Bitter Taste Transduction of Denatonium in the Mudpuppy Necturus maculosus

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Volume 17, Number 10, Issue of May 15, 1997 pp. 3580-3587
Copyright ©1997 Society for Neuroscience

Bitter Taste Transduction of Denatonium in the Mudpuppy Necturus maculosus

Tatsuya Ogura¹, Alan Mackay-Sim¹^,², and Sue C. Kinnamon¹
¹ Department of Anatomy and Neurobiology, Colorado State University, Fort Collins, Colorado 80523, and Rocky Mountain Taste and Smell Center, University of Colorado Health Sciences Center, Denver, Colorado 80262, and ² School of Biomolecular and Biomedical Science, Griffith University, Nathan, QLD 4111 Australia

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Bitter substances are a structurally diverse group of compounds that appear to act via several transduction mechanisms. Thebitter-tasting denatonium ion has been proposed to act via twodifferent G-protein-regulated pathways, one involving inositol1,4,5-trisphosphate and raised intracellular calcium levels, theother involving phosphodiesterase and membrane depolarizationvia a cyclic nucleotide-suppressible cation channel. The aim ofthe present study was to examine these transduction mechanismsin taste cells of the mudpuppy Necturus maculosus by calcium-imagingand whole-cell recording. Denatonium benzoate increased intracellularcalcium levels and induced an outward current independently ofextracellular calcium. The denatonium-induced increase in intracellularcalcium was inhibited by U73122, an inhibitor of phospholipaseC, and by thapsigargin, an inhibitor of calcium transport intointracellular stores. The denatonium-induced outward current wasblocked by GDP- $beta$ -S, a blocker of G-protein activation. Neitherresting nor denatonium-induced intracellular calcium levels wereaffected by inhibition of phosphodiesterase (with IBMX) or adenylatecyclase (with SQ22536) or by raising intracellular cyclic nucleotidesdirectly (with cell permeant analogs). Our results support thehypothesis that denatonium is transduced via a G-protein cascadeinvolving phospholipase C, inositol 1,4,5-trisphosphate, and raisedintracellular calcium levels. Our results do not support the hypothesisthat denatonium is transduced via phosphodiesterase and cAMP.
Key words: bitter taste transduction; mudpuppy; taste receptor cells; fura-2; calcium imaging; whole-cell recording

INTRODUCTION

There are a large number of compounds that taste bitter to humans (Belitz and Weiser, 1985). Given the structural diversityof these compounds, it is expected that there may be multipletransduction mechanisms or multiple receptor proteins in tastereceptor cells. Unexpected perhaps is evidence that the bitter-tastingdenatonium ion may operate via two separate transduction pathways.One hypothesis proposes that denatonium activates phospholipaseC (PLC), thus increasing intracellular levels of inositol 1,4,5-trisphosphate(IP₃) to release calcium ions from intracellular stores (Akabaset al., 1988; Hwang et al., 1990; Spielman et al., 1994b). Theincrease in intracellular calcium is proposed to lead to neurotransmitterrelease, thereby completing the transduction step (Akabas et al.,1988; Spielman et al., 1994b). Another hypothesis is that denatoniumactivates phosphodiesterase to decrease intracellular levels ofcyclic nucleotides (Ruiz-Avila et al., 1995; Wong et al., 1996),which would depolarize the cell by relieving the cyclic nucleotideblock of a membrane cation channel (Kolesnikov and Margolskee,1995). The influx of cations (including calcium) is proposed todepolarize the cell leading to neurotransmitter release.

These two hypotheses predict several conflicting properties of the responses induced by denatonium. First, although both hypothesespredict a denatonium-induced rise in intracellular calcium, theformer predicts that this is attributable to calcium release fromintracellular stores, whereas the latter predicts that it is attributableto calcium influx from the extracellular medium. Second, althoughthe former hypothesis makes no prediction about the effect ofdenatonium on the membrane potential, the latter hypothesis predictsthat denatonium should depolarize taste cells. Finally, each hypothesispredicts testable pathway-specific effects of pharmacologicalagents.

In the present report, bitter transduction was studied to test the predictions arising from these two hypotheses. Denatonium-inducedresponses were examined in taste cells of mudpuppy Necturus maculosus.Mudpuppies can detect denatonium, and it is aversive to them (Oguraet al., 1996). Mudpuppy taste receptor cells are large, easilyisolated, and amenable to study (Kinnamon et al., 1988a), andpreliminary experiments indicated that the majority were responsiveto denatonium. Denatonium-induced responses of these cells wereexamined using whole-cell patch-clamp recording and calcium imagingusing the Ca²⁺-sensitive dye fura-2.

