that was found to specificallyinteract with GABA_C receptor $rho$ 1 subunits, was proposed to linkthe receptor to the cytoskeleton (Hanley et al., 1999). The MAPproteins are known to stabilize microtubules, the most abundantmembers of the family being the proteins tau and MAP2, which arelocated predominantly in axons and dendrites, respectively. Bycontrast, GABA_A receptors were found to be linked to the cytoskeletonvia gephyrin (Kneussel et al., 1999) or GABA receptor-associatedprotein (GABARAP) (Wang et al., 1999).

In the retina, GABA_C receptors have been recorded in bipolar cells (Feigenspan et al., 1993; Lukasiewicz et al., 1994), horizontalcells (Qian and Dowling, 1993; Dong et al., 1994), and ganglioncells (Zhang and Slaughter, 1995). In the mammalian retina, GABA_Creceptor currents were first reported in bipolar cells (Feigenspanet al., 1993; Euler and Wässle, 1998). This bipolar cell localizationwas confirmed by immunocytochemistry (Enz et al., 1996; Koulenet al., 1998) and in situ hybridization (Enz et al., 1995). Consistentwith its proposed linkage to GABA_C receptors, MAP1B was distributedin the inner plexiform layer and more specifically at bipolarcell terminals (Hanley et al., 1999). The $rho$ 3 subunits were localizedby in situ hybridization to cells in the ganglion cell layer (Ogurusuet al., 1997). The presence of GABA_A and GABA_C receptors in mammaliancones was recently suspected after recording porcine photoreceptorsusing a pure photoreceptor cell culture (Picaud et al., 1998).However, this physiological evidence of GABA_C receptors in coneswas neither supported by previous immunocytochemical nor in situhybridization studies (Enz et al., 1995, 1996; Koulen et al.,1998).

To determine whether cones do normally express GABA_C receptors, their responses to GABA were recorded in flat-mounted mouseretina. In parallel, retinal sections were immunolabeled withantibodies directed against either MAP1B or the $rho$ subunits. Thisstudy further suggests the implication of GABA_C receptors in conephysiology and is in agreement with GABA_C receptor interactionwithMAP1B.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Electrophysiological recording. C3H/He/J mice homozygous for the retinal degeneration (rd1) gene aged 20-30 d were procuredfrom Janvier Animal Suppliers (Le Genest St. Isle, France) andmaintained in standard laboratory conditions. After killing, theeyes were removed and placed in Ringer's saline. The lens andvitreous were removed, and the retina was separated from the posterioreyecup and placed flat with the photoreceptor surface up in aperfusion chamber. The retina was maintained flat by overlayingwith a nylon mesh. As previously described for preparing cultures,retinal cells were enzymatically dissociated in 0.2% papain for30 min (Picaud et al., 1998). Conventional whole-cell patch-clamprecordings were performed on photoreceptor cells at room temperatureusing bath solutions containing (in mM): 135 NaCl, 5 KCl, 1 CaCl₂,1 MgCl₂, 10 glucose, and 5 HEPES (pH-adjusted to 7.75 using NaOH).The patch pipettes were pulled from thin-walled borosilicate glass(TW 150F; World Precision Instruments) using a Brown and Flamingtype puller (P-87; Sutter Instruments, Novato, CA). They werefilled with the recording solutions containing (in mM): 140 KCl,1 MgCl₂, 0.5 EGTA, 5 ATP (disodium), and 4 HEPES (pH-adjustedto 7.4 with KOH). When using the equilibrium potential (E_Cl) at $-$ 30 mV, 98 mM K-gluconate was substituted for KCl. The membranecurrents were measured using an RK-400 patch amplifier (Biological,Grenoble, France). Liquid junction potentials were corrected byusing standard procedure. Data acquisition and analysis were performedusing Patchit and Tack software packages, respectively (Grantand Werblin, 1994). Data were filtered at 3 kHz and digitizedat either 10 kHz during voltage steps or 1 Hz during neurotransmitterapplications using a data acquisition labmaster board (ScientificSolution, Solon, OH) mounted in an IBM-compatible personal computer(PC).

Drugs were added to the bath solutions and were applied by a local gravity-driven perfusion system controlled by a manualsolution changer. A 1 mM concentration of GABA was puffed on theproximity of the recorded cell through a pulled glass capillary(TW 100F; World precision Instruments) that was controlled (durationas indicated in the figure legends; 20 psi) by a picospritzer(Picospritzer II General Valve Corporation, Fairfield, NJ), monitoredthrough the PC. All experiments were performed on at least threecells, and the results are represented as mean ±SEM.

