Contribution of Different Taste Cells and Signaling Pathways to the Discrimination of "Bitter" Taste Stimuli by an Insect

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The Journal of Neuroscience, August 15, 2002, 22(16):7281-7287

Contribution of Different Taste Cells and Signaling Pathways to the Discrimination of "Bitter" Taste Stimuli by an Insect
John I. Glendinning, Adrienne Davis, and Sudha Ramaswamy
Department of Biological Science, Barnard College, Columbia University, New York, New York 10027

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
CONCLUSION
REFERENCES

Animals can discriminate among many different types of foods. This discrimination process involves multiple sensory systems,but the sense of taste is known to play a central role. We askedhow the taste system contributes to the discrimination of different"bitter" taste stimuli in Manduca sexta caterpillars. This insecthas approximately eight bilateral pairs of taste cells that respondselectively to bitter taste stimuli. Each bilateral pair of bitter-sensitivetaste cells has a different molecular receptive range (MRR); someof these taste cells also contain two signaling pathways withdistinctive MRRs and temporal patterns of spiking. To test fordiscrimination, we habituated the caterpillar's taste-mediatedaversive response to one bitter taste stimulus (salicin) and thenasked whether this habituation phenomenon generalized to fourother bitter taste stimuli (caffeine, aristolochic acid, Grindeliaextract, and Canna extract). We inferred that the two compoundswere discriminable if the habituation phenomenon failed to generalize(e.g., from salicin to aristolochic acid). We found that M. sextacould discriminate between salicin and those bitter taste stimulithat activate (1) different populations of bitter-sensitive tastecells (Grindelia extract and Canna extract) or (2) different signalingpathways within the same bitter-sensitive taste cell (aristolochicacid). M. sexta could not discriminate between salicin and a bittertaste stimulus that activates the same signaling pathway withinthe same bitter-sensitive taste cell (caffeine). We propose thatthe heterogeneous population of bitter-sensitive taste cells andsignaling pathways within this insect facilitates the discriminationof bitter tastestimuli.

Key words: discrimination; bitter taste; taste cell; habituation-generalization paradigm; insect; Manduca sexta

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
CONCLUSION
REFERENCES

Many naturally occurring foods taste "bitter" to humans and elicit an aversive response in animals (Garcia and Hankins, 1975;Brower, 1984). Because some of these foods are toxic and yet othersare nutritious or medicinally active (Rouseff, 1990; Vitazkovaet al., 2001), animals would benefit from an ability to discriminateamong them (Glendinning, 1994). In insects, the detection of differentbitter taste stimuli is not mediated by a uniform population ofbroadly tuned bitter-sensitive taste cells. Instead, it is segregatedacross a heterogeneous population of bitter-sensitive taste cellsand signaling pathways that have different molecular receptiveranges (MRRs) (Glendinning and Hills, 1997; van Loon and Schoonhoven,1999; Glendinning et al., 1999, 2001b). There is evidence thatmammals also possess a heterogeneous population of bitter-sensitivetaste cells (Caicedo and Roper, 2001), but this result is controversial(Adler et al., 2000). Our goal was to determine whether the presenceof bitter-sensitive taste cells and signaling pathways with differentMRRs would help insects discriminate among bitter tastestimuli.

We used the herbivorous caterpillar Manduca sexta for three reasons. First, it has only eight bilateral pairs of bitter-sensitivetaste cells (bipolar sensory neurons) that are distributed acrossfour different classes of sensillum (see Fig. 1). Second, becausethe different classes of bitter-sensitive taste cell have differentMRRs (see Fig. 2), they do not contribute equally to the aversiveresponse to any given bitter taste stimulus (see Table 1). Third,some of the bitter-sensitive taste cells contain two signalingpathways with different response properties. For example, thebitter-sensitive taste cells in the lateral styloconic and epipharyngealsensilla each contain one signaling pathway that responds to caffeineand salicin and another that responds to aristolochic acid. Thecaffeine-activated pathway exhibits a tonic pattern of firing,whereas the aristolochic acid-activated pathway exhibits an acceleratingpattern of firing (see Fig. 2B). Furthermore, the maximal firingrate of the aristolochic acid-activated pathway is twice thatof the caffeine-activated pathway, at least in the bitter-sensitivetaste cell within the lateral styloconic sensillum (see Fig. 2B,C).