MATERIALS AND METHODS
Isolation of taste receptor cells. Mudpuppies (Necturus maculosus) were obtained from commercial suppliers and kept in largeaquaria maintained at 10°C. They were fed live minnows weekly.Taste receptor cells were isolated from mudpuppies, as describedpreviously (Kinnamon et al., 1988a). Briefly, mudpuppies wereanesthetized by immersion in ice water and decapitated. The lingualepithelium was dissected from the underlying connective tissue.To distinguish mature taste cells from other cell types, theywere labeled at the apical membrane by incubating the epitheliumfor 15 min in fluorescein isothiocyanate-conjugated wheat germagglutinin [FITC-WGA, 0.5 mg/ml in amphibian physiological saline(APS)] (Kinnamon et al., 1988b). The epithelium was then incubatedin APS that contained collagenase (1 mg/ml, Worthington Biochemical,Freehold, NJ), albumin (1 mg/ml), and glucose (5 mM), until themucosal layers of the nongustatory epithelium could be gentlypeeled free from the underlying lamina propria, which left thetaste buds attached to their papillae. The remaining tissue wastreated with Ca²⁺-free APS to dissociate the taste buds. Isolated cells were platedin recording chambers made with coverslips (for calcium imaging)or slides (for whole-cell recording) coated with Cell-Tak (CollaborativeResearch, Bedford, MA).

Intracellular [Ca²⁺] measurement. Isolated cells in the chamber were loaded with the cell-permeable, Ca²⁺-sensitive, fluorescent dye fura-2 AM (5 µM, Molecular Probes,Eugene, OR) for 30 min, then washed with normal APS for 20 min.Images were acquired with an intensified CCD camera (IC100-ICCD,Paultek Imaging, Grass Valley, CA) through an oil-immersion objectivelens (Fluor 40×, 1.3 NA, Nikon) of an inverted microscope (DiaphotTMD, Nikon). The video signal from the camera was captured witha frame grabber board (Quick Capture, Data Translation) on anMacintosh computer (Quadra 800, Apple Computer). For dual-wavelengthratiometric Ca²⁺ measurements, pairs of fluorescent images were recorded at 350and 380 nm of excitation light using a filter wheel (EMPIX Imaging).Emitted light was collected by a 510-580 nm bandpass filter (ChromaTechnology). In our system, space resolution is ~3000 pixels/cell.Pseudocolor Ca²⁺ images (e.g., Fig. 1C) were generated as 20 level color imagesfrom ratios of 350 and 380 nm images using the public domain NationalInstitutes of Health (NIH) Image program (developed at NIH andavailable on the Internet at http://rsb.info.nih.gov/nih-image/).Intracellular Ca²⁺ concentration ([Ca²⁺]_i) in selected areas was calculated from the ratio of 350 and380 nm images (Grynkiewicz et al., 1985). Ca²⁺ calibration curves were obtained with calcium calibration kitII (C-3009, Molecular Probes). For plotting the time course of[Ca²⁺]_i (e.g., Fig. 2), we averaged the [Ca²⁺]_i over most of the cell area, avoiding the edges of the cell.With a recording chamber volume of ~200 µl, <10 sec was requiredto totally exchange solutions by superfusion.
Fig. 1. Denatonium increased intracellular calcium levels. A, Light image of an isolated taste cell. Scale bar, 20 µm. B, Fluorescenceimage of the same cell showing the apical tip of the taste celllabeled with FITC-WGA. The labeled region is shown in white inthis pseudocolor image. C, Calcium images of the same taste cellloaded with the Ca²⁺-sensitive dye fura-2. The pseudocolor scale of [Ca²⁺]_i is shown on the right. a, [Ca²⁺]_i before and b, immediately after application of 5 mM denatoniumbenzoate. The increase in [Ca²⁺]_i begins at the apical tip. c, [Ca²⁺]_i 30 sec after application of denatonium benzoate. [Ca²⁺]_i increases over entire cell. d, [Ca²⁺]_i after washing the cells for 2 min with APS. [Ca²⁺]_i returns to resting level. D, Typical time course of denatonium-inducedcalcium responses. Denatonium benzoate (5 mM) was applied duringthe periods labeled DN. Note that the denatonium-induced responsesare similar after repeated application of denatonium.
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Fig. 2. Time courses of changes in [Ca²⁺]_i. Measurements of [Ca²⁺]_i in individual cells using fura-2. Denatonium benzoate (5 mM) was appliedduring the periods labeled DN. A, The denatonium-induced calciumresponse was present in Ca²⁺-free extracellular solution. B, Thapsigargin (1 µM) abolishedthe denatonium-induced calcium response. C, The denatonium-inducedcalcium response was not affected by ryanodine (10 µM). D, Thedenatonium-induced calcium response was abolished by the PLC inhibitorU73122 (5 µM).
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Cells were bathed in normal APS until the resting intracellular calcium level was stable. The bath was then perfused withAPS containing denatonium benzoate (5 mM, Sigma, St. Louis, MO).This was followed by washing with normal APS until the intracellularcalcium again reached prestimulus levels. Cells were then perfusedwith other APS solutions including Ca²⁺-free APS, ryanodine (10 µM for 2-5 min or 200 µM for 10 min,Calbiochem, La Jolla, CA), thapsigargin (1 µM for 12-16 min, Sigma),U73122 (5 µM for 12-17 min, Calbiochem), isobutyl methoxyxanthine(IBMX, 100 or 200 µM for 1-3 min, Sigma), SQ22536 (2.5 mM for30-40 min, Calbiochem); dibutyryl-cAMP (db-cAMP, 5 mM for 1-3min, Sigma); dibutyryl-cGMP (db-cGMP, 5 mM for 1-3 min, Sigma),and a mixture of db-cGMP (2 mM for 1-3 min, Sigma) and 8-chlorophenylthio-cAMP(8-cpt-cAMP, 2 mM for 1-3 min, Sigma). Some cells were incubatedin pertussis toxin (PTX, 0.5 or 2 µg/ml in APS, Sigma) for >20hr at 4°C.

