Regulation of the On Bipolar Cell mGluR6 Pathway by Ca2+

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The Journal of Neuroscience, June 15, 2000, 20(12):4471-4479

Regulation of the On Bipolar Cell mGluR6 Pathway by Ca²⁺
Scott Nawy
Departments of Ophthalmology and Visual Science and of Neuroscience, Albert Einstein College of Medicine, Bronx, New York 10461

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Glutamate produces a hyperpolarizing synaptic potential in On bipolar cells by binding to the metabotropic glutamate receptormGluR6, leading to closure of a cation channel. Here it is demonstratedthat this cation channel is regulated by intracellular Ca²⁺. Glutamate-evoked currents were recorded from On bipolar cellsin light-adapted salamander retinal slices in the presence of2 mM external Ca²⁺. When glutamate was applied almost continuously, interruptedonly briefly to measure the size of the response, the glutamateresponse remained robust. However, currents elicited by intermittentand brief applications of glutamate exhibited time-dependent rundown. Run down of the glutamate response was also voltage dependent,because it was accelerated by membrane hyperpolarization. Rundown was triggered, at least in part, by a rise in intracellularCa²⁺; measured as a function of time or voltage, it was attenuatedby intracellular buffering of Ca²⁺ with BAPTA or by omitting Ca²⁺ from the bathing solution. Current-voltage measurements demonstratedthat Ca²⁺ induced run down of the glutamate response by downregulatingcation channel function, rather than by preventing closure ofthe channel by glutamate and mGluR6. A major source of the Ca²⁺ that mediated this inhibition is the cation channel itself, whichwas found to be permeable to Ca²⁺, accounting for the use dependence of the run down. These resultssuggest that Ca²⁺ influx through the cation channel during background illuminationcould provide a signal to close the cation channel and repolarizethe membrane toward its dark potential, an adaptive mechanismfor coping with changes in ambientlight.

Key words: calcium; mGluR6; cation channel; metabotropic; retina; bipolar cell

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The synapse between photoreceptors and On bipolar cells is one of the initial synapses in the visual system and is the firstopportunity for modification of the visual signal. At this synapse,glutamate, the photoreceptor transmitter, hyperpolarizes On bipolarcells via activation of a G-protein-coupled receptor (Nawy andJahr, 1990a; Shiells and Falk, 1990), identified molecularly asmGluR6 (Nakajima et al., 1993). Hyperpolarization results whenthe G-protein-mGluR6 complex suppresses a cation current thatkeeps the On bipolar cells continuously depolarized. The mGluR6receptor is selectively activated by the glutamate agonist L-2-amino-4-phosphonobutyrateand is therefore characterized as a group III metabotropic receptor(for review, see Pin and Duvoisin, 1995). The G-protein, mostlikely G_o (Vardi, 1998; Nawy, 1999a), may inhibit channel functionvia a direct interaction with the channel, a common pathway forG_o (Hille, 1994) .

The photoreceptor-On bipolar cell synapse has long been recognized as a potentially important site for a photoreceptor-independentform of light adaptation within the retina (Dowling, 1987), althoughthe underlying cellular mechanism has not been resolved. New insightinto this problem was provided by a recent study showing thattightly buffering intracellular Ca²⁺ with BAPTA reduces adaptive changes in the light response ofOn bipolar cells (Shiells and Falk, 1999). The authors concludedthat Ca²⁺ may mediate adaptive changes to the light response in On bipolarcells, as it does in photoreceptors. Their study raises a numberof important questions. For example, the target of Ca²⁺ within the mGluR6 pathway is unclear. Ca²⁺ could be interacting with the receptor or G-protein, diminishingthe ability of the receptor to close the channel, or it may downregulatethe channel directly. Also, the source of the Ca²⁺ that mediated these adaptive changes is unclear. It has beensuggested that it may be the synaptic cation channel itself (Shiellsand Falk, 1999), but there is currently no evidence that the channelis permeable to Ca²⁺. In addition, information about the kinetics of Ca²⁺ action is lacking. Resolution of these issues is necessary toprovide a clearer understanding of Ca²⁺-dependent modulation of postsynaptic responses in On bipolarcells.