There are two ways to test for taste discrimination in animals. One can determine whether subjects can be trained to responddifferentially to two taste stimuli (Spector and Kopka, 2002).Both stimuli are assumed to be discriminable if the training issuccessful. Alternatively, one can determine whether habituatinga subject's aversive response to one taste stimulus generalizesto another taste stimulus. Both taste stimuli are assumed to bediscriminable if the habituation phenomenon fails to generalize(Glendinning and Gonzalez, 1995; Wes and Bargmann, 2001). We adoptedthe latter paradigm because M. sexta caterpillars exhibit weakassociative learning (Dethier and Yost, 1979). Our approach involvedexposing caterpillars to a diet containing an aversive concentrationof salicin for 24 hr. This procedure habituates the caterpillar'staste-mediated aversive response to salicin through a centralgustatory mechanism (Glendinning et al., 2001a). We predictedthat this habituation phenomenon would generalize only to bittertaste stimuli that activate the same taste cells and signalingpathways assalicin.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
CONCLUSION
REFERENCES

Subjects and rearing conditions. The M. sexta caterpillars were reared from eggs on a wheat germ-based artificial diet (Belland Joachim, 1976) and maintained in an environmental chamberwith a 16 hr light/8 hr dark cycle at 25°C. All experiments wereconducted with caterpillars in the 1st or 2nd day of their fifthlarval growth stage (instar). All caterpillars were naive to thetaste stimuli before testing. To control for any potential differencesamong caterpillars from different egg batches, individuals fromeach batch were interspersed indiscriminately across treatmentlevels according to a blind procedure. Sample sizes for each experimentare provided in the figurelegends.

Habituation protocol. The habituation protocol is described in detail elsewhere (Glendinning et al., 2001a). In brief, the"habituated" caterpillars received a block of their rearing dietcontaining a 6% concentration (fresh mass) of salicin (157 mM/kgdiet) as their only source of food and water for 24 hr. This procedurecompletely habituates the aversive response of the caterpillarsto salicin concentrations as high as 12% fresh mass (Glendinninget al., 2001a). The nonhabituated caterpillars received a salicin-freeblock of the same diet containing 6% alphacel (an indigestibleform of cellulose; ICN Biomedicals) as their only source of foodand water for 24hr.

Substrates for presenting taste stimuli. We used two substrates for presenting the taste stimuli. In some tests, the tastestimuli were presented in the caterpillar's rearing diet. Specificconcentrations of each compound were produced by heating the dietto ~60°C, adding the appropriate quantity of compound, stirringvigorously for 3 min, and then pouring the diet into a test cakemold (1.5 cm in diameter and 0.4 cm deep). Once the diet cooled,it assumed a firm and rubbery consistency. Consumption was quantifiedby weighing the caterpillar before and after the taste test (tothe nearest 0.1 mg) on an analytical balance; any increase inmass reflected the amount of diet eaten. The control diets weretreated identically, except that no taste stimulus was added tothem.

In the other taste tests, chemical stimuli were presented in a glass-fiber disk. Four hundred microliters of taste stimulus(dissolved in deionized water) were pipetted onto a glass-fiberdisk (Whatman GF/A, 4.25 cm diameter; Whatman International, Maidstone,UK) and then offered to a caterpillar immediately afterward (tominimize evaporative water loss). Consumption was quantified byrecording the number of bites taken over the 2 min taste test,using a software-based event recorder (Glendinning et al., 2000b).

Brief-access taste test. After a 30 min period of food deprivation, the caterpillar was weighed and then placed on the testplatform (i.e., an inverted Petri dish) so that its head contactedthe test diet. Care was taken to ensure that the caterpillar'slegs grasped the test diet. The 2 min taste test began once thecaterpillar took its first bite. After the test ended, the caterpillarwas weighed a second time and then returned for 30 min to thediet it received during the habituation period so that it couldovercome any hunger that might have developed over the courseof the test. Next, it was food deprived for 30 min and then subjectedto another brief-access taste test. The caterpillar was offeredthe control diet during the first test and a bitter diet duringthe secondtest.