Cells were considered to respond to denatonium if it caused an increase in [Ca²⁺]_i, which was >2 SD values above the mean resting level of eachcell. The effects of drug treatments on the denatonium responsewere assessed using Student's t tests. Statistical values arepresented as mean [Ca²⁺]_i ± SEM.

Giga-seal whole-cell recording. Membrane currents were measured using giga-seal whole-cell recording (Hamill et al., 1981).Electrodes were fabricated from microhematocrit capillary tubes(American Scientific Products, McGaw Park, IL) pulled on a two-stagevertical puller (Narishige). When filled with intracellular saline,resistances ranged from 1.8 to 3.5 M $Omega$ . Cells were viewed at amagnification of 400×, using a Nikon Diaphot inverted microscopefitted with Hoffman optics. Seals of 1-10 G $Omega$ were obtained bygentle suction, and whole-cell recordings were achieved by deliveryof a short depolarizing pulse to the pipette. Whole-cell currentswere measured at room temperature using an Axopatch 1D patch-clampamplifier (Axon Instruments, Foster City, CA). Signals were prefilteredat 5 kHz (low-pass filter) and recorded digitally at 100 µsecintervals unless otherwise specified. Data were stored using alaboratory computer (11/23, Digital Equipment, Maynard, MA) equippedwith a Cheshire data interface and Basic 23 software (Indec Systems).The computer also generated all voltage commands. In some experiments,data were also stored on a Pentium computer (Applied ComputerTechnology), using Axoscope software (Axon Instruments). Unlessotherwise noted, leak and linear capacitative currents were subtractedfrom all records by computer. Series resistance, which was typically<10 M $Omega$ , was not compensated. Gravity-fed stimuli were bath-appliedto the 0.5 ml recording chamber. To prevent loss of the seal andto prevent perfusion artifacts during whole-cell recording, theperfusion rate was lowered to 2-3 ml/min. To ensure that datawere obtained from viable taste receptor cells, only cells exhibitingvoltage-gated Na⁺ currents and input resistances >0.5 G $Omega$ were selected for dataanalysis.

After whole-cell recording was obtained and membrane capacitance was electronically compensated, membrane currents were measuredin normal APS by stepping the cell membrane from $-$ 60 to 80 mVin 10 mV increments. The bath was then perfused with 1 mM denatoniumbenzoate, and membrane currents were again measured. Finally,the denatonium was washed out of the bath with normal APS andthe currents again measured. In some cells, the tip of the pipettewas filled with the normal pipette solution but backfilled witha solution containing 1 mM GDP- $beta$ -S (Sigma). In some experiments,1 µM tetrodotoxin (TTX, Sigma) was added to the bath to blockNa⁺ currents. There was no effect of TTX on the response to denatonium.

For comparison, control and denatonium-induced currents were measured at 35 msec after the membrane potential was steppedto +80 mV. Statistical values are presented as mean currents ±SEM.

Solutions. Normal APS contained (in mM): 112 NaCl, 2 KCl, 8 CaCl₂, 3 HEPES, buffered to pH 7.2 with NaOH. Ca²⁺-free APS contained either 1 mM BAPTA (for cell isolation) or1 mM EGTA (for calcium imaging). Patch pipette solution contained(in mM): 114 KCl, 2 NaCl, 0.09 CaCl₂, 2 MgCl₂, 1 BAPTA, 1 ATP,0.4 GTP, 10 HEPES, buffered to pH 7.2 with KOH.