Accordingly, the present study was undertaken to assess the role of Ca²⁺ in the function and regulation of the mGluR6 pathway. The resultspresented here suggest that the nonselective cation channel thatis closed by glutamate is highly permeable to Ca²⁺ and that the entry of Ca²⁺ through this channel will then cause the channel to close. Thisfeedback can be observed within a second after the opening ofthe cation channel. Ca²⁺ could provide a signal to close cation channels that have beenopened by steady illumination. This process would help to restorethe On bipolar cell to its dark membrane potential and operatingrange.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Preparation of slices and solutions. Slices of retina from larval tiger salamanders (Kons Scientific, Germantown, WI) wereprepared as described previously (Nawy and Jahr, 1990b; Walterset al., 1998). Briefly, salamanders were anesthetized with 3-aminobenzoicacid ethyl ester and decapitated, and the eyes were enucleated.Whole retinas were isolated and placed on a 0.65 µm celluloseacetate/nitrate membrane filter (Millipore, Bedford, MA) thatwas secured with vacuum grease to a glass slide adjacent to therecording chamber. Slices were then cut to a thickness of 150-200µm with a tissue slicer (Stoelting, Wood Lane, IL), transferredto the recording chamber while remaining submerged, and viewedwith a Zeiss (Thornwood, NY) Axioskop equipped with a water-immersion40× objective with Hoffman modulation contrast (Modulation Contrast,Greenvale, NY). All manipulations were performed in normal roomlight. Slices were bathed in a solution containing (in mM): 108NaCl, 2 CaCl₂, 2.5 KCl, 1.2 MgCl₂, 10 HEPES, 10 glucose, and 0.1picrotoxin, pH 7.6 (with NaOH). Total Na⁺ was 110 mM. The solution was perfused continuously through therecording chamber at a rate of ~1 ml/min. In some experiments,the metabotropic receptor antagonist (R,S)- $alpha$ -cyclopropyl-4-phosphonophenylglycine(CPPG; Tocris Cookson, Ballwin, MO) was added to the control flowpipe solution. For the Ca²⁺-free solution, CaCl₂ was replaced with 2 mM EGTA. The 20 mM Ca²⁺ solution contained 85 mM Na⁺. For reversal potential experiments, MgCl₂ was omitted. Thesesolutions were applied to cells through the flow pipes (see below).The pipette solution was composed of (in mM): 85 K⁺gluconate, 10 KCl, 10 HEPES, 10 EGTA, 4 MgATP, and 1 LiGTP, pH7.4 (with KOH). Final [K⁺] was 144 mM.

Electrophysiology and drug application. Patch pipettes were fabricated from borosilicate glass (WPI, Sarasota, Fl) using atwo-stage vertical puller (Narishige, Sea Cliff, NY) and werefire-polished to resistances of 2-3 M $Omega$ . Whole-cell recordingswere obtained with an Axopatch 200A amplifier (Axon Instruments,Foster City, CA) and had input and series resistances of ~1 G $Omega$ and 10-19 M $Omega$ , respectively. On bipolar cells were identified bytheir position in the slice and by their characteristic outwardresponses to glutamate. Cells were discarded if the series resistanceexceeded 20 M $Omega$ , if the holding current changed suddenly, or ifthe holding current during the first application of agonist exceeded $-$ 20 pA (i.e., current measured while the sustained inward currentwas suppressed) at $-$ 40 mV. Holding potentials were corrected forthe liquid junction potential, which was measured to be 10 mVwith the standard K⁺gluconate pipette solution. Data were acquired with Axobasic softwareand the Digidata 1200 interface (Axon instruments) and analyzedwith Kaleidagraph (Synergy Software, Reading,PA).

Drugs were applied via two polymer-coated fused silica tubes (outer diameter, 350 µm; inner diameter, 250 µm; Polymicro Technologies,Phoenix, AZ) positioned close to the cell. One tube containedcontrol bathing solution, and the other contained bathing solutionto which 1 mM glutamate was added. The tubes were mounted to acomputer-controlled piezobimorph (Morgan-Matroc, Bedford, OH).Each tube was supplied by two separate reservoirs, which weremanually switched. One reservoir contained low Ca²⁺, either 0 or 2 mM Ca²⁺, and the other contained higher Ca²⁺ concentrations, either 5 or 20 mM Ca²⁺. The other set of reservoirs contained the same solutions, butwith added glutamate. I-V plots were constructed first in low-Ca²⁺ and then in high-Ca²⁺ solutions without repositioning the tubes. Switching from lowto high Ca²⁺ took ~15 sec. The bath solution always contained the standard2 mM Ca²⁺solution.

Measurement of reversal potentials. Direct measurement of the reversal potential of the glutamate response was often hamperedby a pronounced outward rectification of the I-V relation, particularlywith elevated Ca²⁺. The reversal potential was therefore obtained from the linearleast squares fit to the outward limb of individual I-V plots.Reversal potentials were pooled from all cells to obtain a meanand SE for each Ca²⁺ concentration. Analysis of reversal potential shifts in singlecells yielded results that were nearly identical to the shiftsobtained by pooling the data. The permeability ratio Ca²⁺/Na⁺ was obtained from experimentally determined reversal potentialsusing the Goldman-Hodgkin-Katz (GHK) constant field equation extendedto include divalent ions using ion activities (Jan and Jan, 1976;Mayer and Westbrook, 1987). Ion activity was calculated as theproduct of the ion concentration and activity coefficient $gamma$ . Activitycoefficients used to calculate ion activities were $gamma$ Na⁺ = 0.74, $gamma$ K⁺ = 0.72, and $gamma$ Ca²⁺(2 mM) = 0.23 [references cited in Gilbertson et al. (1991)] and $gamma$ Ca²⁺(20 mM) = 0.44 (Taschenberger et al., 1999).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Use-dependent regulation of the mGluR6 cascade

