Expression of the Voltage-Gated Chloride Channel ClC-2 in Rod Bipolar Cells of the Rat Retina

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The Journal of Neuroscience, November 15, 1999, 19(22):9841-9847

Expression of the Voltage-Gated Chloride Channel ClC-2 in Rod Bipolar Cells of the Rat Retina
Ralf Enz², Brenda J. Ross¹, and Garry R. Cutting¹
¹ Institute of Genetic Medicine and Department of Pediatrics, The Johns Hopkins University School of Medicine, Baltimore, Maryland 21287, and ² Institut für Biochemie, Friedrich-Alexander-Universität Erlargen-Nürnberg, 91054 Erlangen, Germany

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Voltage-gated chloride channels (ClC) are highly conserved during evolution and appear to participate in a variety of physiologicalfunctions. Recently, ClC-2 was proposed to play a role in stabilizingthe chloride equilibrium potential near or below the resting membranepotential in neurons expressing ligand-gated chloride channels.Because rod bipolar cells in mammalian retina express three formsof inhibitory ligand-gated chloride channels, we decided to studyClC-2 localization and function in the rat retina. RNA encodingClC-1, -2, -3, -4, and -5 was detected by reverse transcription-PCRin the rat retina. ClC-2-specific antibodies identified proteinon cell bodies and in synaptic layers. Double-immunofluorescencestaining revealed that intense ClC-2 immunoreactivity colocalizedwith PKC-stained rod bipolar cells. Patch-clamp experiments performedwith individual rod bipolar cells demonstrated the presence ofa time-dependent, inwardly rectified current activated at hyperpolarizingmembrane potentials. This current demonstrated selectivity fordifferent anions (Cl > I > gluconate), was inhibited by Cd²⁺, and was minimally reduced by 4,4'-diisothiocyanatostilbene-2,2'-disulphonicacid. These features are consistent with currents generated byClC-2 channels. Our data indicate that functional ClC-2 channelsare present in retinal rod bipolar cells and support a role forClC-2 in maintaining Cl homeostasis in neurons with ligand-gated chloridechannels.

Key words: voltage-gated chloride channel; ClC; ligand-gated ion channel; GABA receptor; CNS; retina; rod bipolar cell

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The voltage-gated chloride channel (ClC) family in mammals consists of nine different proteins, most of which are of unknownfunction (Jentsch and Günther, 1997). The third member of thisfamily, ClC-2, is ubiquitously expressed and is associated witha time-dependent, inwardly rectified chloride conductance activatedby cell swelling, extracellular acid pH, or membrane hyperpolarization(Gründer et al., 1992; Thiemann et al., 1992; Staley et al.,1996; Jordt and Jentsch, 1997; Schwiebert et al., 1998). Despitethe wide distribution of ClC-2, it has been suggested that ClC-2channels in neurons act in concert with chloride transportersto facilitate neurotransmitter-mediated inhibition (Smith et al.,1995; Staley et al., 1996).

In most mature neurons, outward-directed chloride transporters, such as the potassium-chloride cotransporter or the sodiumlinked chloride-bicarbonate exchanger, drive the chloride equilibriumpotential (E_Cl) negative relative to the cell resting membranepotential (E_m) (Thompson and Gähwiler, 1989b; Staley et al.,1996; Jentsch and Günther, 1997; Jarolimek et al., 1999; Riveraet al., 1999). Under this situation, opening of GABA- or glycine-gatedchloride channels results in hyperpolarization of the neuron.However, prolonged stimulation of inhibitory receptors can reducethe degree of hyperpolarization and can even lead to depolarizationbecause of intracellular chloride accumulation (McCarren and Alger,1985; Thompson and Gähwiler, 1989a,b; Staley et al., 1995). Furthermore,certain neurons are depolarized by activation of GABA receptors,and it has been shown that E_Cl is positive relative to E_m in thesecells (Misgeld et al., 1986; Rohrbough and Spitzer, 1996).

Two observations indicate that ClC-2 channels underlie a noninactivating inwardly rectifying chloride conductance that preventsE_Cl from becoming positive relative to E_m in cells hyperpolarizedby inhibitory neurotransmitters (Staley, 1994; Staley et al.,1996). First, pyramidal neurons that are hyperpolarized by GABAexpressed ClC-2 channels, whereas dorsal root ganglion (DRG) neuronsthat are depolarized by GABA lacked ClC-2 expression (Misgeldet al., 1986; Thompson and Gähwiler, 1989b; Staley, 1994; Smithet al., 1995; Rohrbough and Spitzer, 1996). Second, expressionof ClC-2 in DRG neurons using an adenoviral vector reduced E_Clto levels close to E_m and attenuated GABA-mediated depolarization(Staley et al., 1996).