Immunohistochemistry and cell identification. Recorded cells were filled during the experiments by including Sulforhodamine-101in the pipette recording solution. Retinas were fixed for 1 hrat 4°C with 4% paraformaldehyde in 0.1 M PBS. Rods were labeledwith the rhodopsin antibody rho-4D2 (Hicks and Molday, 1986; kindlyprovided by D. Hicks) with a similar protocol as the one describedbelow on sections. Immunolabeling for MAP1B (Clone AA6; Sigma,St. Louis, MO) and GABA_C receptor (gift of Dr. R. Enz and Prof.H. Wässle, Max Planck Institute, Frankfurt, Germany), as wellas staining with peanut agglutinin lectin (Sigma), were performedon frozen retinal sections (8 µm thickness). For the GABA_C receptorantibody, the anterior segment was removed, and the whole eyecupwas fixed in 4% paraformaldehyde in 0.1 M PBS for 5 min. For MAP1Bimmunolabeling, fixation was performed directly on sections. Sectionswere washed in PBS, permeabilized in PBS containing 0.1% TritonX-100 for 5 min, then bathed in PBS containing 1% bovine serumalbumin for 30 min at 37°C and incubated in the same solutionwith the primary antibody for 2 hr at room temperature. The sectionswere washed three times and incubated with the secondary antibody[rabbit anti-mouse conjugated to Texas Red or fluorescein isothiocyanate(Molecular Probes, Eugene, OR) diluted 1:200] for 1 hr at roomtemperature. The lectin staining was obtained by bathing the sectionswith peanut agglutinin lectin coupled to Texas Red (50 µg/ml finalconcentration) for 1 hr at room temperature. Diamidino-phenylindole(DAPI) nuclear labeling was finally performed in PBS during 2min.

Western blot of retinal homogenates. Homogenates from entire porcine retinas were centrifuged (65 × g) for 5 min at 4°C inTris buffer (10 mM, pH 7.4). Pellets were suspended in the Trisbuffer containing 1 mM EDTA, a mixture of protease inhibitors(protease inhibitor cocktail tablets; Boehringer Mannheim, Mannheim,Germany), 100 µM phenylmethylsulfonylfluoride (PMSF), and centrifuged(11,000 × g) for 10 min at 4°C. Cytoplasmic proteins in the supernatantwere denatured in SDS sample buffer containing 100 mM dithiothreitol;their concentration was measured using bovine serum albumin asa standard. Protein samples of 20 µg were then electrophoresedon a 8% SDS-PAGE and transferred onto a nitrocellulose membrane(Schleicher and Schuell, Dassel, Germany). The membrane was incubatedin 1% bovine serum albumin, 0.1 M PBS, pH 7.4, at 37°C for 1 hr,and then with MAP1B monoclonal antibody (1:500 in 1% bovine serumalbumin and 0.1% Tween 20, 0.1 M PBS, pH 7.4) for 2 hr at roomtemperature. After a 15 min wash, the nitrocellulose membranewas incubated with the secondary antibody, and rabbit anti-mouseIgGs were conjugated to the alkaline phosphatase (1:5000) for2 hr at room temperature. The enzyme was visualized with nitroblue tetrazolium/5-bromo-4-chloro-3-indolyl phosphate in 0.1 MTris-acetate, pH 9.5.

Chemicals and proteins. All chemicals, lectin, and antibodies for which the source is not mentioned were provided from Sigma.The GABA_A antagonist 2-(carboxy propyl-3-amino-6,4-methoxy phenyl)pyradazynium bromide (SR95531) was purchased from Research Biochemicals(Natick, MA), and GABA_C antagonist (1,2,5,6-tetrahydro-pyridine-4-yl)methyl phosphonic acid (TPMPA) was obtained from Tocris (Bristol,UK).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Rod and cone identification in flat-mounted retinas