Whole-cell recordings were obtained from On bipolar cells in slices of tiger salamander retina that were light-adapted byroom light. Under light-adapted conditions, synaptic release ofglutamate from photoreceptors should be minimal. This was confirmedwith CPPG, a type III metabotropic receptor antagonist (Jane etal., 1996; von Gersdorff et al., 1997). Application of 300 µMCPPG to On bipolar cells produced no response (data not shown),indicating a lack of endogenous glutamate. At 30 sec intervalsafter obtaining recordings, cells were exposed to glutamate for5 sec, to monitor the amplitude of the response. This will bereferred to as the 20/120 protocol. Figure 1A shows three currenttraces in a cell that was voltage clamped at $-$ 40 mV. Each traceis composed of the average of four glutamate responses, obtainedduring the time period indicated above each trace. The responseappears outward because glutamate activates the metabotropic receptormGluR6 and shuts off an inward cation conductance (Nawy and Jahr,1990a; Shiells and Falk, 1990). There was a time-dependent rundown of the response associated with a decrease in baseline current,as has been reported previously (Nawy and Jahr, 1990b). Overall,the amplitude of the response decreased to 35.3 ± 6.5% of itsinitial size after 15 min of recording (Fig. 1C).

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Figure 1. Run down of the glutamate response is use dependent. A, Example of responses obtained when glutamate was applied for 5 sec at 30 sec intervals (20/120 application protocol). Each trace is the average of four responses obtained during the time intervals indicated above each trace. B, Example of responses from a different cell obtained by washing off glutamate for 5 sec at 2 min intervals (115/120 protocol). Each trace is a single response to the application of the control bathing solution at the time indicated above each trace. The bathing solution contained the group III metabotropic receptor antagonist CPPG (300 µM). Note that even when CPPG was present, the kinetics of wash off was slowed with successive trials. The reason for this is unclear but may be attributable to increased extrusion of glutamate by glia after long periods of glutamate application. Without CPPG present, the kinetics of washout was extremely slow and variable from cell to cell. C, The mean (±SE) responses to glutamate, normalized to the size of the initial response in each individual cell receiving nearly continuous (115/120 sec; filled squares; n = 11) or brief intermittent (20/120 sec; open circles; n = 7) exposure to glutamate. The holding potential for all cells was $-$ 40 mV.

In darkness, photoreceptors release glutamate continuously at their maximum rate onto On bipolar cells. Consequently, a largefraction of the mGluR6 receptors are bound, and the cation conductanceis primarily suppressed. These conditions were mimicked in thepresent study by continuously applying glutamate during establishmentof whole-cell recording. Thereafter, it was washed away once every2 min for 5 sec to measure the size of the response. Thus glutamatewas present for 115 of 120 sec (115/120). Figure 1B shows a seriesof three responses to the wash off of glutamate at different timesduring the recording. The responses are inward because the removalof glutamate activated the cation conductance. Although therewas a small change in the kinetics of the response to glutamateremoval (see Fig. 1B legend), the amplitude of the response wasessentially unchanged throughout the recording period. Overall,cells exposed nearly continuously to glutamate exhibited no significantchange in response amplitude (103.6 ± 11.8% of the initial response)over a 20 min recording period (Fig. 1C).

To examine better the mechanism and kinetics of response run down after glutamate deprivation, I first measured responsesto glutamate in cells using the 115/120 protocol. Response rundown was then initiated by switching to the low-glutamate, 20/120protocol. An example of the result is shown in Figure 2A. In thiscell, which had the largest response of all of the cells thatwere observed, the decay of the glutamate response (Fig. 2A, filledcircles) could be resolved as the sum of two exponentials, withtime constants of 53.9 sec and 7.7 min. However, in six othercells, only a single exponential was required to obtain an adequatefit of the averaged data (Fig. 2A, inset), with a time constantof 1.4 min. In several experiments, the order of application protocolswas reversed. Continuous application of glutamate for as longas 30 min failed to reverse run down that was induced by the 20/120protocol (n = 4 cells; data not shown). Thus, with conventionalwhole-cell recording, the run down of the glutamate response wasessentially irreversible.

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Figure 2. Use-dependent run down is associated with a loss of the underlying cation conductance. A, Plot of the decay of the response to glutamate (filled squares) and the suppressible cation current (open squares) in the same cell exposed to both glutamate application protocols. Because there is no known selective blocker of the cation channel, an independent measure of the total cation current was not possible. Instead, the amount of current was estimated by assuming that glutamate suppressed all of the cation current immediately before switching to the 20/120 protocol, when the response reached a maximum. The continuous line is a double exponential fit to the response data. Inset, Averaged decay of the response after switching to the 20/120 protocol. Data are from six cells and were reasonably well fitted by a single exponential. Norm. resp., Normalized response. B, Single responses to the withdrawal (left) or application (center, right) of glutamate at the times indicated by the numbers 1-3 in A. The decay of the response is caused solely by a loss of holding current. C, Left, Currents elicited by ramping the holding voltage from $-$ 80 to +30 mV. The duration of each ramp was ~8 sec. Voltage ramps were obtained immediately before, and then 10 min after, switching to the 20/120 protocols. Right, Ramp subtraction showing that the change in holding current during the experiment can be attributed to the loss of a conductance with a reversible potential near 0 mV. Records shown in C are from a different cell than that producing records in A and B.