RESULTS

Denatonium increased intracellular calcium levels
We measured [Ca²⁺]_i in isolated mudpuppy taste cells using calcium imaging with the Ca²⁺-sensitive fluorescent dye fura-2. Mature taste cells were identifiedby their elongate shape and apical fluorescence of the FITC-WGAapplied to the epithelium before dissociation (Fig. 1A,B). Undercontrol conditions, isolated taste cells had intracellular calciumlevels of 71 ± 1 nM (n = 203). Denatonium benzoate increased [Ca²⁺]_i in >80% of the taste cells tested. The increase in [Ca²⁺]_i occurred initially at the apical tip of the taste cell, thenspread basolaterally until [Ca²⁺]_i was increased over the entire cell (Fig. 1C). The initial responseoccurred in the apical end, even though the denatonium was bath-appliedto the entire cell. The time course of the response is shown inFigure 1D. The peak response occurred near the first measurement,which was ~5 sec after application of denatonium to the recordingchamber. Intracellular Ca²⁺ levels began to decline in the presence of denatonium and thendecreased further to baseline levels after the denatonium waswashed from the chamber (Figs. 1D, 2). The peak [Ca²⁺]_i elicited by 5 mM denatonium benzoate was usually 50-150% ofthe resting [Ca²⁺]_i (133 ± 4 nM, n = 203). Repeated applications of denatoniumto the same cell resulted in similar increases in [Ca²⁺]_i, as long as the cell was washed for at least 3 min after eachapplication of denatonium (first application, 130 ± 12 nM; secondapplication, 133 ± 14 nM, n = 16) (Figs. 1D, 3). Sodium benzoate(5 mM) failed to increase [Ca²⁺]_i in five taste cells that responded to denatonium benzoate (5mM), suggesting that benzoate itself has no effect on the tastecells. We also measured [Ca²⁺]_i in nontaste lingual epithelial cells; denatonium failed toincrease [Ca²⁺]_i in any of these cells.
Fig. 3. Denatonium-induced changes in [Ca²⁺]_i depended on intracellular stores. This graph shows maximum denatonium-induced changesin [Ca²⁺]_i expressed as a percentage of resting [Ca²⁺]_i. Cells were tested twice, before (hatched bars) and duringor after (open bars) the treatments indicated, as illustratedin Figure 2 [Ca²⁺-free bath solution (0 Ca; n = 17), thapsigargin (n = 34), ryanodine(n = 12), and U73122 (n = 18)]. Control cells were tested twice,as illustrated in Figure 1D (n = 16), the first and second stimulationsindicated by the hatched and open bars, respectively.
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Calcium was released from intracellular stores
To determine whether extracellular Ca²⁺ was required, we measured [Ca²⁺]_i in response to denatonium in Ca²⁺-free APS. In this medium, the resting [Ca²⁺]_i was reduced (initial level, 73 ± 6 nM; Ca²⁺-free APS, 65 ± 2 nM; n = 17), but not significantly (paired,one-tailed Student's t test = 1.52, df = 16, p = 0.07). The denatoniumresponse persisted in all taste cells tested, although the magnitudeof the response was usually smaller than in Ca²⁺-containing APS (Figs. 2A, 3). This reduction in the denatoniumresponse was statistically significant (paired Student's t test= 2.37, df = 16, p < 0.05). These data illustrate that the responseto denatonium persisted in Ca²⁺-free APS and suggest that at least the major part was mediatedby calcium release from intracellular stores. To investigate therole of calcium stores in the response, we used thapsigargin,a Ca²⁺-ATPase inhibitor. Thapsigargin prevents calcium uptake into theintracellular stores (Chu et al., 1988; Meyer and Stryer, 1990;Thastrup et al., 1990). This results in a gradual depletion ofcalcium from the intracellular stores as the calcium leaks outand is not replenished. We tested the effect of thapsigargin on34 cells that responded to denatonium. Thapsigargin (1 µM) increased[Ca²⁺]_i to a variable extent in all of these cells. This increase in[Ca²⁺]_i was slow, and the peak [Ca²⁺]_i was smaller than the denatonium responses in most cells tested(initial level, 79 ± 4 nM; after thapsigargin, 108 ± 7 nM; n =34). After a 16 min incubation with thapsigargin, which shouldbe sufficient for store depletion, 5 mM denatonium failed to increase[Ca²⁺]_i in 27 of 29 cells tested (Figs. 2B, 3). This effect of thapsigarginon the response to denatonium was statistically significant (pairedStudent's t test = 5.40, df = 26, p < 0.0001). These data stronglysuggest that denatonium releases calcium from internal storesand not from extracellular influx, because thapsigargin inhibitedcompletely the denatonium response. Thus, the decrease in theresponse to denatonium in Ca²⁺-free APS may be attributable to a requirement of extracellularCa²⁺ for reloading of the intracellular stores, as has been shownin neurons (Thayer et al., 1988).