To control for individual differences in biting rate and motivational state during the brief-access taste tests, the followingresponse variable was calculated separately for each caterpillar:percentage of control response = (amount of bitter taste stimuluseaten/amount of control taste stimulus eaten) × 100. This parameteryielded a value of 100% when the caterpillar ingested equal amountsof the bitter and control taste stimulus, indicating that thetwo stimuli were not treated differently. Values approaching 0indicated that the bitter taste stimulus was substantially lesspalatable than the control tastestimulus.

Same/different taste test. After a 30 min period of food deprivation, the caterpillar was placed on a test platform with thecontrol disk (see below). The test platform was an inverted Petridish with a piece of cork (1 cm diameter, 0.4 cm tall) attachedto the center; the glass-fiber disk was pinned to the cork. Carewas taken to ensure that the caterpillar's legs and prolegs graspedthe control disk. Once the caterpillar began to bite the controldisk (but before it had taken >30 bites), it was transferred tothe experimental disk (see below). To minimize disturbance ofthe caterpillar during the transfer, the experimental disk waspositioned next to its head, and the animal was permitted to walkonto the disk on its own. Once the caterpillar grasped the experimentaldisk with its prolegs, the disk was pinned to a second test platform.The 2 min taste test began once the caterpillar took its firstbite from the experimental disk. We recorded the timing of allbites.

We assumed that the transfer from control to experimental disk did not disturb the caterpillar if it took $>=$ 20 bites from theexperimental disk during the taste test. However, if the caterpillartook <20 bites on the experimental disk, then we could not becertain whether the lack of biting was produced by (1) the aversivetaste stimulus in the experimental disk or (2) the transfer procedure.To distinguish between these two possibilities, we transferredthe caterpillar back to the control disk immediately after the2 min test. If it initiated vigorous biting on the control disk(i.e., took >20 bites in <30 sec), then we assumed that the aversivetaste stimulus inhibited biting. If the caterpillar failed toinitiate feeding on the control disk, then we assumed that thetransfer procedure itself inhibited biting. We used data onlyfrom those caterpillars that either took $>=$ 20 bites from the experimentaldisk during the feeding test or reinitiated vigorous biting onthe control disk after the 2 min feedingtest.

After the first same/different test, the caterpillar was permitted to feed ad libitum on its rearing diet for 30 min. Then,it was food deprived for 30 min and run through a second same/differenttaste test with an experimental disk containing a different bittertaste stimulus. Because each caterpillar was tested with two bittertaste stimuli, the presentation order of each taste stimulus wasrandomized separately for eachcaterpillar.

Experiment 1: does the habituation phenomenon generalize to other bitter taste stimuli? To address this question, we usedboth of the taste-testing protocols described above. We used thebrief-access taste test to determine whether the habituation phenomenonwould generalize to four other bitter taste stimuli. To this end,we tested each habituated and nonhabituated caterpillar twice,once with a control substrate and a second time with a bittersubstrate. The bitter substrates contained salicin (157 mM/kgdiet, fresh mass; Sigma-Aldrich), caffeine (7.7 mM/kg diet; Sigma-Aldrich),aristolochic acid sodium salt (0.76 mM/kg diet; Sigma-Aldrich),Grindelia extract [1.2% fresh mass; see Glendinning et al. (1998)for the extraction procedure], or Canna extract [a 0.3× concentration;see Peterson et al. (1993) for details]. All bitter taste stimuli,except for the Canna extract, were presented in the test diet.The Canna extract was presented in a glass-fiber disk; the controldisk for this test was treated with water alone. We selected theindicated concentrations of each bitter taste stimulus becausethey are isoaversive (i.e., the lowest concentrations of eachtaste stimulus that elicit a robust aversive response in M. sexta)and because their aversive behavioral effects are mediated exclusivelyby gustatory input (de Boer and Hanson, 1987; Glendinning et al.,1998, 1999).

We ran two different types of same/different taste tests. First, we asked whether habituated and nonhabituated caterpillarswould exhibit an aversive response after being transferred fromthe control disk containing 5 mM myo-inositol (a palatable tastestimulus) (Glendinning et al. 2000b) to an experimental disk containing5 mM caffeine or 0.1 mM aristolochic acid. Second, we asked whetherhabituated caterpillars would exhibit an aversive response afterbeing transferred from the control disk containing 5 mM caffeineto an experimental disk containing 5 mM caffeine or 0.1 mM aristolochicacid.