Anatomic, electrophysiological, and molecular studies indicate that activation of GABA_A, GABA_C, or glycine receptors causeshyperpolarization of retinal bipolar cells (GABA_A receptors: Karschinand Wässle, 1990; Grigorenko and Yeh, 1994; Greferath et al.,1995; GABA_C receptors: Feigenspan et al., 1993; Enz et al., 1995;Enz et al., 1996; Euler and Wässle, 1998; Fletcher et al., 1998;glycine receptors: Karschin and Wässle, 1990; Enz and Bormann,1994; Greferath et al., 1994). However, the expression patternof voltage-gated chloride channels in the retina is unknown. Asa first step to explore the possible role of ClC channels in visualsignal transduction, we analyzed retinal mRNA for members of theClC family. Subsequently, the expression of ClC-2 was studiedin detail, using ClC-2-specific antibodies in combination withcolocalization techniques. Patch-clamp experiments were performedon dissociated retinal neurons to verify the results of the immunocytochemicalstudies. We conclude that rod bipolar cells express functionalClC-2 chloridechannels.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

cDNA synthesis and PCR. Five micrograms of rat retina poly(A⁺) RNA (Clontech, Palo Alto, CA) were incubated for 30 min at 37°Cwith 50 U of DNaseI (Boehringer Mannheim, Mannheim, Germany) and40 U of RNasin (Boehringer Mannheim) in a final volume of 100µl to remove possible contamination from chromosomal DNA. To removethe enzyme, acid phenol extraction and ethanol precipitation wasperformed by adding 16 µl of 2 M sodium acetate, pH 4.0, 100 µlof acid phenol, and 50 µl of chloroform/isoamylalcohol (49:1)following the protocol of Chomczynski and Sacchi (1987). All chemicalswere purchased from Sigma (St. Louis, MO). cDNA synthesis wasperformed in 40 µl of cDNA synthesis buffer, containing 50 mMTris-HCl, pH 8.3, 3 mM MgCl₂, 75 mM KCl, 10 mM dithiothreitol,and 0.5 mM each dNTP, 250 ng of p(dN)₆, 40 U of RNasin (BoehringerMannheim), and 800 U of SuperscriptII RNaseH reverse transcriptase (Life Technologies, Grand Island, NY).Incubation times were 15 min at room temperature followed by 2hr at 42°C. For PCR, oligonucleotides specific for seven membersof the rat ClC family were used (Table 1). Amplification wasperformed with 100 ng of reverse-transcribed RNA in 50 µl of PCRbuffer [20 mM Tris-HCl, pH 8.0, 50 mM KCl, 1.5 mM MgCl₂, 0.2 mMdNTPs, 0.2 µM each primer, and 5 U of Taq-polymerase (Life Technologies)]using a programmable thermocycler (Perkin-Elmer Cetus, Norwalk,CT) with the following parameters: 94°C for 3 min followed by30 cycles at 94°C for 45 sec, 58°C for 60 sec, 72°C for 45 sec,and a final incubation at 72°C for 10 min. To detect splice variantsof ClC-2, annealing was performed at 55°C. Ten microliters ofeach PCR product were separated on a 1.5% agarose gel and stainedwith ethidium bromide. Controls were treated as described above,except adding reverse transcriptase. To verify the identity ofthe DNA fragments, PCR solutions were purified using Microcon-100spin columns (Amicon, Beverly, MA) or geleluted (Qiagen, Hilden,Germany) and subjected to dideoxy sequencing (Sanger, 1977).