Loss of the response could be because of the failure of the receptor $---$ G-protein complex to close the open cation channel orbecause cation channels are no longer open and available to beclosed by glutamate. In Figure 2A, total cation current is plottedas a function of time (open squares) along with the glutamateresponse. Total cation current was estimated by assuming thatduring the largest response that was observed, glutamate suppressedall of the cation current (i.e., the total cation current wasset equal to the size of the glutamate response at the time pointlabeled 1 in Fig. 2A). The striking similarity in the magnitudeand rate of decay of the response and the loss of current thatcould be suppressed by glutamate is consistent with the idea thatthe cation channel was downregulated with time, thus accountingfor the run down of the response. This can be appreciated by comparingthe peak and baseline of the response during glutamate removal(Fig. 2b, left) with the peak and baseline of the trace obtainedimmediately (middle) and 10 min (right) after switching protocols.The holding current in the presence of glutamate, when the cationchannels were closed, was essentially unchanged during the courseof the experiment. Similar results were obtained in six of sevencells.

Further evidence that a loss of the cation current was responsible for the overall change in holding current was obtainedby using voltage ramps to measure the cell I-V relation duringthe 115/120 phase of the experiment (glutamate was not appliedduring the ramp) and then again after switching to the 20/120protocol. In three of three cells, one of which is shown in Figure2C, the change in baseline was associated with a decrease in conductance(left) with a reversal potential near 0 mV (right), as expectedif the conductance decrease was caused by the closure of a nonselectivecationchannel.

Use-dependent regulation of the channel involves Ca²⁺

Ca²⁺ has been postulated as a mediator of adaptive changes in On bipolar cell light responses (Shiells and Falk, 1999). To testthe possibility that Ca²⁺ is involved in mediating the use-dependent effect of glutamatedescribed here, experiments were performed with BAPTA as the Ca²⁺ chelator rather than EGTA. The mean amplitude of the responseelicited by the 115/120 protocols in cells dialyzed with BAPTAwas essentially unchanged during the same time period (Fig. 3C;98.5 ± 19.9% of the initial response), similar to the result obtainedwith EGTA-dialyzed cells using the same glutamate applicationprotocol. However, dialysis with 10 mM BAPTA decreased time-dependentrun down of the response observed with the 20/120 applicationprotocol. An example of the glutamate responses obtained withBAPTA in the pipette and 2 mM Ca²⁺ in the bathing solution is shown in Figure 3A. Overall, the amplitudeof the response was 79.2 ± 10.4% of the initial response after15 min of recording (Fig. 3C).

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Figure 3. BAPTA reduces use-dependent run down. A, Currents elicited by glutamate with the 20/120 protocol, recorded from an On bipolar cell with a pipet solution containing 10 mM BAPTA. Responses exhibited only moderate run down. B, C, Time course of the response to glutamate in BAPTA-dialyzed cells, using the 20/120 application protocol (B; n = 9) or the 115/120 protocol (C; n = 8). With BAPTA, the time course of the response with both protocols was similar, suggesting that intracellular Ca²⁺ mediates use-dependent run down.

Although BAPTA effectively diminished time-dependent run down, a significant amount of run down was still observed. BAPTAmay not have reached the dendrites in time to prevent the initiationof a Ca²⁺-dependent process, leading to run down. Alternatively, one ormore sites of Ca²⁺ action may not be accessible to BAPTA. Accordingly, glutamateresponses were measured in a bathing solution containing no addedCa²⁺ and 2 mM EGTA. In this experiment, 2 mM Ca²⁺ was present in the bath to facilitate seal formation and break-in.Immediately after breaking into the cell, the bath solution wasswitched to a Ca²⁺-free solution, and the response to glutamate was measured usingthe 20/120 protocol. After a delay of several minutes, a run-upof the glutamate response was typically observed, and the amplitudeof the response was 139.2 ± 28.7% of the initial response (Fig.4A). Although there was a large degree of variability from cellto cell, as can be appreciated by the SE, run down was seen inonly one of six cells, and in that one cell, the size of the responseafter 15 min was ~90% of the initial response.

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Figure 4. Run down is prevented by removing Ca²⁺ from the bathing medium but not by blocking voltage-gated Ca²⁺ channels. A, A summary of the run down of the glutamate response, obtained with the 20/120 protocol, is shown. Cells were bathed in solution containing 2 mM EGTA and no added Ca²⁺ (filled circles; n = 6) or 2 mM Ca²⁺ and 100 µM nifedipine (open circles; n = 5). B, This concentration of nifedipine was sufficient to block Ca²⁺ currents in On bipolar cells fully. A Ca²⁺ current was elicited with a voltage ramp from $-$ 60 to +30 mV lasting ~2 sec. The addition of 100 µM nifedipine through a flow pipe blocked the current. Nifedipine also blocked Ca²⁺ current in two other cells. For this experiment, Ca²⁺ was replaced with 10 mM Ba²⁺ in the bathing solution. Nifed, Nifedipine.