Cone photoreceptors were recorded from 20- to 30-d-old rd mice, in which a mutation in the rod cGMP-dependent phosphodiesteraseinduces early onset of rod cell degeneration, leaving cones easilyaccessible to the patch-clamp recording pipette. Figure 1 illustratesa recorded cell with neighboring photoreceptors. Only very fewremaining rods can be observed after immunolabeling with an anti-rhodopsinantibody (rho-4D2) among photoreceptors stained in the outer nuclearlayer with the nuclear dye DAPI (Fig. 1B,C). Cells were selectedfor recording in the outer nuclear layer under Nomarski optics.Recorded cells were classified in two groups according to theircharacteristics (Fig. 2). Based on the rod to cone ratio, thesegroups were easily assigned to either cones or rods. Figure 2,A and B, illustrates the two representative types of responsesto voltage steps that were recorded in rods and cones, respectively.These responses were similar to those obtained from cultured rodsand cones from the pig retina (data not shown). To verify cellularidentity, recorded cells were filled with sulforhodamine-101 (SR101),and the retina was subsequently labeled with rho-4D2. In Figure1, the recorded cell is brightly stained with SR101 (Fig. 1A)but is immunonegative for rhodopsin (Fig. 1B) (only the nuclearstaining with SR101 leaks through the filter). The outer nuclearlayer location established photoreceptor identity, and the opsinimmunonegativity indicated it was not a rod but a cone. All conesidentified this way had a response to voltage steps similar tothat presented in Figure 2, B and C. The other type of responseto voltage steps (Fig. 2A,C) was attributed to rods because itwas identical to those recorded from cultured pig rods. No dyecoupling was observed between photoreceptor cells. These resultsindicated that both rods and cones can be recorded from the flat-mountedrd mouse.

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Figure 1. Cone morphology in flat-mounted rd mouse retina. The recorded cell (arrow) was stained with the dye sulforhodamine 101, which was included in the recording pipette solution and passively diffused into the cell during the recording (A). After fixation, rods were immunolabeled with the rhodopsin antibody (rho-4D2) and a secondary antibody coupled to fluorescein (B). The recorded cell is not immunolabeled itself, its nuclei was fluorescent under blue illumination because the red fluorescence of sulforhodamine 101 leaked through the filter. Photoreceptor cell nuclei were visualized with the nuclear dye DAPI (C). Note that the recorded cell was in the same focal plane as immunolabeled rods.

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Figure 2. Electrophysiological identification of rod and cone photoreceptors in flat-mounted rd mouse retina. Current responses to voltage steps in a representative rod (A) and cone (B). The potential was stepped from a holding potential of $-$ 70 mV to potentials ranging from $-$ 120 to +40 mV in 20 mV increments. C, Averaged current-voltage curves of rod and cone response to voltage steps (cones, n = 20; rods, n = 5; ±SEM). Cones typically exhibited a large outward current at potential superior to $-$ 30 mV, whereas rods showed an inward current activated at the most negative potentials. D, Rod and cone photoreceptor responses to a GABA puff application (1 mM, 1 sec). GABA elicited a large current in cones but not in rods.

Responses to GABA application

When GABA (1 mM) was puff-applied onto recorded mouse photoreceptors held at a potential of $-$ 70 mV, rods did not show anyresponse (Fig. 2D). By contrast, cones generated a large currentranging from 150 to 375 pA (Fig. 2D). The reversal potential ofGABA-elicited currents was estimated from voltage ramp measurements.Whole-cell currents were recorded in the absence of GABA and duringa long GABA puff (Fig. 3A). The GABA-elicited current was thencalculated by subtracting the measurement in the absence of GABAfrom that in the presence of GABA. In experiments where the Cl concentration was almost symmetrical (Fig. 3B), the reversalpotential of GABA-elicited currents were close to 0 mV ( $-$ 4.16± 3.8 mV; n = 4). When gluconate was substituted for Cl in the recording pipette solution (Fig. 3B), the reversal potentialapproximately followed the Cl equilibrium potential (E_Cl = $-$ 30 mV; E_rev = $-$ 33.96 ± 1.27 mV;n = 3). These results indicated that GABA was activating Cl channels in mouse cone photoreceptors.

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Figure 3. GABA generated a Cl conductance in cone photoreceptors. A, Whole-cell currents were recorded from cone photoreceptors in the presence or absence of a GABA (1 mM) puff application, whereas the membrane potential was ramped from $-$ 100 to 60 mV at 0.72 mV/msec. Between recordings, cells were held at 0 mV to suppress K⁺ currents. B, The GABA-elicited current was calculated by subtracting the whole-cell current measured in the absence of GABA from that obtained in the presence of GABA. This measurement is illustrated for two cells in which the equilibrium potentials for Cl (E_Cl) were set at either $-$ 30 mV (as in A) or 0 mV by using recording pipette solutions with different Cl concentrations (see Materials and Methods). Under these conditions, the reversal potential of the GABA-elicited current approximately follows the equilibrium potential for Cl.