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Table 1. Oligonucleotides used for the detection of members of the ClC family

Immunohistochemistry. After intramuscular injection of ketamine (87 mg/kg; Sigma) and xylazine (13 mg/kg; Sigma), the deeplyanesthetized adult Wistar rats were euthanized via transcardiacpuncture and exsanguination. The eyes were enucleated, and thelens, cornea, and vitreous body were removed. Eyecups were fixedfor 1 hr in 4% paraformaldehyde, cryoprotected in 30% sucrose,embedded in O.C.T. compound (Sakura Finetek, Torrance, CA), andfrozen in isopentane chilled with dry ice. Subsequently, 12 µmcryosections were collected on siliconized slides. Immunostainingwas performed using the indirect fluorescence method with ratanti ClC-2 (1:100) (Staley et al., 1996) and mouse anti-PKC (1:50;Amersham Pharmacia Biotech, Arlington Heights, IL) as primaryantibodies and goat anti-rat conjugated to Cy3 (1:1000; Sigma)and goat anti-mouse conjugated to FITC (1:50; Sigma) as secondaryantibodies. For double-label experiments, sections were firstincubated in a mixture of primary antibodies, followed by a mixtureof secondary antibodies. Controls were prepared by using onlysecondary antibodies or by omitting one of the two primary antibodies.In this case, only immunoreactivity of the remaining primary antibodywas detected. Immunofluorescence was accomplished using an epifluorescencemicroscope (Axiophot; Zeiss, Jena, Germany) equipped with a 40× 1.3 fluorite objective, a filter wheel (Sutter, Novato, CA),a cooled coupling device (CCD camera CH350; Photometrics, Tucson,AZ), and Metamorph software (Universal Imaging Corp., West Chester,PA). Horizontal sections were analyzed using a confocal laser-scanningmicroscope (LSM 410; Zeiss) and Zeiss LSM software (version 3.80).Images were reproduced with Adobe Photoshop (Adobe Systems, SanJose, CA) and a color printer (NP-1600M; Codonics, MiddleburgHeights,OH).

Cell preparation and electrophysiological recordings. Retinas of adult Wistar rats (8 weeks) were dissociated using a combinationof enzymatic and mechanical procedures as described previously(Huba and Hofmann, 1988; Karschin and Wässle, 1990). One hourafter plating on glass coverslips coated with poly-L-lysine (Sigma)and concanavalin A (Sigma), bipolar cells were visually identifiedunder phase-contrast optics of an inverted microscope (Nikon,Melville, NY) with a CF plan flour 20× objective. Cells were continuouslysuperfused with an extracellular bath solution at a rate of 1ml/min containing (in mM): 137 NaCl, 5.4 KCl, 1.8 CaCl₂, 1 MgCl₂,and 5 HEPES, pH 7.4. NaCl was replaced by NaI and sodium gluconatein anion selectivity experiments. Patch pipettes were made fromborosilicate glass (Warner Instruments, Hamden, CT) using a two-stageelectrode puller (Narashige, East Meadow, NY) and had pipetteresistances of 3.7-5.2 M $Omega$ (mean of 4.3 M $Omega$ ; n = 5) when filledwith an intracellular solution containing (in mM): 120 CsCl, 20TEA-Cl, 1 CaCl₂, 2 MgCl₂, 11 EGTA, and 10 HEPES, pH 7.2. Electrodeholder and head stage were mounted on a piezo-electric remote-controlleddevice attached to a three-dimensional mechanical micromanipulator(Burleigh Instruments, Fishers, NY). Membrane currents were recordedin the whole-cell configuration of the patch-clamp method (Hamillet al., 1981) using an Axopatch amplifier (Axon Instruments, FosterCity, CA) and PCLAMP 6.0 software (Axon Instruments). Currentswere low-pass filtered at 2 kHz (four-pole Bessel filter) andsampled with 20 Hz. The recorded data were corrected for errorsresulting from series resistance, estimated to be in the rangeof 15 M $Omega$ (two to five times the pipette resistance) (Marty andNeher, 1995) and from liquid junction potential, calculated tobe + 3.37 mV for NaCl, $-$ 2.42 mV for NaI, and $-$ 7.31 mV for sodiumgluconate (Barry, 1994). Leak subtraction was not applied, becausethe data presented in this paper are qualitative in nature. CdSO₄,4,4'-diisothiocyanatostilbene-2,2'-disulphonic acid (DIDS), NaI,and sodium gluconate (all from Sigma) were applied in the bathsolution with the U-tube application system (Bormann, 1992). Togenerate current-voltage plots, amplitude values measured at 200msec were normalized to 1 for each cell and plotted against theapplied voltage. Error bars represent ±SEM. A modified versionof the Goldman-Hodgin-Katz equation was used to calculate permeationratios (p_Anion/p_Chloride= (e^(Erev * ^F/RT) $-$ ([Chloride]_o/[Chloride]_i))/([Anion]_o/[Chloride]_i).