The possibility that the entry of Ca²⁺ through voltage-gated Ca²⁺ channels might contribute to inhibition of the glutamate responsewas examined. Addition of 100 µM nifedipine to the normal bathingmedium did not prevent run down of the glutamate response (Fig.4A) but did block voltage-gated Ca²⁺ current in On bipolar cells (Fig. 4B), as has been reported previously(Tachibana et al., 1993; Protti and Llano, 1998). It thereforeseems likely that Ca²⁺ entry through nifedipine-sensitive Ca²⁺ channels, the prominent type of voltage-gated Ca²⁺ channel in On bipolar cells, does not contribute to regulationof the mGluR6pathway.

Ca²⁺ causes a run down of the glutamate response principally via downregulation of the cation channel. Figure 5 illustratesan experiment in which the bathing medium was switched from Ca²⁺-free to a solution containing 2 mM Ca²⁺. During this time, glutamate was applied briefly every 30 sec.The addition of Ca²⁺ produced a small transient change in the peak of the glutamateresponse. This was commonly observed, and the reason is unclear,but the long-lasting effect of added Ca²⁺ was a shift in the baseline (Fig. 5B). Voltage ramps made inthe absence and presence of Ca²⁺ (Fig. 5C, left) clearly show that the decrease in holding currentwas associated with a conductance decrease with a reversal potentialnear 0 mV. On the other hand, voltage ramps generated during glutamateapplication show that membrane conductance was relatively unchangedby Ca²⁺ when the cation channels were held closed by glutamate. Similarresults were obtained in seven other On bipolar cells. These resultssuggest that the use-dependent inhibition described in the previoussection shares a common mechanism with Ca²⁺, both downregulating function of the cation channel.

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Figure 5. Ca²⁺ induces run down via downregulation of the cation conductance. A, At the indicated time, control and glutamate bathing solutions with 2 mM EGTA and no added Ca²⁺ were switched with solutions containing 2 mM Ca²⁺. Ca²⁺ shifted the baseline and reduced the amplitude of the response. There was a 15 sec period during which there was no acquisition before each response to glutamate. B, Glutamate responses indicated by the boxes in A are displayed on a faster time scale. Note the undershoot after removal of glutamate in the 2 mM bathing solution, although the acquisition sequence ended before the response recovered to baseline. The holding potential for this cell was $-$ 40 mV. C, Responses to voltage ramps from $-$ 80 to +30 mV and ~8 sec long, obtained in 0 mM Ca²⁺ (thin line) and 2 mM Ca²⁺ (thick line) solution in the absence (left) and presence (right) of glutamate, are shown. In the presence of glutamate, when the cation channels were closed, Ca²⁺ had no effect on the I-V relation. In the absence of glutamate, Ca²⁺ decreased membrane conductance with a reversal potential near 0 mV, suggesting that the decrease in conductance was caused by an overall downregulation of cation channel function. The cell in C is different from the cell in A and B.

The cation channel that couples to the mGluR6 receptor is permeable to Ca²⁺

One potential route for Ca²⁺ entry that is consistent with the data presented above is through the cation channel itself. Becausethere is presently no evidence that the channel is permeable toCa²⁺, this possibility was examined by measuring the reversal potentialof the glutamate response while varying the external Ca²⁺ concentration. An example of this experiment is illustrated inFigure 6. In the absence of Ca²⁺, the response reversed near 0 mV (Fig. 6A). However, when a portionof the external Na⁺ was substituted with 20 mM Ca²⁺ (see Materials and Methods), the reversal potential was shiftedin the positive direction (Fig. 6B).

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Figure 6. Cation-selective channels in On bipolar cells are permeable to Ca²⁺. A, B, Records from an On bipolar cell obtained in 0 mM Ca²⁺ (A) and 20 mM Ca²⁺ (B). Raising external Ca²⁺ produces a positive shift in the reversal potential of the glutamate response. C, Mean (±SE) of the outward limb of the I-V relation measured with 0 mM Ca²⁺ (n = 9), 5 mM Ca²⁺ (n = 14), or 20 mM Ca²⁺ (n = 13) in the bath. D, Mean reversal potential as a function of external Ca²⁺. Fit is from the extended GHK equation (Mayer and Westbrook, 1987) with a Ca²⁺/K⁺/Na⁺ ratio of 4.9:1.27:1.

The mean reversal potential measured in Ca²⁺-free solution was $-$ 0.24 ± 0.74 mV, corresponding to a Na⁺/K⁺ permeability ratio near unity (1.27:1). In 5 mM Ca²⁺, the reversal potential was +2.7 ± 1.7 mV. In the presence ofhigher external Ca²⁺, the glutamate response rectified strongly near the reversalpotential, making direct measurements of the reversal potentialdifficult. For this reason, the reversal potential was determinedby a linear extrapolation of the outer limb of the I-V relation,as illustrated in Figure 6C. In 20 mM Ca²⁺, the reversal potential was +10.1 ± 1.9 mV. In Figure 6D thereversal potential of the glutamate response is plotted as a functionof Ca²⁺ concentration. The continuous line is the GHK equation with aCa²⁺/Na⁺/K⁺ ratio of 4.9:1.27:1, adjusted for the activities of Ca²⁺, K⁺, and Na⁺ (see Materials and Methods). Thus, the shift in the reversalpotential of the glutamate response suggests that the cation channelis significantly permeable to Ca²⁺.