Pharmacology of GABA responses

Figure 4 shows the pharmacological profile of the GABA-evoked current recorded from cone photoreceptors voltage-clamped toa holding potential of $-$ 70 mV. When the GABA_A receptor blockerSR95531 (100 µM) was bath-applied (Fig. 4A), GABA responses werereduced by 74.6% (±1.2%; n = 6), and responses were recoveredafter washing. Responses were further suppressed by 93.8% (±1.5%)in the same cells when the GABA_C receptor antagonist TPMPA (50µM; Ragozzino et al., 1996), was coapplied with SR95531 to theretina (Fig. 4A). Similarly, TPMPA alone decreased the GABA responseby 30.8% (±4.0%; n = 5) (Fig. 4A). Bicuculline (100 µM), anotherknown GABA_A receptor antagonist, also partially blocked the GABAresponse by 47.81% (±6.6%; n = 3). To measure the effect of picrotoxin(100 µM) on the GABA_C receptor, it was applied together with bicuculline.Under these conditions, picrotoxin suppressed 91.89% (±1.3%; n= 3) of the GABA_C receptor current (Fig. 4B). In the latter experiment,photoreceptors were pharmacologically isolated from the retinalnetwork with a solution containing CNQX (50 µM), strychnine (30µM), and AP-4 (100 µM). The observation of both a GABA_A and aGABA_C receptor component under these conditions (Fig. 4B) confirmedthat GABA acted directly on the recorded cells. These pharmacologicaldata strongly suggest that both GABA_A and GABA_C receptors arepresent in cone photoreceptors. Note that the decay of GABA_A receptor-mediatedcurrent was much faster compared to those of GABA_C receptors inthe same cell (Fig. 4C). Variations in the onset of the responseswere also observed from cells to cells and were attributed tothe different accessibility to the synaptic cleft in this retinalwhole-mount preparation. In experiments described below, the GABA_Creceptor current was isolated by bath applying SR95531, whereasthe GABA_A receptor component was obtained by using TPMPA in theperfusion solution.

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Figure 4. Pharmacology of cone GABA currents in flat-mounted rd retina. A, GABA puffs (1 mM, 1 sec) were successively applied, as indicated in the presence of either GABA_A or GABA_C receptor antagonists SR95531 (100 µM) and TPMPA (50 µM), respectively, or both. B, GABA puffs (1 mM, 50 msec) were applied in presence of bicuculline (100 µM) alone and together with picrotoxin (100 µM). These effects of bicuculline and picrotoxin were measured in a bathing solution containing CNQX (50 µM), strychnine (30 µM), and AP-4 (100 µM) to pharmacologically isolate cones. C, The kinetics of the SR95531- and TPMPA-resistant currents are compared after normalizing the recording shown in A.

Modulation of GABA receptors

A major difference between GABA_A and GABA_C receptors is their respective sensitivity to benzodiazepines, GABA_A receptor currentsbeing greatly increased, whereas GABA_C currents are not affected(Shimada et al., 1992). To verify the presence of these two typesof currents, the effect of pentobarbital (100 µM) was tested onthe respective components pharmacologically isolated as describedabove. Figure 5 illustrates the pentobarbital-induced increasein the TPMPA-resistant GABA_A receptor current in a cone whilethe SR95531-resistant GABA_C receptor component was barely affectedin the same cell. The GABA_A receptor current increased by 85±4.6% (n = 3) in amplitude, whereas the GABA_C receptor currentshowed a slight increase (20 ± 0.35%) in the same three cells.These effects are consistent with the presence of both GABA_A andGABA_C receptor components in cone photoreceptor GABA response.

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Figure 5. Pentobarbital (PBT) modulation on GABA_A and GABA_C receptor currents in flat-mounted rd mouse retina. Pentobarbital (100 µM) was bath-applied together with either SR95531 or TPMPA, which isolated the GABA_C and GABA_A receptor currents, respectively. Pentobarbital had no significant effect on the SR95531-resistant or GABA_C receptor current, whereas it increased the amplitude and slowed down the decay of the TPMPA-resistant or GABA_A receptor current (GABA puff, 1 mM, 1 sec).

Kinetics of the GABA response

To further assess the kinetics of the GABA response, GABA was applied for long duration (6 sec). When the GABA_C receptor componentwas suppressed by TPMPA application (50 µM; Fig. 6), the remainingGABA_A response desensitized during the 6 sec application by 84%of its initial amplitude. By contrast, the GABA_C receptor componentisolated in the presence of SR95531 (100 µM) was only reducedby 24% during the 6 sec application (Fig. 6). These differentkinetics are consistent with the expression of desensitizing GABA_Areceptors and nondesensitizing GABA_C receptors in cone photoreceptors.