Calcium was released from IP₃-sensitive stores
Two different types of calcium stores have been identified: one coupled to an inositol IP₃ receptor and another coupled toa ryanodine-sensitive calcium receptor (Sharp et al., 1993; Simpsonet al., 1995). To investigate which intracellular calcium receptorsare involved in the denatonium response, we applied denatoniumin the presence of 10 µM ryanodine. Ryanodine did not change resting[Ca²⁺]_i (initial level, 77 ± 6 nM; after ryanodine, 79 ± 6 nM; n =12) and did not affect the [Ca²⁺]_i increase in response to denatonium (Figs. 2C, 3) (125 ± 22nM; n = 12). High concentrations of ryanodine have been shownto inhibit Ca²⁺ release from ryanodine receptor-coupled calcium stores (Sutkoet al., 1985). To determine whether higher concentrations of ryanodinewould inhibit the denatonium response, we incubated taste cellsin 200 µM ryanodine for 11 min, but there was no significant effecton the denatonium response. Thus, ryanodine receptor-coupled calciumstores are not likely to be involved in the response to denatonium.To determine whether calcium stores in taste cells are IP₃ receptor-coupled,we used the PLC inhibitor U73122, because IP₃ is produced viathe PLC pathway (Thompson et al., 1991; Salari et al., 1993).U73122 (5 µM) increased [Ca²⁺]_i in all cells (initial level, 78 ± 5 nM; U73122, 97 ± 6 nM;n = 18). The increase of [Ca²⁺]_i by U73122 itself might be mediated by calcium release fromIP₃ receptor-coupled calcium stores, as shown in rat liver microsomes(De Moel et al., 1995). After a 17 min incubation with U73122,calcium responses induced by denatonium were inhibited (Figs.2D, 3). This effect of U73122 on the response to denatonium wasstatistically significant (paired Student's t test = 7.37, df= 17, p < 0.0001). These results strongly suggest that IP₃ isinvolved in the response of mudpuppy taste cells to denatonium.

Denatonium hyperpolarizes mudpuppy taste cells
We also used giga-seal whole-cell recording to study denatonium transduction in isolated taste cells. Isolated mudpuppy tastecells have resting potentials of approximately $-$ 65 mV and inputresistances of ~1.4 G $Omega$ (Kinnamon and Roper, 1988). Under voltage-clampconditions, we measured voltage-activated current in responseto 1 mM denatonium. Denatonium increased outward currents in 20of 25 cells elicited by step depolarizations from a holding potentialof $-$ 80 mV (Fig. 4A). The increase in outward current was observedat all potentials positive to $-$ 40 mV (Fig. 4B). The outward currentinduced by denatonium was close to 50% greater than the currentrecorded in APS (APS before, 2.7 ± 0.3 nA; 1 mM denatonium benzoate,4.0 ± 0.5 nA; APS after, 3.4 ± 0.7 nA; n = 11). The time courseof the effect is shown in Figure 5. The time course of the currentresponse was similar to the time course of the Ca²⁺ response (e.g., Figs. 1, 2), suggesting that the current responsewas produced by an increase in [Ca²⁺]_i in response to denatonium. Indeed, Ca²⁺-dependent K⁺ (Cummings and Kinnamon, 1992) and Cl (Taylor and Roper, 1994) conductances have been identified inmudpuppy taste cells, and activation of these conductances wouldelicit an increase in outward current under our recording conditions.The current increased, then began decreasing, in the continuedpresence of denatonium. To confirm that the denatonium-inducedincrease in outward current would hyperpolarize the cells, weused current-clamp recording. As expected, the increase in outwardcurrent was accompanied by a 3-10 mV hyperpolarization of theresting potential (n = 2 cells).
Fig. 4. Electrophysiological response of a mudpuppy taste cell to denatonium. The bath contained TTX to block inward Na⁺ currents. A, Whole-cell recording under control conditions andin response to 1 mM denatonium benzoate (DN). The cell was heldat $-$ 80 mV, and the membrane was stepped to +20 mV to elicit outwardcurrent. Leak and linear capacitative currents were subtractedfrom the record by computer. B, Current-voltage relationship ofthe denatonium response in the same cell, as shown in A. Noticethat denatonium increased outward currents at most voltages (solidcircles).
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Fig. 5. Time course of the electrophysiological response to denatonium. The cell was held at $-$ 80 mV, and the membrane was steppedto +20 mV for 175 msec every 3 sec. Data were digitized at 125Hz and plotted with Axoscope software. TTX was present in thebath solution to block Na⁺ currents. Note that 1 mM denatonium elicited an increase in outwardcurrent, which is similar in kinetics to the [Ca²⁺]_i response shown in Figures 1 and 2.
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In some experiments, denatonium was applied focally to taste cells with a picospritzer during whole-cell recording. Underthese conditions, denatonium activated an outward current thatwas similar to the current that was activated by bath applicationof denatonium (data not shown).