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Expression of voltage-gated chloride channels in the rat retina

The presence of mRNA transcripts encoding seven members of the ClC family in the adult rat retina was studied using reversetranscription (RT)-PCR. Single strand cDNA obtained after reversetranscription of retinal mRNA was amplified with oligonucleotidesspecific for the seven ClC genes (Table 1). DNA fragments wereamplified from ClC-1,-2,-3,-4, and -5 mRNA transcripts but notfrom ClC-K1 or ClC-K2 (Fig. 1A). Alternative splicing of ClC-2in rat brain has been reported. Skipping of exon 20 produced mRNAtranscripts that were 60 nucleotides shorter (Chu et al., 1996;Chu and Zeitlin, 1997). DNA fragments of the expected size forthe exon 20 splice variant were amplified from rat retina (Fig.1B). For all PCR experiments, control reactions without addingreverse transcriptase excluded contamination.

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Figure 1. Expression of RNA encoding voltage-gated chloride channels in the rat retina. Ethidium bromide stained RT-PCR products amplified from rat retina RNA using primers specific for seven different ClC genes (A) and primers flanking exon 20 of the rat ClC-2 gene (B). The identity of all PCR products was determined by DNA sequencing. A, The ClC type is indicated above the agarose gel, and the 600 bp fragment of a 100 bp ladder (lane M) is shown on the left. The faintly stained fragments in lane K2 and lane 5 are attributable to nonspecific amplification. B, The exon 20 splice variant of rat ClC-2 was detected in retinal RNA (+ lane). The expected sizes of fragments amplified from ClC-2 transcripts with exon 20 (202 bp) and without exon 20 (142 bp) are indicated on the right. The fragment without an indicated size is because of formation of a heteroduplex of the two smaller DNA fragments. Absence of amplified product in the reaction without reverse transcriptase ( $-$ lane) excluded contamination.

Immunohistochemical localization of ClC-2 in rod bipolar cells

A polyclonal immunoserum raised in rabbit that specifically recognizes ClC-2 (Staley et al., 1996) was applied to verticalcryostat sections of the adult rat retina. Immunoreactivity couldbe detected in all retinal layers (Fig. 2A). Cell bodies in theouter nuclear layer (ONL) were faintly labeled, whereas cell bodiespresent in the inner nuclear layer (INL) and ganglion cell layer(GCL) were intensely stained. Within the INL, ClC-2 immunoreactivitywas visible as bright regions in cell bodies lying at the outerhalf of the INL, presumably being bipolar cell bodies. In addition,fluorescence could be detected in both the outer plexiform layer(OPL) and the inner plexiform layer (IPL). The strong stainingof photoreceptor inner segments was nonspecific, because it wasalso visible in sections that were incubated without primary antibodies(Fig. 2B). To indicate the position of retinal layers, a Nomarskiphotograph is shown in Figure 2C.

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Figure 2. Immunohistochemical detection of ClC-2 in the rat retina. A, A fluorescence micrograph of a vertical cryostat section through the rat retina was incubated with antibodies specific for ClC-2 and visualized using secondary antibodies coupled to Cy3. Immunofluorescence could be seen throughout the retina, most prominent at cell bodies present in the outer half of the INL and in the IPL. Scale bar, 25 µm. B, Control experiment in which only the secondary antisera was used. Nonspecific staining of photoreceptor inner segments can be seen. C, Retinal layers are shown using Nomarski optics. IS, Inner segments of photoreceptors; ONL, outer nuclear layer; OPL, outer plexiform layer; INL, inner nuclear layer; IPL, inner plexiform layer; GCL, ganglion cell layer.

To determine which type of neurons stained brightly in the outer half of the INL, we performed double-immunofluorescence experiments.Labeling for ClC-2 was visualized with secondary antibodies coupledto Cy3 (Fig. 3A, red fluorescence). Intense staining was visiblein the outer half of the INL, as well as throughout the IPL. Thesame section was also incubated with an antibody against the $alpha$ isoform of PKC, which is used to identify rod bipolar cells (Greferathet al., 1990). Binding of this antibody was visualized with secondaryantibodies coupled to FITC (Fig. 3B, green fluorescence). Rodbipolar cell bodies were seen in the outer half of the INL. Theirdendrites terminated in the OPL, and their axons proceeded verticallyto the lower border of the IPL in which they ended in a broadband of varicose swellings. Double exposure of this section superimposedthe red staining for ClC-2 in the upper half of the INL on nearlyevery green-labeled rod bipolar cell body. The resulting yellowsignals were visible as bright regions in the upper part of theINL and appeared to be within the rod bipolar cell bodies (Fig.3C). In addition, intense ClC-2 immunoreactivity was colocalizedwith the axon terminal systems of rod bipolar cells in the IPL(stars).