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Figure 6. Kinetics of the GABA_A and GABA_C receptor currents. Long GABA puff applications (1 mM, 6 sec) were delivered in the absence or presence of SR95531 (100 µM) and TPMPA (50 µM). The SR95531-resistant or GABA_C receptor current remained sustained during the time of application, whereas the TPMPA-resistant or GABA_A receptor current rapidly decreased in amplitude during the puff.

Recordings of freshly dissociated photoreceptors

To test whether cones in wild-type mice would similarly generate GABA_A and GABA_C receptor currents, retinal neurons from C57mouse retina were dissociated and immediately recorded. Becausecones represent only 1% of all photoreceptors in the mouse retina,many experiments were required to identify and record only fourcones. These cones had similar responses to voltage steps (Fig.7A) as those recorded from cones in the rd mouse (Fig. 2B). GABAapplication elicited responses that were blocked partially (70.6± 2.56%; n = 4) by SR95531 (100 µM) and completely (97.62 ± 0.27%)by coapplication of SR95531 together with TPMPA (50 µM) (Fig.7B,C). This observation confirmed our results on the rd mouse,demonstrating the presence of GABA_A and GABA_C receptors in mammaliancone photoreceptors in situ.

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Figure 7. GABA_A and GABA_C receptors in freshly dissociated C57 mouse cones. A, Current responses to voltage steps in an isolated cone voltage-clamped at $-$ 70 mV and stepped in 20 mV increments from $-$ 120 to +40 mV. B, GABA-elicited response in the same freshly dissociated cone in the presence of GABA_A receptor antagonist SR95531 alone and with TPMPA, respectively (GABA puff 1 mM, 1 sec). C, Maximum amplitude of the GABA responses in the absence or presence of SR95531 (100 µM) and TPMPA (50 µM).

GABA_C receptor and MAP1B localizations in the outer retina

To determine whether GABA_C receptors are expressed in mammalian cone photoreceptors, we investigated the distribution of thereceptors and that of protein MAP1B in the outer retina. Becausethe MAP1B antibody did not cross-react with mouse tissue, we examinedMAP1B localization in the rat retina (Fig. 8). Photoreceptor outersegments, fibers in the outer nuclear layer, and structures inthe outer plexiform layer were MAP1B-immunopositive (Fig. 8A).To verify that these structures represented cone terminals, retinalsections were labeled with peanut agglutinin lectin that bindsselectively to cone extracellular matrix. A few cones were stainedin each microscopic field at the level of their outer segments(Fig. 8B-D). Similar to the MAP1B antibody, structures with thesame shape were also heavily stained at the same position andspacing in the outer plexiform layer, suggesting that cone terminalswere MAP1B-immunopositive. In addition to the inner plexiformlabeling previously described (Hanley et al., 1999), rare cellbodies were also brightly stained in the proximal part of theinner nuclear layer with processes extending in the inner plexiformlayer (data not shown).

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Figure 8. GABA_C receptor and MAP1B immunolocalizations in the rat retina. A-D, Rat retinal sections were labeled with a MAP1B antibody (A), peanut agglutinin lectin (B), and nuclear stain DAPI (C) or visualized with Nomarski image (D). Photographs (B-D) were taken from the same section, only the right part of B is shown in C and D. MAP1B immunolabeling (A) is observed in photoreceptor outer segments, processes crossing the outer nuclear layer and structures in the outer plexiform layer (A, small arrow). Similar structures are also observed in sections stained with peanut agglutinin lectin that selectively labels cones (B, large arrow) identifying these structures as cone photoreceptor terminals (B, small arrow). E, Western blot of MAP1B from a retinal homogenate showing that the antibody identified a retinal protein at the expected molecular mass (~300 kDa; Edelmann et al., 1996) of protein MAP1B. F-H, Rat retinal sections were labeled for the GABA_C receptor (F, G) and peanut lectin agglutinin (H). A punctate immunolabeling is observed in the outer plexiform layer where some immunopositive structures (G, arrows) are also stained with the cone peanut agglutinin lectin (H, arrow). Scale bar: A-D, 10 µm; F, 16 µm; G, H, 7.3 µm.