G-protein involvement in the response to denatonium
To investigate the involvement of G-proteins in the denatonium response, we used patch pipettes containing a nonhydrolyzableGDP analog, GDP- $beta$ -S (1 mM) (Burch and Axelrod 1987; Gilman, 1987).Six minutes after the establishment of the whole-cell configuration,denatonium still increased the outward current elicited by a voltagestep to +80 mV (Fig. 6A). By 15 min, however, denatonium failedto increase outward currents (Fig. 6B). Three other cells showedsimilar results. Control cells held for similar periods did notshow an appreciable decline in the response to denatonium, makingit unlikely that the decline with GDP- $beta$ -S was attributable eitherto rundown or to desensitization. These results suggest that G-proteinsare required for transduction of denatonium.
Fig. 6. Effect of GDP- $beta$ -S on the denatonium-induced outward current. This cell was held at $-$ 80 mV, and the membrane was stepped to+80 mV. TTX was present in the bath solution to block Na⁺ currents. A, After 6 min of whole-cell recording and B, after15 min of whole-cell recording. Note that the GDP- $beta$ -S (1 mM inpipette solution) abolished the denatonium response, suggestingthat the response was G-protein-dependent.
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To determine which type of G-protein is involved in the pathway, we incubated lingual epithelia in PTX, which inhibits G_i,G_o, gustducin, and transducin by ADP ribosylation of the G-protein $alpha$ subunit (Birnbaumer, 1990; Simon et al., 1991). Dissected lingualepithelia were treated with PTX (0.5 and 2 µg/ml in APS) for >20hr at 4°C. Incubation with PTX affected neither the resting levelsof intracellular calcium (control group, 74 ± 2 nM, n = 13; PTX-treatedgroup, 73 ± 3 nM, n = 24) nor the response to denatonium (Fig.7).
Fig. 7. Denatonium-induced changes in [Ca²⁺]_i did not depend on intracellular cAMP. This graph shows maximum denatonium-induced changesin [Ca²⁺]_i expressed as a percentage of resting [Ca²⁺]_i. Control cells are those illustrated in Figure 3. PTX cellsrepresent two groups of cells: a control group incubated overnightin APS (hatched bar, n = 13) and a treatment group incubated overnightin PTX (open bar, n = 24). Other cells were tested twice before(hatched bars) and during or after (open bars) the treatmentsindicated: IBMX (n = 17); cell permeant cyclic nucleotides (cNMP:db-cAMP, n = 4; db-cGMP, n = 6; 8-cpt-cAMP + db-cGMP, n = 3),and SQ22536 (n = 3).
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cAMP involvement in the response to denatonium
The involvement of cAMP in the denatonium response was examined by increasing intracellular cyclic nucleotides (using IBMX,a phosphodiesterase inhibitor, and cell permeant cAMP and cGMPanalogs) and by decreasing intracellular cyclic nucleotides (usingSQ22536, an inhibitor of adenylate cyclase) (Harris et al., 1979;Goldsmith and Abrams, 1991). Incubation with IBMX did not affectresting [Ca²⁺]_i (initial level, 68 ± 3 nM; after IBMX, 64 ± 3 nM; n = 17).Although IBMX reduced the response to denatonium in some cells,it had no effect on the mean response (Fig. 7). Incubation withcyclic nucleotides did not affect resting [Ca²⁺]_i [db-cAMP (5 mM) before, 66 ± 5 nM and after, 64 ± 4 nM; n =7; db-cGMP (5 mM) before, 62 ± 7 nM and after, 60 ± 7 nM, n =7; 8-cpt-cAMP (2 mM) + db-cGMP (2 mM) before, 67 ± 2 nM and after,65 ± 7 nM, n = 3]. None of the cyclic nucleotides affected thedenatonium-induced calcium response. (Responses are grouped togetherand shown in Fig 7.) Incubation of the cells with SQ22536 (2.5mM for 30 or 40 min) did not affect resting [Ca²⁺]_i (initial level, 54 ± 4 nM; after SQ22536, 55 ± 2 nM; n = 3)and did not affect the denatonium-induced calcium response (Fig.7).

DISCUSSION
In this study, we used calcium-imaging and whole-cell patch recording to examine the transduction of denatonium in isolatedmudpuppy taste cells. The results support the hypothesis thatdenatonium increases [Ca²⁺]_i via a G-protein cascade involving PLC and IP₃ (Hwang et al.,1990; Spielman et al., 1994b). Our evidence does not support thehypothesis that denatonium is transduced via a pathway involvingphosphodiesterase and membrane depolarization via a cyclic nucleotide-suppressiblecation channel (Kolesnikov and Margolskee, 1995; Wong et al.,1996).

The IP₃-mediated hypothesis is supported by a number of observations. First, denatonium benzoate increased intracellular calciumvia calcium release from intracellular stores and not via calciuminflux, as indicated by the effects of thapsigargin and U73122.Second, denatonium induced an outward current across the cellmembrane and not an inward current, as predicted by the phosphodiesterasehypothesis. The denatonium-induced response was not dependenton extracellular calcium; when the concentration of extracellularCa²⁺ was reduced to zero, the denatonium still elicited a calciumresponse. Third, the denatonium-induced response was mediatedvia a G-protein; GDP- $beta$ -S blocked the denatonium-induced outwardcurrent. Finally, neither increases nor decreases in intracellularcAMP levels affected either resting [Ca²⁺]_i or the denatonium-induced response. In combination, these datasupport strongly the hypothesis that denatonium is transducedvia an IP₃-mediated rather than a cAMP-mediated pathway in mudpuppy.