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Figure 3. Localization of ClC-2 on rod bipolar cells. A, Fluorescence micrographs of a vertical cryostat section labeled with a ClC-2-specific antiserum (Cy3-coupled secondary antisera, red fluorescence). B, Incubation of the same section as in A with antisera specific for the $alpha$ subunit of PKC, which identifies rod bipolar cells (FITC-coupled secondary antisera, green fluorescence). C, Double exposure of the section revealed staining for ClC-2 on the upper half of rod bipolar cell bodies (yellow fluorescence) and on rod bipolar cell axon terminal systems (stars). Scale bar, 25 µm.

Further studies were performed to determine the location of the ClC-2 immunoreactivity in the INL and the IPL. An enlargedvertical section of the outer half of the INL is shown in Figure4A. Every rod bipolar cell body (identified by green PKC immunoreactivity)was also labeled with the ClC-2 antiserum, seen as intense costaining(yellow). ClC-2 was also present on neurons other than rod bipolarcells (Fig. 4A, star). To evaluate whether the ClC-2 immunoreactivityon rod bipolar cell bodies was localized to the membrane or whetherthe protein was present in intracellular structures, a horizontalplane of a double-labeled rod bipolar cell body was visualizedby confocal laser-scanning microscopy (Fig. 4B). Superimposureof the PKC immunoreactivity (left, green fluorescence) with theClC-2 staining (middle, red fluorescence) suggested that ClC-2is localized in or near the cell membrane of rod bipolar cellbodies (right, yellow fluorescence). An enlarged view of the IPLis shown in Figure 4C. The left shows vertically oriented axonsof rod bipolar cells terminating in their terminal systems atthe lower border of the IPL (green fluorescence). The ClC-2 immunofluorescenceof the same section is shown in the right of Figure 4C (red fluorescence).Colocalization of rod bipolar cell axon terminals with ClC-2 stainingwas evident (stars). In summary, ClC-2 seems to be expressed ataxon-terminal systems of rod bipolar cells, thus being in thevicinity of GABA and glycine receptors. In addition, we foundClC-2 to be expressed in surprisingly high concentrations in rodbipolar cell bodies, most likely present in the membrane of theseneurons.

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Figure 4. Subcellular distribution of ClC-2 on rod bipolar cells. A, Enlarged view of a vertical cryostat section immunolabeled as in Figure 3. Cell bodies of rod bipolar cells were located in the outer half of the inner nuclear layer (green fluorescence). ClC-2 immunoreactivity (red fluorescence) was present on every cell body, resulting in yellow signals. In addition, ClC-2 staining outlined other cells (star). B, Horizontal single-section confocal fluorescence micrographs of a rod bipolar cell body double-immunolabeled as described in Figure 3. PKC immunoreactivity was predominantly localized to the cell membrane (left, green fluorescence). Expression of ClC-2 is shown in the middle (red fluorescence). The double exposure demonstrated that ClC-2 immunoreactivity seemed to be mostly present within or near the cell membrane (right, yellow). C, Enlarged view of the lower border of the IPL of double-labeled vertical cryostat sections. Axon terminal systems of rod bipolar cells were double-immunolabeled with antibodies recognizing PKC (left, green fluorescence). ClC-2 immunoreactivity (red fluorescence) was present at identical positions (stars). Furthermore, ClC-2 immunoreactivity was observed at other regions within the IPL. Scale bars: A, C, 10 µm; B, 5 µm.