Ca²⁺ confers voltage dependence on the glutamate response

Downregulation of the cation conductance by Ca²⁺ was strongly potentiated by membrane hyperpolarization. This is illustratedin the experiments summarized in Figure 7. Cells were held at $-$ 20 mV, and the holding potential was then stepped from +30 to $-$ 80 mV. In some experiments, cells were held at each potentialfor 5 sec before glutamate was applied (Fig. 7A, left). In otherexperiments, the step length before glutamate application wasincreased to 65 sec (Fig. 7A, right). The mean (± SE) amplitudeof the glutamate response after long and short voltage steps isplotted as a function of the step voltage in Figure 7B. The externalsolution always contained 2 mM Ca²⁺. With both step lengths, the slope conductance of the voltage-responseplot was similar over the range of $-$ 20 to +30 mV (short step,2.07 nS; long step, 1.79 nS). At holding potentials more negativethan $-$ 20 mV, the slope conductance declined dramatically. Withshort steps, the slope conductance was 0.68 nS, and with longersteps, it was 0.14 nS. The inhibition of the response at morenegative holding potentials was not readily reversible and resultedin a depression of the current suppressed by glutamate irrespectiveof holding potential (data not shown).

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Figure 7. Inhibition of the steady-state glutamate response by Ca²⁺ is potentiated by long hyperpolarizing steps. A, Three examples of glutamate-elicited currents during a series of 10 mV voltage steps from +30 to $-$ 80 mV. Left, Responses to glutamate, applied 5 sec after the beginning of each step (Short step). The early portion of the trace at +30 mV has been omitted because of contamination from voltage-gated K⁺ currents. Middle, Responses from another cell to glutamate applied 65 sec after the initiation of each step (Long step). Right, Same as the middle panel except that this cell was dialyzed with BAPTA. Voltage protocols are shown above each series of responses. For clarity, only responses during odd voltage steps are shown. Calibration: left, right, 100 pA; middle, 50 pA. B, Mean (± SE) of the I-V plot obtained with short steps (open circles; n = 15), long steps (open squares; n = 17), and long steps in cells dialyzed with BAPTA (filled squares; n = 11). Slope conductances for each condition were obtained from the linear regression of the averaged data over the voltage ranges of +30 to $-$ 20 and $-$ 30 to $-$ 80 mV. For short steps, slope conductances were 2.07 and 0.68 nS, respectively (dashed lines). For long steps, the slope conductances were 1.79 and 0.14 nS, respectively (continuous lines). For long steps with BAPTA in the pipette solution, the slope conductances were 1.51 and 0.79 nS, respectively.

These data are consistent with the idea that hyperpolarization increases the driving force for Ca²⁺ through the cation channel and hastens run down of the response.Support for this idea was obtained by measuring the I-V relationusing the long-step protocol and including BAPTA in the pipettesolution (Fig. 7A, right). The slope conductance from $-$ 80 to $-$ 20mV was 0.79 nS, similar to the conductance obtained with the shortstep with EGTA in the pipette solution (Fig. 7B). This experimentindicates that the rectification of the I-V relation is attributableto enhancement of Ca²⁺ inhibition at negative potentials. However, substantial rectificationof the I-V relation was still observed in cells dialyzed withBAPTA. It is not clear whether this rectification persists becauseBAPTA is simply overwhelmed by the local increase in Ca²⁺ or whether Ca²⁺ acts at other targets that are not accessible to BAPTA, suchas the channel pore (seeDiscussion).

Many cells, particularly early in the recording, displayed a prominent undershoot after the removal of glutamate, which decayedback to baseline over the course of several seconds. An exampleof this undershoot in a cell recorded with 5 mM Ca²⁺ in the bathing solution is shown in Figure 8A (thick trace).Glutamate would be expected to close nearly all of the cationchannels. Thus would eliminate Ca²⁺ influx and favor upregulation of the cation channel. Accordingto this model, upregulation is revealed briefly after the removalof glutamate, until the cation current decays to a smaller steady-statevalue as a result of Ca²⁺ influx. In support of this idea, switching to a Ca²⁺-free bathing solution almost completely abolished the undershootand increased the steady-state amplitude of the glutamate response(Fig. 8A, thin trace). In six of six cells that displayed a prominentundershoot, the undershoot was eliminated by switching to Ca²⁺-free solution. In the cell illustrated in Figure 8A, the timeconstant of decay was 0.84 sec, the fastest decay observed. Insix cells, all of which could be fitted with a single exponential,the average time constant was 3.2 ± 1.4 sec.