There is evidence in rat and mouse that denatonium acts via the PLC-IP₃ pathway. In rat, IP₃ receptors and Ca²⁺-ATPase are found in taste buds of the circumvallate papilla,at their highest densities near the taste pore (Hwang et al.,1990). Denatonium enhances intracellular levels of IP₃ in thesecells, (Hwang et al., 1990), and IP₃ depletes accumulated Ca²⁺ from intracellular stores in a dose-dependent manner (Hwang etal., 1990). Denatonium increases [Ca²⁺]_i in some rat taste cells (Akabas et al., 1988; Bernhardt etal., 1996). In mouse circumvallate and foliate papillae, denatoniumactivates PLC (Spielman et al., 1994b).

The concentrations of denatonium required to elicit calcium responses in mudpuppy taste cells were higher than those requiredto elicit calcium responses from rat taste cells (Akabas et al.,1988) or IP₃ responses from mouse taste tissue (Spielman et al.,1994b). However, the concentrations were consistent with thosereported to activate a denatonium receptor in bovine taste membranes(Ruiz-Avila et al., 1995). In addition, in behavioral studies,mudpuppies reject food pellets containing 1-10 mM denatonium aftertasting them, suggesting that it is aversive to them (Ogura etal., 1996).

In mouse taste cells, another transduction pathway has been suggested for denatonium; activation of phosphodiesterase viathe G-proteins transducin and gustducin (Ruiz-Avila et al., 1995).By analogy with phototransduction, phosphodiesterase reduces intracellularcAMP. This relieves a cAMP block of a cyclic nucleotide-suppressiblecation channel and causes the cell to depolarize (Kolesnikov andMargolskee, 1995). This hypothesis is supported by the observationthat transgenic mice, which lack gustducin, are less sensitiveto denatonium (Wong et al., 1996). This model of bitter transductionwas not supported by our data in mudpuppy. First, denatonium hyperpolarizedtaste cells; it did not depolarize them. Second, the denatonium-inducedincrease in [Ca²⁺]_i arose from intracellular release and not from influx througha cation channel. Finally, modulation of intracellular cyclicnucleotide levels failed to affect intracellular calcium levels,ruling out a direct effect of cyclic nucleotides on [Ca²⁺]_i. Our evidence that intracellular cyclic nucleotide levels failedto affect the denatonium-induced response also rules out cyclicnucleotide modulation of the IP₃ pathway in mudpuppy taste cells(Lindemann, 1996a).

The identity of the G-protein involved in denatonium transduction in the mudpuppy is moot. In mouse, sucrose octa-acetate,another potent bitter compound, acts via a PTX-sensitive G-proteinsuch as G_i or G_o (Spielman et al., 1994b), but in mudpuppy, PTXfailed to abolish the denatonium-induced response. We do not believethat the lack of effect of PTX resulted from an insufficient incubationperiod, because a similar incubation period was sufficient todemonstrate inhibition by PTX of a G-protein modulated calciumcurrent in mudpuppy taste cells (Delay et al., 1997). These datasuggest that a PTX-insensitive G-protein, such as a member ofthe G_q family (Simon et al., 1991; Taylor et al., 1991), may activatePLC in mudpuppy taste cells. $alpha$ -Subunits of the G_q family havebeen identified in mouse and rat taste tissue (Spielman et al.,1994a; Tabata et al., 1996). It has been suggested that the $beta$ $gamma$ -subunitsof gustducin may activate PLC (Wong et al., 1996); however, becausemouse gustducin has PTX-binding sites, it probably plays no rolehere. Gustducin has not been examined in mudpuppy. Additionalexperiments are necessary to determine which G-proteins couldbe responsible for the denatonium response in mudpuppy taste cells.

Although other bitter stimuli such as caffeine, strychnine, and sucrose octa-acetate activate PLC in mouse taste cells (Spielmanet al., 1994b), not all bitter compounds are transduced via theIP₃ pathway. Some bitter compounds, such as quinine and CaCl₂,directly block the voltage-dependent K⁺ channels that are located on the apical end of mudpuppy tastecells (Kinnamon et al., 1988b; Bigiani and Roper, 1991; Cummingsand Kinnamon, 1992). These K⁺ channels are open at rest, and blocking them causes depolarization.In mouse taste cells, denatonium also blocks voltage-dependentK⁺ channels (Spielman et al., 1989), although the apical locationof these channels has not been established for mouse. In mudpuppy,it is probable that taste cells may have both transduction pathwaysfor bitter stimuli because ~80% of cells responded to quinineand CaCl₂ (Bigiani and Roper, 1991) and a similar percentage respondedto denatonium. It is not clear whether the mudpuppy can discriminateamong these bitter taste stimuli. Behavioral studies show thatmost bitter stimuli are rejected by the mudpuppy (Bowerman andKinnamon, 1994; Ogura et al., 1996). Because mudpuppies do notrespond well to appetitive taste stimuli such as sugars, it isnot surprising that most taste cells respond to bitter stimuli.