Experiment 2: can caterpillars discriminate sensory input from different signaling pathways within the same taste cells? Thisexperiment asked whether habituated caterpillars, lacking theirmedial sensilla, would still exhibit an aversive response to salicin,caffeine, or aristolochic acid. We wanted to determine whethersensory input from the medial sensilla was necessary to elicitan aversive response to aristolochic acid in habituated caterpillars.The medial styloconic sensillum contains a bitter-sensitive tastecell that exhibits a vigorous excitatory response to aristolochicacid but not to salicin or caffeine. We reasoned that the centralprojection sites for the bitter-sensitive taste cell in this sensillummay not become habituated by 24 hr of dietary exposure to salicinand thus may play a key role in mediating the aversive responseto aristolochic acid in habituatedcaterpillars.

We used standard procedures (Glendinning et al., 1999) for surgically ablating the medial sensilla from all caterpillars onthe first day of the fifth instar (Fig. 1). Then, we exposed theablated caterpillars to the control or salicin diet for 24 hr.Finally, we ran these nonhabituated and habituated caterpillarsthrough two consecutive brief-access taste tests, the first withthe control diet and the second with a bitter diet containingsalicin (157 mM/kg diet; fresh mass), caffeine (7.7 mM/kg diet),or aristolochic acid (0.76 mM/kg diet) (Fig. 2).

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Figure 1. A, Diagram of the head of M. sexta, as viewed from below. An enlargement of a maxilla (indicated with an arrow) is provided to show the location of the medial and lateral styloconic sensilla. The epipharyngeal sensilla are located underneath the labrum and thus are not visible in this diagram. There are four taste cells in each of the lateral and medial styloconic sensilla, three taste cells in each of the epipharyngeal sensilla, and three to four taste cells in each of the gustatory sensilla on the maxillary palp. One of the taste cells in each sensillum is bitter sensitive. [This illustration was adapted from Bernays and Chapman (1994), their Fig. 3.4.] B, Diagram of the tip recording method (Hodgson et al., 1955) for recording excitatory responses of taste cells (or neurons) located within a single taste sensillum (for examples, see Fig. 2A). During a recording, the tip of a taste sensillum is inserted into the end of a glass recording/stimulating electrode, which is filled with an electrolyte solution (0.1 M KCl in deionized water) and the taste stimulus. The stimulus solution diffuses through a pore in the tip of the sensillum and activates a transduction mechanism(s) on the distal end of the dendritic process of the taste cell; the electrode records the ensuing action potentials. For clarity, only one taste cell is indicated. Note that the axonal process of the taste cell projects directly to the CNS.

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Figure 2. Illustration of how the peripheral taste system of M. sexta mediates the aversive response to the five "bitter" taste stimuli used in this study. A, Excitatory responses of the four different classes of taste sensilla to five bitter taste stimuli (10 mM salicin, 5 mM caffeine, 0.1 mM aristolochic acid, 0.3× Canna extract, and 1× Grindelia extract; see Materials and Methods for additional details). These neural responses are typical of habituated and nonhabituated caterpillars (Glendinning et al., 1998, 1999, 2001a; J. Glendinning, unpublished data). The onset of stimulation occurred at the beginning of each trace, and each vertical line reflects the occurrence of an action potential. In most of the traces containing a large number of action potentials, there is a single taste cell (the bitter-sensitive taste cell) firing regularly and another taste cell (the salt-sensitive taste cell) firing sporadically. The only exception is the multiunit response of the maxillary palp sensilla to the Grindelia extract, which probably contains action potentials from several bitter-sensitive taste cells. Because all bitter taste stimuli were presented in a 0.1 M KCl solution, we also show representative responses of each sensillum to the electrolyte solution alone for comparison (see bottom row of traces). Note that each bitter taste stimulus selectively activates bitter-sensitive taste cells in a subset of the taste sensilla (e.g., the Grindelia extract stimulated bitter-sensitive taste cells only in the maxillary palp). Furthermore, note that the only taste sensilla that are sufficient to mediate an aversive response to a particular bitter taste stimulus (Table 1) are the ones that contain a bitter-sensitive taste cell that responds vigorously to the same bitter taste stimulus. B, Instantaneous firing rates (total impulses/100 msec; median ± median absolute deviation) of the bitter-sensitive taste cell in the lateral styloconic sensillum to 5 mM caffeine, 10 mM salicin, and 0.1 mM aristolochic acid across 1000 msec of stimulation (Glendinning and Hills, 1997). It is revealed in B (and shown in the traces in A) that caffeine and salicin elicit a relatively tonic pattern of spiking, whereas aristolochic acid elicits an accelerating pattern of spiking. C, Excitatory responses (impulses per second; median ± median absolute deviation) of the bitter-sensitive taste cell in the lateral styloconic and epipharyngeal sensilla to a range of aristolochic acid, caffeine, and salicin concentrations (Glendinning et al., 1999). Note that aristolochic acid elicits a maximal firing rate in the lateral styloconic sensillum that is twice that elicited by caffeine and salicin; no such difference is apparent in the epipharyngeal sensillum.