When rat retinas were stained with GABA_C receptor antibodies, punctate immunolabeling was observed in the outer plexiformlayer (Fig. 8F). By contrast to the porcine retina (Picaud etal., 1998), no staining was found in the outer nuclear layer.Double staining of the sections with the peanut agglutinin lectinidentified some of the immunopositive structures as cone terminals(Fig. 8G,H). A similar GABA_C receptor staining was also observedin the mouse outer retina (Fig. 9A), where immunopositive structuresappeared to colocalize with the peanut agglutinin lectin stainingof cone terminals (Fig. 9B-D). Although these stainings clearlydemonstrated that GABA_C receptors were not restricted to coneterminals in the outer plexiform layer, they indicated that MAP1Band GABA_C receptors were both localized at mammalian cone terminals.

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Figure 9. GABA_C receptor immunostaining in the mouse retina. Mouse retinal sections were labeled with the GABA_C receptor antibodies (A, C) and peanut lectin agglutinin (B). A punctate immunolabeling is observed in the outer plexiform layer where some immunopositive structures (C, arrows) appear also stained with the cone peanut agglutinin lectin (B, arrows). An image taken with the two stainings superimposed is presented to ease the localization of the cone terminals labeled with the peanut agglutinin lectin (D, arrows). Scale bar: A, 30 µm; B-D, 9 µm.

The distribution of MAP1B was also investigated in the pig retina because cones are more numerous than in rats and are moreeasily identifiable as a single row of nuclei at the distal edgeof the outer nuclear layer (Fig. 10). Furthermore, the presenceof GABA_C receptors in porcine cones was suggested by our previousstudy on cultured photoreceptors (Picaud et al., 1998). MAP1Bimmunolabeling was mostly restricted to the outer retina (Fig.10A,B), but weak discrete staining was also observed in the innerplexiform layer and in ganglion cell axons. At higher magnification,photoreceptor outer segments, a row of nuclei at the distal borderof the outer nuclear layer, their cell processes, and terminalsin the outer plexiform layer were all intensely labeled (Fig.10D). To confirm that immunopositive terminals in the outer plexiformlayer belonged to cones, retinal sections were double-stainedwith peanut agglutinin lectin (Fig. 10F) and MAP1B antibody (Fig.10G). Cone terminals that were stained with the lectin were clearlyimmunolabeled with the MAP1B antibody (Fig. 10F,G, arrows). Therecording of GABA_C receptors in cones and the MAP1B immunostainingof these neurons are consistent with the notion that MAP1B maylink GABA_C receptors to the cytoskeleton in mammalian cone photoreceptors.

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Figure 10. MAP1B distribution in porcine retinal sections. Porcine retinal sections were examined after staining with MAP1B antibody (A, D, F), DAPI (B, E) and peanut agglutinin lectin (G) or visualized under Nomarski image (C). An intense MAP1B immunolabeling is observed in the outer retina contrasting with the weak or no labeling in the inner retina (A, B). At higher magnification (D), this labeling is found in photoreceptor outer segments, a row of nuclei at the distal border of the outer nuclear layer where cone cell bodies are localized, in the axons of these cell bodies, and finally in their terminals located at the distal border of the outer plexiform layer. When retinal sections were double-labeled with fluorescein for MAP1B (F) and Texas Red for peanut agglutinin lectin (G), lectin-stained terminals (G, arrows) were also immunopositive for MAP1B (F, arrows), identifying these labeled cells as cone photoreceptors. Scale bar: A, B, 20 µm; C-G, 10 µm.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In the present study, mouse rods and cones were electrophysiologically recorded in situ. Both GABA_A and GABA_C receptor activationwas detected in cone photoreceptors, whereas rods did not respondto GABA application. MAP1B that is known to link GABA_C receptorsto the cytoskeleton was localized throughout mammalian cone photoreceptorsup to their terminals. This localization of MAP1B in cone terminalsis in agreement with the idea that GABA_C receptors are localizedat cone photoreceptor terminals. This was confirmed by GABA_C receptorimmunolabeling of mouse and rat cone terminals. This distributionof GABA receptors would be consistent with cone photoreceptorsreceiving a GABA feedback at theirterminals.

GABA_A and GABA_C receptors in cones

In the outer retina of nonmammalian vertebrates, the functional role of GABA feedback is still a matter of controversy (Werblin,1991; Piccolino, 1995; Kamermans and Spekreijse, 1999). Classically,horizontal cells are considered to release GABA by a carrier-mediatedmechanism (Schwartz, 1982, 1987; Yazulla and Kleinschmidt, 1983),the cone photoreceptors responding to transmitter at GABA_A receptorsas been demonstrated in turtle cones (Kaneko and Tachibana, 1986).This feedback could mediate the complex surround response in conephotoreceptors and thus contribute to enhancing contrast at theborder of objects (Piccolino, 1995). However, producing the surroundresponse has also been attributed to Ca²⁺ channel modulation, the GABA feedback would then adjust conephotoreceptor light sensitivity and responsiveness (Kamermansand Spekreijse, 1999).