Hyperpolarization-activated chloride currents in rod bipolar cells

To investigate whether functional ClC-2 chloride channels are present in cell membranes of rod bipolar cells, we performedwhole-cell patch-clamp studies on isolated rod bipolar cells.It has been shown previously that cells in retinal dissociatesthat have the appearance of bipolar cells (Fig. 3B) are rod bipolarcells, because they can be stained with an antibody against the $alpha$ subunit of PKC (Greferath et al., 1990; Karschin and Wässle,1990). Rod bipolar cells were visually identified under an invertedmicroscope, and voltage-activated currents were recorded usinga specific protocol: initial depolarization from 0 to +40 mV,than voltage steps in $-$ 20 mV increments to a potential of $-$ 140mV (Fig. 5, left). Maximal currents at $-$ 140 mV were between 1000and 3000 pA. A representative current tracing is shown in Figure5 (middle). At negative voltages, the chloride channel openedin a time-dependent manner over a 250 msec interval and showedinward rectification, characteristics typical of ClC-2 recordedin mammalian cells (Carew and Thorn, 1996; Ferroni et al., 1997;Park et al., 1998; Schwiebert et al., 1998). To compare current-voltagerelationships of different bipolar cells, current values for eachcell were normalized by dividing the current recorded at eachvoltage step by the current recorded at $-$ 140 mV. Normalized datafrom 12 different cells are shown in a current-voltage plot (Fig.5, right). Inward rectification of the observed chloride conductancewas observed at potentials negative to $-$ 60 mV.

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Figure 5. Hyperpolarization-activated chloride currents on isolated rod bipolar cells. A hyperpolarizing voltage step protocol (left) generated inwardly rectified, noninactivating currents from an isolated rod bipolar cell (middle). Data recorded from 12 different bipolar cells are summarized in a current-voltage plot (right). The current amplitudes have been normalized (I/I_c) to the currents at $-$ 140 mV (I_c; see Materials and Methods for details).

To characterize the nature of the observed currents, hyperpolarization-activated currents were recorded in bath solutionscontaining different anions. The relative anion selectivity forClC-2 has been shown to be Cl > I > gluconate (Thiemann et al., 1992; Ferroni et al., 1997; Jordtand Jentsch, 1997; Clark et al., 1998; Schwiebert et al., 1998).When 137 mM NaCl was substituted with sodium iodide or sodiumgluconate, the amplitudes of the recorded currents decreased inthe order Cl > I > gluconate at all potentials (Fig. 6A). Normalized data areshown in a current-voltage plot. Mean reductions at $-$ 100 mV were38.6 ± 10.7% (iodide) and 60.1 ± 3.3% (gluconate) and were statisticallysignificant (chloride-iodide, p = 3.5 × 10⁴; iodide-gluconate, p = 3.8 × 10²). The reversal potentials (E_rev) were +0.29 ± 0.4 mV for symmetricalchloride, +3.3 ± 0.25 mV, and + 16.6 ± 4.2 mV after substituting137 mM chloride with iodide or gluconate. From the mean values,permeation ratios relative to chloride were calculated for iodide(0.85) and for gluconate (0.47).

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Figure 6. Electrophysiological characterization of hyperpolarization-activated currents in rod bipolar cells. A, Representative current tracings of a single rod bipolar cell recorded in different anionic solutions. Current amplitudes and the degree of inward rectification decreased in NaI, further decreased in Na gluconate, and returned to original levels in NaCl. The current-voltage plot on the right represents calculated mean data. Currents were normalized (I/I_c) using current amplitudes at $-$ 120 mV in NaCl (I_c). The voltage protocol was the same as described in Figure 5, except that the applied potentials ranged from + 60 to $-$ 120 mV. B, Representative current tracings of a single rod bipolar cell exposed to extracellular DIDS or CdSO₄. The first and fourth recordings were performed in symmetrical chloride solutions alone. The voltage-activated currents were partially inhibited by the application of 500 µM DIDS and substantially reduced by 500 µM CdSO₄. Inhibition of each compound was reversible. The current-voltage plot of normalized mean data are shown at the right. Currents have been normalized as described in A.