Data analysis. Because the behavioral data were not distributed normally, we used nonparametric statistical procedures throughout.When comparing the "percentage of control response" to 100%, weused a one-sample Wilcoxon matched-pairs signed-rank test. Whencomparing "number of bites" taken from the two experimental disks,we used a two-sample Wilcoxon matched-pairs signed-rank test.The $alpha$ level was 0.05. We uses the median as a measure of centraltendency and the median absolute deviation (i.e., the median absolutedifference of all values from the sample median) as a measureofvariation.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
CONCLUSION
REFERENCES

Experiment 1: does the habituation phenomenon generalize to other bitter taste stimuli?

In the brief-access taste tests, the nonhabituated caterpillars ate significantly less of the bitter diets than of the correspondingcontrol diets, yielding a percentage of control response thatwas significantly below 100% in all cases (p < 0.05) (Fig. 3A).The habituated caterpillars, on the other hand, exhibited a morecomplex pattern of response (Fig. 3B). The percentage of controlresponse for salicin and caffeine was statistically indistinguishablefrom 100% (p > 0.05), whereas that for aristolochic acid, Cannaextract, and Grindelia extract was significantly below 100% (p< 0.05). These data show that the habituation phenomenon generalizedto caffeine but not to aristolochic acid, Canna extract, or Grindeliaextract.

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Figure 3. The habituation phenomenon generalizes to caffeine but not to three other bitter taste stimuli in the brief-access taste test. We show the percentage of control response in nonhabituated (A) and habituated (B) caterpillars during two sequential tests. The caterpillars received the control taste stimulus in the first test and one of the following bitter taste stimuli in the second test: salicin (157 mM/kg diet; fresh mass), caffeine (7.7 mM/kg diet), aristolochic acid (0.76 mM/kg diet), Grindelia extract [1.2% fresh mass; see Glendinning et al. (1998) for details], and Canna extract [400 µl of 0.3× stock solution/glass-fiber disk; see Peterson et al. (1993) for details]. We calculated the percentage of control response by dividing total intake from a bitter diet by total intake from the corresponding control diet (and then multiplying this number by 100). To determine whether a bitter diet elicited an aversive response (i.e., elicited a median response that was significantly <100%), we used a one-sample Wilcoxon matched-pairs signed-rank test (* p $<=$ 0.05). A dashed line was placed at 100% for comparison. Each bar indicates the median ± median absolute deviation (n = 20-25 caterpillars per median).

We conducted two types of same/different taste tests. In the first, we treated the control disk with 5 mM myo-inositol. Thistaste stimulus elicited vigorous biting in the nonhabituated andhabituated caterpillars. However, when the nonhabituated caterpillarswere transferred from the control disk to the experimental disktreated with 0.1 mM aristolochic acid or 5 mM caffeine, they ceasedbiting immediately (Fig. 4A). There was no significant differencein the number of bites taken from the aristolochic acid-treated(median = 1.0) or caffeine-treated (median = 1.5; p > 0.05) disks.The habituated caterpillars, on the other hand, behaved quitedifferently after being transferred to the experimental disks.They continued biting vigorously on the caffeine-treated diskbut ceased biting precipitously on the aristolochic acid-treateddisk (Fig. 4B). In fact, the habituated caterpillars took significantlyfewer bites from the aristolochic acid disk (median = 1.0; p <0.05) than from the caffeine disk (median = 62.0).