In the mammalian retina, recording of GABA_A and GABA_C receptors in cultured porcine cone photoreceptors suggested the existenceof a GABA feedback to cone photoreceptors (Picaud et al., 1998).The presence of GABA_A receptors in mammalian cones was supportedby immunocytochemical staining of cat retina (Hughes et al., 1991).In the case of GABA_C receptors, their expression in mammaliancones was not consistent with previous in situ hybridization studies(Enz et al., 1996; Ogurusu et al., 1997) but could explain theimmunostaining observed in the outer plexiform layer that wasattributed to bipolar cells (Enz et al., 1995; Koulen et al.,1998). Our immunolabeling of rat retinal sections is in agreementwith GABA_C receptor localization in the cone terminals. Becausethe labeling was not restricted to cone terminals, the receptormight also be expressed in bipolar cell dendrites as previouslyproposed.

The picrotoxin sensitivity of cone GABA_C receptor currents indicates these receptors may not contain $rho$ 2 subunits that arepicrotoxin-insensitive and can confer this picrotoxin resistanceto the heteromeric channels in the mouse retina (Greka et al.,1998). The presence of MAP1B that specifically interacts withthe $rho$ 1 subunits (Hanley et al., 1999) suggests that $rho$ 1 subunitsare also present in cone GABA_C receptors. These reported interactionsdoes not necessarily mean, however, that MAP1B presence is requiredand sufficient for $rho$ 1 subunit expression. The glycine transporterGLYT-1 was indeed found to similarly interact with $rho$ 1 subunits(Hanley et al., 2000), although it does not colocalize with GABA_Creceptors in the retina (Pow and Hendrickson, 1999). The 20% pentobarbital-elicitedincrease in the GABA_C receptor current may indicate that $rho$ 1 subunitscan form heteromeric channels with GABA_A receptor subunits, asreported by Qian and Ripps (1999). These results suggest that $rho$ 1 subunits and not $rho$ 2 subunits are included in the compositionof cone GABA_Creceptors.

The localization of GABA receptors in mammalian cone photoreceptors in situ is consistent with the notion that mammalian conephotoreceptors receive a GABA feedback. In contrast to nonmammalianvertebrate animals (Kaneko and Tachibana, 1986), this GABA feedbackto cones may not be solely mediated by GABA_A receptors but byboth GABA_A and GABA_C receptors. This combination of receptorscould extend the range of sensitivity and allow differential modulation(Bormann, 2000). Furthermore, nondesensitizing GABA_C receptorsmight be more adapted to process the graded signals generatedin the outer retina. The sign of this feedback signal that dependson the equilibrium potential for Cl (E_Cl) and its origin are still unclear. GABA could indeed bereleased by either horizontal cells that can be immunolabeledfor GABA and glutamic acid decarboxylase (GAD) (Nishimura et al.,1985) or by interplexiform cells that can also be immunolabeledwith GABA (Ryan and Hendrickson, 1987) or can take up radioactiveGABA (Nakamura et al., 1980). Further studies will address thisquestion on the respective functional contribution of GABA_A andGABA_C receptors to cone lightresponses.

Protein MAP1B and GABA_C receptors

Protein MAP1B mutant homozygous mice were found to die in utero, whereas the heterozygous mice survived but with major lossin visual acuity caused by eye malformation. Histological examinationof the retina revealed a disorganization of the inner and outernuclear layers with a loss of demarcation at the external plexiformlayer (Edelmann et al., 1996). Such an alteration of the outernuclear and plexiform layers is consistent with our localizationof MAP1B in photoreceptors and especially at cone terminals inthe outer plexiformlayer.

MAP1B is found in embryonic nervous tissue within developing axonal processes (Schoenfeld et al., 1989) where phosphorylatedMAP1B seems to play an important role in neurite elongation byinterfering with microtubule extension (Goold et al., 1999). Inthe adult tissue, although its expression normally regresses,it was recently proposed to link the $rho$ 1 subunits of GABA_C receptorsto the cytoskeleton, as exemplified on rat retinal bipolar cells(Hanley et al., 1999). In the present study we localized MAP1Bto cone photoreceptor terminals by double staining with a cone-specificlectin. The recording of GABA_C receptors in cones and the immunolocalizationof the receptors to cone terminals are in agreement with the notionthat MAP1B links GABA_C receptors to the cytoskeleton. This propertywould provide another fundamental distinction from GABA_A receptorsthat were found to be linked to the cytoskeleton via gephyrin(Kneussel et al., 1999) or GABARAP (Wang et al., 1999).