To further characterize the hyperpolarization-activated currents in isolated bipolar cells, Cd²⁺ or DIDS were applied in the external solution. Cadmium has beenshown to be a potent reversible inhibitor of ClC-2-mediated chloridecurrents, whereas DIDS only minimally affects ClC-2 currents (Madisonet al., 1986; Chesnoy-Marchais and Fritsch, 1994; Fritsch andEdelmann, 1996; Ferroni et al., 1997; Clark et al., 1998; Schwiebertet al., 1998). Application of 500 µM Cd²⁺ reduced the voltage-activated current by 86.4 ± 2.7% at $-$ 120mV (Fig. 6B). In contrast, the application of 500 µM DIDS hada minor effect on the recorded current traces ( $-$ 26.3 ± 10.1% at $-$ 120 mV). Normalized data from five different cells are shownin a current-voltage plot. Thus, rod bipolar cells generated time-dependentinwardly rectifying currents at hyperpolarizing voltages thatshowed anion-selectivity (Cl > I > gluconate), sensitivity to Cd²⁺, and minimal inhibition byDIDS.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Very little is known of the expression pattern of voltage-gated chloride channels in the retina. Using RT-PCR, we detectedtranscripts for ClC-1,-2,-3,-4, and -5 in the adult rat retina.ClC-1 is considered to be muscle-specific; thus, our observationson the expression of ClC-1 outside muscle suggests a broader distributionof this channel than previously thought. Indeed, ClC-1 has alsobeen detected in hair cells of the rat cochlea (Kawasaki et al.,1999). Considering the potential importance of ClC-2 in inhibitoryneurotransmission, we decided to perform an extensive study onits cellular distribution in the retina. Incubation of verticalcryostat sections of retina with ClC-2-specific antibodies revealedthe presence of ClC-2 protein on the cell bodies of all nuclearlayers, as well as in both synaptic layers, consistent with thewide tissue distribution of ClC-2 (Thiemann et al., 1992). However,intense staining was consistently noted in the outer half of theINL that colocalized with PKC-stained rod bipolarcells.

Confocal microscopy revealed that the ClC-2 staining appeared to be in, or near, the cell membranes of rod bipolar cells.ClC-2 has been found in the proximity of cell membranes in airwayepithelia of the rat and human embryonic kidney cells (HEK 293)and in secretory granules at the apical pole of pig pancreaticcells (Murray et al., 1995; Carew and Thorn, 1996; Park et al.,1998). In the IPL of the rat retina, axon terminals of rod bipolarcells were intensely stained by the ClC-2 antibodies. Many subunitsof glycine and GABA receptors are present at the axon terminalsystems of these cells (Karschin and Wässle, 1990; Greferathet al., 1995; Enz et al., 1996). Therefore, ClC-2 seems to bepresent in a region of bipolar cells in which massive chlorideinflux is predicted to occur. However, we cannot rule out thepossibility that localization in the IPL is a result of expressionof ClC-2 on amacrine cells that form reciprocal synapses withbipolar cell terminals. This issue might be solved using electronmicroscopy.

Patch-clamp experiments were performed on single rod bipolar cells to corroborate the anatomical localization of ClC-2 tothese neurons. The isolated cells exhibited time-dependent inwardlyrectified currents that activated within milliseconds at hyperpolarizingmembrane potentials. The anion selectivity (Cl > I > gluconate) of these currents indicated that a chloride selectiveion channel was responsible for a substantial fraction of thecurrents. Furthermore, the observed reversal potential (E_rev)in symmetrical chloride (+0.3 mV) was close to the predicted E_revfor a chloride current under these conditions (0 mV). Substitutionof extracellular chloride with iodide or gluconate caused a shiftof E_rev to positive voltages as expected, but the magnitude ofthe shift was less than predicted by the Nernst equation. Themuted shift in reversal potential may be caused by inactivationof ClC-2 at depolarizing voltages, as reported previously (Jordtand Jentsch, 1997). This concept is supported by the observationthat ClC-2 channels activated by acidic pH remain open at positivevoltages and display more substantial shifts of E_rev in iodideand gluconate solutions (Jordt and Jentsch, 1997; Schwiebert etal., 1998).

The characteristics and anion selectivity of the chloride currents were consistent with those reported previously for ClC-2.Exchange of extracellular chloride with other anions reduced thecurrent amplitudes at negative and positive membrane potentials,indicating an effect that was independent of the direction ofion flow (Thiemann et al., 1992; Ferroni et al., 1997; Clark etal., 1998; Schwiebert et al., 1998). Furthermore, ClC-2 expressedin mammalian cells has been shown to activate in milliseconds,as observed in the rat bipolar cells (Carew and Thorn, 1996; Ferroniet al., 1997; Schwiebert et al., 1998). In contrast, mammalianforms of ClC-2 have considerably slower activation kinetics whenexpressed in Xenopus oocytes (Thiemann et al., 1992; Jordt andJentsch, 1997). To further characterize the observed chlorideconductance, we applied Cd²⁺ and DIDS, two compounds used to study ClC-2 in other cell systems(Ferroni et al., 1997; Clark et al., 1998; Schwiebert et al.,1998). Extracellular Cd²⁺ substantially reduced the voltage-activated chloride current,whereas DIDS had a minor effect, most likely because of its negativecharge, consistent with previous studies of ClC-2 (Ferroni etal., 1997; Clark et al., 1998; Schwiebert et al., 1998). Therefore,our electrophysiological studies appear consistent with ClC-2immunoreactivity in, or near, the cell membrane of rod bipolarcells (Fig. 4B) and support the idea that at least a fractionof ClC-2 protein is located within themembrane.