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Figure 4. The habituation phenomenon generalizes to caffeine but not to aristolochic acid in the same/different test. Once each caterpillar initiated vigorous biting on the control disk, it was transferred to the experimental disk. We show the median (± median absolute deviation) number of bites taken by each caterpillar from the experimental disk across the 2 min trial. Each panel contains results from two tests that were conducted sequentially on the same caterpillar. In A, nonhabituated caterpillars were offered a control disk treated with 5 mM myo-inositol and experimental disks treated with 0.1 mM aristolochic acid or 5 mM caffeine. In B, habituated caterpillars were offered a control disk treated with 5 mM myo-inositol and an experimental disk treated with 0.1 mM aristolochic acid or 5 mM caffeine. In C, habituated caterpillars were offered a control disk treated with 5 mM caffeine and an experimental disk treated with 0.1 mM aristolochic acid or 5 mM caffeine. We compared total number of bites taken from the caffeine- and aristolochic acid-treated disks, separately for each panel, using the Wilcoxon matched-pairs signed-rank test (NS, p > 0.05; *p $<=$ 0.05). n = 14-16 caterpillars per panel.

In the second same/different taste test, we used only habituated caterpillars and treated the control disk with 5 mM caffeine.All of the caterpillars initiated rapid biting on the controldisk. They continued to bite rapidly after being transferred tothe experimental disk containing 5 mM caffeine but ceased bitingafter being transferred to the experimental disk containing 0.1mM aristolochic acid. The habituated caterpillars took significantlyfewer bites from the aristolochic acid disk (median = 1.0; p <0.05) than from the caffeine disk (median = 73.0).

Taken together, the results from the same/different test corroborate those from the brief-access taste test, confirming thatthe habituation phenomenon generalizes to caffeine but not toaristolochicacid.

Experiment 2: can caterpillars discriminate sensory input from different signaling pathways within the same taste cells?

This experiment sought to determine whether ablating the medial sensilla altered the behavioral response of habituated andnonhabituated caterpillars to salicin, caffeine, or aristolochicacid. The nonhabituated (ablated) caterpillars, as expected, exhibitedan aversive response to the caffeine, salicin, and aristolochicacid diets (Fig. 5A). In contrast, the habituated (ablated) caterpillarsexhibited an aversive response that was exclusive to the aristolohchicacid diet (Fig. 5B). Consumption from the salicin and caffeinediets was nearly identical to that from the control diet. Theseresults show that habituation phenomenon generalized to caffeinebut not aristolochic acid, regardless of whether the medial styloconicsensilla were present or absent.

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Figure 5. The habituation phenomenon generalizes to caffeine but not to aristolochic acid in caterpillars lacking their medial styloconic sensilla. We show the percentage of control response by nonhabituated (A) and nonhabituated (B) caterpillars during two sequential brief-access taste tests. The insects received the control diet in the first test and one of the following bitter diets in the second test: salicin (157 mM/kg diet; fresh mass), caffeine (7.7 mM/kg diet), or aristolochic acid (0.76 mM/kg diet). We calculated the percentage of control response by dividing total intake from a bitter diet by total intake from the corresponding control diet (and then multiplying this number by 100). To determine whether a bitter diet elicited an aversive response (i.e., elicited a median response that was significantly <100%), we used a one-sample Wilcoxon matched-pairs signed-rank test (*p $<=$ 0.05). A dashed line was placed at 100% for comparison. Each bar indicates the median ± median absolute deviation (n = 20-24 caterpillars per median).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
CONCLUSION
REFERENCES

We found that the 24 hr of dietary exposure to salicin completely habituated the aversive response of M. sexta to salicin.This habituation phenomenon generalized to caffeine but not toaristolochic acid, Canna extract, or Grindelia extract. Becausethe aversive response to all of these bitter taste stimuli ismediated exclusively by sensory input from the bitter-sensitivetaste cells (de Boer and Hanson, 1987; Glendinning et al., 1998,1999), the habituation phenomenon must have been limited to thegustatory neuraxis. Furthermore, because the habituation phenomenonis mediated centrally (Glendinning et al., 2001a), the observedpattern of generalization cannot be explained by a reduction inperipheral responsiveness to the bitter taste stimuli (Glendinninget al., 2001b). It follows, therefore, that exposure to the salicindiet must have selectively habituated the CNS of M. sexta to thepattern of gustatory input elicited by salicin andcaffeine.