The IP₃ pathway is not unique to bitter taste transduction, because it is activated in some mammalian taste cells by syntheticsweeteners (Bernhardt et al., 1996). Other sweet stimuli are transducedvia an adenylate cyclase-cAMP cascade (Striem et al., 1991; Cummingset al., 1993, 1996; Kinnamon and Margolskee, 1996).

The final step in the IP₃ transduction pathway is yet to be confirmed. In rat and mudpuppy taste cells, denatonium increases[Ca²⁺]_i by 50-100 nM (Akabas et al., 1988; Bernhardt et al., 1996;present study). Although this concentration has been suggestedto lead to transmitter exocytosis from synaptic release sites(Akabas et al., 1988; Spielman et al., 1994b; Bernhardt et al.,1996; Kinnamon and Margolskee, 1996), this has yet to be demonstrateddirectly. Compared with these relatively small increases of [Ca²⁺]_i in taste cells, neuroendocrine cells require at least 200 nM(reaching a peak at 1 µM) for exocytosis (Augustine and Neher,1992), whereas goldfish retinal presynaptic terminals requireat least 50 µM [Ca²⁺]_i (Von Gersdorff and Matthews, 1994). Total [Ca²⁺]_i rarely rose above 300 nM in any of the cells we tested. Fortechnical reasons, the measured [Ca²⁺]_i may underestimate the true maximum at synaptic release sites,because we measured [Ca²⁺]_i over the center of the whole cell to avoid edge artifacts andmay have missed contributions from synaptic release sites. Further,the true maximum may have been underestimated because of out-of-focusblur from above and below the image plane. Lindemann (1996b) hasshown that peak transients of [Ca²⁺]_i in taste cells can be underestimated using fura-2, by factorsof >3, unless deblurring algorithms are used to reduce the focaldepth. In addition, the measured maximum [Ca²⁺]_i was usually the first measurement made after denatonium stimulation,and we may have missed the true maximum because of the slow timeresolution of our system. Also, it is possible that the kineticsof calcium binding to fura-2 may have influenced our ability toidentify the true maximum [Ca²⁺]_i (Nowycky and Pinter, 1993). Finally, the data do not rule outthe possibility that denatonium elicits calcium influx throughthe plasma membrane triggered by store depletion, as has beenobserved in several cell types (Striggow and Ehrlich, 1996). Suchan influx could mediate large increases in [Ca²⁺]_i near the membrane that might not be detected by the imagingsystem because of blurring of the signal. Nevertheless, the maximumincreases in [Ca²⁺]_i observed here are similar to those observed in taste cellsin rat and mouse in response to various tastants (Akabas et al.,1988; Bernhardt et al., 1996; Hayashi et al., 1996). This posesthe interesting question of whether these levels of intracellularcalcium are sufficient to cause transmitter release, because theselevels are less than those necessary for exocytosis in neuroendocrinecells and neuronal presynaptic terminals. However, taste cellsare neither neuroendocrine cells nor neurons and may not use thesame mechanisms for exocytosis. For example, taste receptor cellslack synaptophysin, which is an integral transmembrane proteinassociated with synaptic vesicles of the size found in taste cells(Nelson and Finger, 1990). Therefore, the mudpuppy taste cellis a useful model in which to study this problem, because denatoniumincreases [Ca²⁺]_i without depolarizing the cell. Membrane depolarization couldconfound the analysis by increasing [Ca²⁺]_i locally at transmitter release sites. These studies are underway.

FOOTNOTES

Received Jan. 22, 1997; revised March 3, 1997; accepted March 5, 1997.

This work was supported in part by National Institutes of Health Grants DC00244 and DC00766 to S.C.K. We thank Dr. Peter Guthriefor his help in establishing our calcium-imaging system and forcomputer programming, as well as Andrew Bowerman, Vanessa Madsen,and Megan Litster for excellent technical assistance.

Correspondence should be addressed to Dr. Tatsuya Ogura, Department of Anatomy and Neurobiology, Colorado State University,Fort Collins, CO 80523.

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Volume 17, Number 10, Issue of May 15, 1997 pp. 3580-3587 Copyright ©1997 Society for Neuroscience

Bitter Taste Transduction of Denatonium in the Mudpuppy Necturus maculosus

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Volume 17, Number 10, Issue of May 15, 1997 pp. 3580-3587
Copyright ©1997 Society for Neuroscience