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Figure 8. Ca²⁺-induced changes in response kinetics contribute to inhibition of the response during hyperpolarization. A, Each trace is the average of four responses obtained in a bathing solution with 0 mM Ca²⁺ (thin trace) or 5 mM Ca²⁺ (thick trace). Ca²⁺ depressed the steady-state cation current, but in this cell the depression was relieved briefly after the wash off of glutamate. Inset, The Ca²⁺-dependent decay of cation current was exponential, with a time constant of ~0.8 sec in this cell. Calibration: 20 pA, 1 sec. B, I-V relations of the glutamate response using brief voltage steps as described in Figure 7 are shown. Steady-state responses were measured in 0 mM Ca²⁺ (filled circles; n = 10) or 5 mM Ca²⁺ (open circles; n = 9). The slope conductance for 0 mM Ca²⁺ was 2.06 nS. In a third group of cells, the "peak" response was measured in cells that displayed a significant undershoot (open squares; n = 11), by summing the size of the undershoot and the steady-state response. This group was obtained by pooling cells that were recorded with 5 mM Ca²⁺ (7 cells) and 2 mM Ca²⁺ (4 cells). The 0 mM Ca²⁺ group includes only cells that displayed a significant undershoot with Ca²⁺ in the bathing medium.

Perhaps because of the increased driving force for Ca²⁺ through the channel, the size of the undershoot was enhanced relativeto the steady-state glutamate response at negative holding potentials.Current-voltage relations for the glutamate response in bathingsolution containing 5 or 0 mM Ca²⁺ are shown in Figure 8B. The responses were generated using theshort-step protocol as in Figure 7A. In 5 mM Ca²⁺, the steady-state response rectified sharply. Between $-$ 20 and+30 mV, the slope conductance was 1.48 nS, and it was 0.49 nSbetween $-$ 30 and $-$ 80 mV. In 0 mM Ca²⁺, the relation was relatively linear over the entire voltage range,with an overall slope conductance of 2.10 nS. When the instantaneousamplitude of the glutamate response in Ca²⁺ (data for 2 and 5 mM Ca²⁺ were pooled) was measured by incorporating the undershoot, Ca²⁺-dependent inhibition was minimized, and the response-voltagefunction more closely resembled the 0 mM Ca²⁺function.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Synaptic responses in the dendrites of On bipolar cells are generated by current flow through a nonselective cation channel.The channel is negatively regulated by the mGluR6-G_o-protein complex,which is localized to the dendrites (Vardi et al., 1993; Nakanishi,1994; Nomura et al., 1994; Vardi and Morigiwa, 1997; Vardi, 1998).As a result, the cation channel is closed in darkness, when glutamatelevels in the synapse are high, and opens when light hyperpolarizesthe presynaptic photoreceptor and decreases transmitter release.In this study I show that this cation channel is regulated ina use-dependent manner. When the channels were held close by continuousapplication of glutamate, a large fraction of them opened in responseto brief periods of glutamate removal. However, when the channelswere allowed to remain open, the cation current quickly ran down.Run down was triggered, at least in part, by a rise in intracellularCa²⁺, because it was attenuated by buffering Ca²⁺ with BAPTA or removing Ca²⁺ from the bathing solution. A potential source of Ca²⁺ entry is the cation channel itself, which was shown to have significantCa²⁺permeability.

At physiological concentrations, external Ca²⁺ appears to inhibit On bipolar cell cation channel function primarily by bindingto an intracellular site rather than via channel block, such ashas been observed for other cation channels. The effect of Ca²⁺ described here is much slower than can be accounted for by divalentopen channel block (Haynes et al., 1986; Zimmerman and Baylor,1986; Mayer and Westbrook, 1987; Jahr and Stevens, 1993; Zagottaand Siegelbaum, 1996). Furthermore, inhibition of channel functioncould be primarily prevented by buffering intracellular Ca²⁺ with BAPTA. Downregulation of the cation current by Ca²⁺ probably also accounts for the pronounced voltage dependenceof the glutamate response described here. During long hyperpolarizingsteps (in the absence of glutamate), a greater accumulation ofCa²⁺ within the dendrites might be expected, because of a larger drivingforce for Ca²⁺ (Vernino et al., 1992), and this would promote further downregulationof the channel. Significant downregulation during hyperpolarizingsteps as brief as 5 sec could be observed, and one such examplecan be seen in the $-$ 80 mV record in Figure 7A. I-V relations withlong voltage steps were relatively linear when cells were bufferedwith BAPTA. Furthermore, instantaneous measurements of the I-Vrelation for the channel made in previous studies, constructedeither with very brief steps or with ramps, do not exhibit pronouncedrectification (Nawy and Jahr, 1991; Thoreson and Miller, 1993;Tian and Slaughter, 1994; Thoreson et al., 1995; Nawy, 1999a).

Higher concentrations of Ca²⁺, such as those used to measure permeability of the cation channel to Ca²⁺, inhibited the cation channel at all voltages that were examined.Inhibition of the cation conductance with high external Ca²⁺ might result from channel block, because BAPTA was unable toproduce any relief from this inhibition. Alternatively, high externalCa²⁺ might overwhelm BAPTA and raise intracellular Ca²⁺ near its intracellular target (Legendre et al., 1993).