The hyperpolarization-activated currents we observed in the rod bipolar cells have characteristics similar to a potassiumconductance studied by Karschin and Wässle (1990). The authorsreported that addition of cesium in the patch pipette blockedthe potassium current completely. Although shape and activationcharacteristics of the potassium currents were similar to thetraces presented in this paper, it is unlikely that the conductancewe described was caused by potassium. First, all recordings wereperformed with 120 mM CsCl and 20 mM TEA-Cl in the patch-pipette;thus, potassium-mediated currents should be completely blocked.Second, all recordings were performed with symmetrical chlorideconcentrations without potassium inside the cell. Under theseconditions, a potassium current would reverse at a very positivevoltage. In contrast, the observed reversal potential of our currentswas close to 0 mV, consistent with the predicted reversal potentialof a chloride current under our recording conditions. We cannot,however, exclude the possibility that a minor portion of the voltage-activatedcurrent could be carried by an inwardly rectified potassium currentbecause of an incomplete block by Cs⁺ and TEA⁺, and/or by a Cd²⁺-sensitive nonselective cationconductance.

Among retinal neurons, only rod bipolar cells express three ligand-gated chloride channels (glycine, GABA_A, and GABA_C, receptors).It has been shown that GABA and glycine can be coreleased fromindividual synaptic vesicles in interneuron-motoneuron synapsesof the rat spinal cord, producing simultaneous activation of GABAand glycine receptors (Jonas et al., 1998). Although the samephenomenon has not been observed in the retina, simultaneous releaseof both neurotransmitters may occur at a single synapse usingdifferent vesicles. Thus, GABA and glycine receptors might beactivated simultaneously, which could result in a substantialchloride influx into rod bipolar cells. Reduction of the chloridegradient could lower the inhibitory effect of GABA and glycineon the bipolar cells (Adams and Brown, 1975; Barker and Ransom,1978; Segal and Barker, 1984).

Our results suggest that two mechanisms operate to maintain the chloride gradient and, in turn, the inhibitory effect of GABAand glycine on retinal bipolar cells. First, outward-directedchloride transporters, such as KCC2, could actively transportchloride out of cells to establish a strong inward driving forcefor chloride (Jarolimek et al., 1999; Rivera et al., 1999). Indeed,it has been shown that bipolar cells in primary cultures of thechick retina express the KCC2 isoform of the potassium-chloridecotransporter (Williams et al., 1999). Localization of functionalClC-2 channels to bipolar cells in this report suggests that asecond mechanism may operate in situations of substantial chlorideinflux. Based on the proposition that ClC-2 channels clamp E_Clat or near E_m in cortical neurons, it is possible that these channelsplay the same role in retinal neurons (Smith et al., 1995; Staleyet al., 1996). In this way, ClC-2 could act as a "safety" valvefor chloride ions. The characteristics of ClC-2, inwardly rectifiedchloride channels that open at hyperpolarizing membrane potentialswithout time-dependent inactivation would be well suited for thistask.

  FOOTNOTES

Received ; revised ;accepted.
This work was supported by the Deutsche Forschungsgemeinschaft (R.E.), the Reproductive Scientist Development Program throughNational Institutes of Health Grant 2K12HD00849 (B.J.R.), andNational Institutes of Health Grants EY 09531 and DK 48977 (G.R.C.).We thank Drs. R. Smith and K. Staley for the ClC-2 immunoserum,Dr. S. Chu for ClC-2 oligonucleotides, Dr. M. Milewski for helpwith the confocal microscope, and Drs. J. Wright, W. B. Guggino,and D. Dawson for helpfuldiscussions.

Correspondence should be addressed to Dr. Garry R. Cutting, Institute of Genetic Medicine, CMSC 9-123, The Johns Hopkins UniversitySchool of Medicine, 600 North Wolfe Street, Baltimore, MD 21287.E-mail: gcutting{at}jhmi.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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