Why did the habituation phenomenon generalize to some but not all bitter taste stimuli?

Salicin and caffeine stimulate a common signaling pathway within the same bitter-sensitive taste cells (Glendinning and Hills,1997; Glendinning et al., 1999), and as a result, elicit excitatoryresponses that are virtually identical in terms of maximal firingrate and temporal pattern of firing (Fig. 2). We propose thatthe habituation phenomenon generalized from salicin to caffeinebecause the central gustatory system could not discriminate thepattern of activity elicited by these two tastestimuli.

In contrast, because salicin, Grindelia extract, and Canna extract are all sensed by different populations of bitter-sensitivetaste cells (Fig. 2A, Table 1), they would all produce a distinctspatial pattern of activation within the primary projection siteof the bitter-sensitive taste cells, the subesophageal ganglion(SOG). If we assume that the habituation phenomenon was restrictedto loci in the SOG that receive input from taste cells responsiveto salicin, then we would not expect it to generalize to lociin the SOG that receive input from taste cells responsive to Grindeliaor Canna extract. Although knowledge of the central projectionsites within the insect SOG is fragmentary (Mitchell et al., 1999),there is evidence that axons from individual taste cells in Drosophilamelanogaster (adults) project to spatially restricted regionsof the SOG (Shanbhag and Singh, 1992; Dunipace et al., 2001).


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Table 1. Location of the different classes of bitter-sensitive taste cells in M. sexta

Our most surprising finding was that the salicin habituation phenomenon did not generalize to aristolochic acid, althoughsalicin and aristolochic acid stimulate the same bitter-sensitivetaste cells (Glendinning and Hills, 1997; Glendinning et al.,1999). We can propose two (non-mutually exclusive) explanationsfor this finding. First, the CNS of M. sexta may have habituatedselectively to the low rate of firing rate or the tonic temporalpattern of firing generated by the salicin-activated signalingpathway, (Fig. 2). Second, because salicin stimulates the bitter-sensitivetaste cell within the medial styloconic sensilla only weakly (Fig.2A, Table 1), it is unlikely that 24 hr of dietary exposure tosalicin would have habituated the loci in the SOG that receiveinput from this taste cell. If so, then sensory input from themedial sensilla alone could have mediated the aversive responseto aristolochic acid. We were able to reject this second explanation,however, by showing that habituated caterpillars, lacking theirmedial sensilla, still exhibited an aversive response to aristolochicacid (Fig. 5). This result indicates that although sensory inputfrom the medial sensilla may have contributed to the aversiveresponse to aristolochic acid in intact (habituated) caterpillars,it was notnecessary.

Several investigators have suggested that the colocalization of more than one receptor type or signaling pathway within thesame chemosensory cell should reduce the potential for discrimination(Bernhardt et al., 1996; Adler et al., 2000; Dunipace et al.,2001). Our findings (and those from the nematode, C. elegans;see below) contradict this speculation. We show that the CNS ofM. sexta can discriminate readily between gustatory input fromtwo signaling pathways that are colocalized within the same tastecells. Further work is needed to determine the mechanistic basisof this discrimination. The most likely mechanism would involvea circuit in the CNS that discriminates between the firing rateand temporal patterns of spiking generated by the two signalingpathways (Fig. 2). Previous studies in insects and vertebratesindicate that firing rate (Scott and Giza, 1987; van Loon andSchoonhoven, 1999) or temporal pattern of firing (Katz et al.,2001; Varkevisser et al., 2001; Vickers et al., 2001) could serveas a basis for chemosensorydiscrimination.