Several previous studies have sought to identify a role for Ca²⁺ in regulation of the mGluR6 cascade and have yielded conflictingresults. An early study of rod On bipolar cells isolated fromrat retina showed that removal of extracellular Ca²⁺ increased the magnitude of the cation current, whereas raisingCa²⁺ from 2.5 to 25 mM decreased the current (Yamashita and Wassle,1991). Similar results were obtained in a study of amphibian retinain a slice preparation (Thoreson and Miller, 1993). The conclusionsof these studies are in agreement with the results presented here.One difference is that these previous studies attributed the effectsof Ca²⁺ to a direct block of the cation channel, whereas it is proposedhere that at least a portion of the actions of Ca²⁺ can be attributed to an intracellular site of action (see below).Another laboratory has reported no significant change in the cationcurrent or response to agonist after removal of extracellularCa²⁺ (Shiells and Falk, 1992). One explanation for their result isthat they held the voltage of their cells at $-$ 20 mV, significantlyless negative than the holding potentials in the other studies.At $-$ 20 mV, the driving force for Ca²⁺ is small, and only minor effects of Ca²⁺ on the cation current and, hence, the glutamate response areobserved (see Figs. 7, 8 of this study). In fact, close inspectionof Figure 3A of the study by Shiells and Falk (1992) indicatesa slight potentiation of the cation current in the absence ofexternal Ca²⁺.

The findings of the present study would seem to contradict a previous study from this laboratory that concluded that CaMKII,a kinase that is activated by a rise in intracellular Ca²⁺, upregulates the cation channel (Walters et al., 1998). In thatstudy, but not in the present one, bipolar cells were dialyzedwith pipette solutions containing high concentrations of inorganicphosphate, because it increases the size of the glutamate response.Inorganic phosphate is an inhibitor of phosphatases (Jones andWestbrook, 1997) and probably serves this function in On bipolarcells, because a similar potentiation of the glutamate responsehas been observed when the Ca²⁺-dependent phosphatase calcineurin is inhibited (Nawy, 1999b).Calcineurin is activated by 10- to 100-fold lower Ca²⁺/calmodulin concentrations than is CaMKII (Klee, 1991), Therefore,one explanation for our results is that when the cation channelsare open, recordings with EGTA and no added Ca²⁺ in the pipette allow the intracellular Ca²⁺ concentration near the cation channel to rise sufficiently toactivate calcineurin but not CaMKII. Inhibition of calcineurinwould unmask CaMKII that was activated before initiation of therecording, when intracellular Ca²⁺ may have been higher, or CaMKII that was weakly activated atlow Ca²⁺ concentrations during the recording. There is abundant evidencethat the balance between Ca²⁺-dependent phosphorylation and dephosphorylation at a single sitecan be regulated by Ca²⁺ concentration and preferential activation of CaMKII or calcineurin[see references in Wang and Kelly (1996, 1997)]. It is unclearwhether Ca²⁺ levels in On bipolar cell dendrites become sufficiently highto activate CaMKII near the cation channel. If so, this wouldconstitute a positive feedback pathway, in which the entry ofCa²⁺ through the channel might lead to further upregulation of thecationchannel.

The run down of cation current induced by Ca²⁺ was essentially irreversible. As discussed above, this may be caused by an imbalanceof phosphatase and kinase activities that regulate the channel.Because calcineurin is bound to the plasma membrane (for review,see Yakel, 1997), its activity may be retained during prolongedwhole-cell recording, while the conjugate kinase(s) may be dialyzedfrom the cell. Consistent with this view is the observation thatearly in the recording, usually within the first 2-3 min, Ca²⁺-induced inhibition of the cation current could be reversed (S.Nawy, unpublishedresults).

The results of this study provide evidence of a Ca²⁺-triggered negative-feedback pathway, activated when glutamate levels inthe synapse fall during steady illumination and the fraction ofopen channels increases. Ca²⁺ entering through cation channels would close them, helping torestore the membrane potential and input resistance of On bipolarcells to their preillumination values. This would insure thatthe input resistance of the cell remained high, preventing shuntingof currents evoked by the opening of a few number of channels(Shiells and Falk, 1994). The kinetics of downregulation, estimatedfrom the decay of the cation current after the removal of glutamate,yielded time constants of 1-6 sec, which would allow for relativelyrapid recovery from adapting backgrounds. A recent study of Onbipolar cells of the dark-adapted dogfish retina demonstratedthat BAPTA prevents desensitization to dim light backgrounds,providing support for this model (Shiells and Falk, 1999). Regulationof the mGluR6 pathway by Ca²⁺ would provide the retina with an adaptive mechanism for copingwith changes in ambient light in addition to adaptation withinphotoreceptors.

  FOOTNOTES

Received July 20, 1999; revised March 31, 2000; accepted April 7, 2000.

This work was supported by National Institutes of Health Grant EY 10254 and by an unrestricted grant from Research to PreventBlindnessInc.
Correspondence should be addressed to Dr. Scott Nawy, Kennedy Center Room 525, 1410 Pelham Parkway South, Bronx, NY 10461.E-mail: Nawy{at}aecom.yu.edu.

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DISCUSSION
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