Protein MAP1B was not restricted to cone terminals but was also detected in photoreceptor cell bodies and outer segments (Figs.8, 10). Cone cell bodies were similarly labeled with the $rho$ subunitantibody in the porcine retina (Picaud et al., 1998) but not inthe rat retina (Fig. 8F; Enz et al., 1996). This expression ofMAP1B in photoreceptors is consistent with its isolation by acloning strategy from a photoreceptor cDNA bank (D. Farber, personalcommunication). In rods, it seems unlikely that MAP1B links GABA_Creceptors because these receptors were not recorded from thesecells, either in cultured porcine photoreceptors (Picaud et al.,1998) or in flat-mounted rd mouse retinas (Fig. 2D). Because MAP1Bplays a major role in neurite elongation at embryonic stages (Gooldet al., 1999), it may also contribute to the continuous elongationof photoreceptor outer segments in the adult. Interestingly, MAP1Bwas also found in another ciliated sensory neuron, the hair cell(Jaeger et al., 1994). In these cells, the protein was found atthe base of stereocilia in the cuticularplate.

In all species studied so far, GABA_C receptors have been found in bipolar cell axon terminals. It is therefore unlikely thatthey are not present in porcine bipolar cells, which appears incontradiction to the weak MAP1B immunolabeling in porcine innerplexiform layer (Fig. 10). MAP1B was however reported to only linkto $rho$ 1 subunits, but not to other $rho$ subunits, which can also formhomomeric channels (Cutting et al., 1991; Wang et al., 1994; Zhanget al., 1995; Shingai et al., 1996; Greka et al., 1998). The absenceof MAP1B staining in pig bipolar cells may therefore reveal anabsence of $rho$ 1 subunits in pig bipolar cells. Otherwise, GABA_Creceptors were reported to contribute a minor component of GABAresponses in cone bipolar cells by contrast to rod bipolar cells(Euler and Wässle, 1998). Because pig vision is more cone-dominatedthan that of rats, this difference between rod and cone bipolarcells may partly explain the different MAP1B staining in the innerplexiform layer (Hanley et al., 1999). Moreover, porcine rod bipolarcells stained with protein kinase C antibody exhibit very fineaxon terminals (data not shown), highly contrasting with largebuttons of rat rod bipolar cells (Karschin and Wässle, 1990).Therefore, rod bipolar cell terminals may still be MAP1B-immunopositivein the inner plexiform layer, but their different morphology andlower density may explain the faint MAP1B immunostaining observedin the inner plexiform layer of the pigretina.

Conclusion

The preparation developed in this study should enable us to characterize further the pharmacology of mammalian photoreceptors.The demonstration of GABA_A and GABA_C receptors in mammalian conephotoreceptors already provides some new insight into the physiologicaland pathological functions of the cone pathway. It provides strongevidence that cone photoreceptors receive a GABA feedback in themammalian retina. Analysis of GABA_C receptor knock-out mice (Zhenget al., 1999) should help understand further the contributionof these receptors to cone physiology and, more generally, totheir function in neuronal transmission. Our finding of thesereceptors in another retinal neuron suggest that these nondesensitizingreceptors might be particularly adapted to process graded potentialneurotransmission.

  FOOTNOTES

Received May 19, 2000; revised June 30, 2000; accepted July 6, 2000.

This work was supported by Institut National de la Santé et de la Recherche Médicale, Retina France, Association pour leDeveloppement de la Recherche sur la régénération de la rEtineet sa Transplantation (ADRET-Alsace), Fédération des Aveuglesde France, Ministère de l'Education Nationale et de la Recherche,and Institut de Recherches Internationales Servier. B.P. receiveda fellowship from Retina France. We thank Anne Feltz, David Copenhagen,Alvaro Rendon, and David Hicks for critically reading this manuscriptand Valérie Forster for expert technical assistance. The $rho$ subunitantibody was kindly provided by Ralf Enz and Heinz Wässle.
Correspondence should be addressed to Serge Picaud, Institut National de la Santé et de la Recherche Médicale EMI 99-18,Médicale A, BP426, 1 Place de l'Hôpital, 67091 Strasbourg Cedex,France. E-mail: picaud{at}neurochem.u-strasbg.fr.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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