Like M. sexta, the nematode C. elegans expresses multiple signaling pathways within individual chemosensory neurons and readilydiscriminates among chemical stimuli that activate these colocalizedsignaling pathways. However, unlike M. sexta, the nematode expressesthese signaling pathways asymmetrically across each homologouspair of chemosensory neurons, resulting in neurons with differentmolecular receptive ranges (Pierce-Shimomura et al., 2001; Wesand Bargmann, 2001). The nematode appears to use this functionalasymmetry to help differentiate chemical stimuli (Pierce-Shimomuraet al., 2001; Wes and Bargmann, 2001). It is unlikely that M.sexta uses an analogous discrimination mechanism because eachbilateral pair of bitter-sensitive taste cells displays symmetricalresponse properties. For instance, the left and right bitter-sensitivetaste cells within the lateral styloconic (or epipharyngeal) sensillaboth respond vigorously to caffeine, salicin, and aristolochicacid (J. Glendinning, unpublisheddata).

Are there different subqualities of bitterness?

We found that the CNS of M. sexta can use the segregated input from different bitter-sensitive taste cells and signaling pathwaysto discriminate among bitter taste stimuli. This discriminationcould be mediated by one of the following cognitive mechanisms.First, all of the bitter taste stimuli may elicit the same tastequality (e.g., bitterness), but nevertheless be discriminable,because the habituation phenomenon makes the central gustatorysystem selectively unresponsive to sensory input elicited by salicinand caffeine. Second, if the discriminable bitter taste stimulielicit different taste qualities (e.g., different subqualitiesof bitterness), then the habituation phenomenon could make thegustatory system selectively unresponsive to the taste qualityevoked by salicin and caffeine. To evaluate these two cognitivemechanisms, one could attempt to train nonhabituated caterpillarsto respond differentially to isoaversive concentrations of salicin,aristolochic acid, Grindelia extract, and Canna extract (Spectorand Kopka, 2002). Successful training would indicate that thebitter taste stimuli each produce distinct tastequalities.

The question of whether mammals perceive different subqualities of bitterness is unresolved. On the one hand, electrophysiologicalstudies indicate that the peripheral taste system of mammals segregatesthe detection of different bitter taste stimuli into distinctpopulations of bitter-sensitive taste cells (Caicedo and Roper,2001) and signaling pathways (for review, see Glendinning et al.,2000a) and that this segregation is preserved, albeit weakly,as information flows up the primary afferent fibers (Dahl et al.,1997; Danilova et al., 1999) and into the insular cortex (Scottet al., 1999). Furthermore, short-term (McBurney et al., 1972)and long-term (Zellner et al., 1985) exposure to one bitter tastestimulus appears to reduce the aversiveness of some but not allbitter taste stimuli in humans and rats. On the other hand, thefact that individual taste cells in rodents each express a largerepertoire of bitter taste receptors has led some to infer a limitedpotential for bitter taste discrimination (Adler et al., 2000).In support of this molecular work, psychophysical studies withrats and humans indicate that different bitter taste stimuli produceindiscriminable gustatory sensations (Lindsey and Breslin, 2001;Keast and Breslin, 2002; Spector and Kopka, 2002). Clearly, morestudies are needed to resolve these contradictoryfindings.

  CONCLUSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
CONCLUSION
REFERENCES

Taste discrimination mechanisms help animals distinguish among foods that vary in nutritive value and potential toxicity.The ability to discriminate among bitter-tasting foods would beparticularly useful for herbivorous animals because many planttissues taste bitter, but only a fraction of these bitter planttissues are actually toxic (Rouseff, 1990; Glendinning, 1994).Our results show that the herbivorous M. sexta can readily discriminateamong bitter taste stimuli and that its heterogeneous populationof bitter-sensitive taste cells and signaling pathways facilitatesthis discrimination process. Given that the gustatory system ofinsects also segregates the detection of nutrients into differenttaste cells (Glendinning et al., 2000a) and signaling pathways(Dahanukar et al., 2002), it is possible that the taste discriminationmechanisms proposed herein for bitter taste stimuli may also beused to differentiate different types of carbohydrates and aminoacids.

  FOOTNOTES

Received Feb. 12, 2002; revised May 23, 2002; accepted May 24, 2002.

This project was supported in part by research Grant 5 R29 DC 02416 from the National Institute on Deafness and Other CommunicationDisorders, National Institutes of Health (J.I.G.). We thank AlanSpector and several anonymous reviewers for valuable editorialcomments.

Correspondence should be addressed to John I. Glendinning, Department of Biological Science, Barnard College, Columbia University,3009 Broadway, New York, NY 10027. E-mail: jglendinning{at}barnard.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
CONCLUSION
REFERENCES

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