ATP as a Putative Sensory Mediator: Activation of Intrinsic Sensory Neurons of the Myenteric Plexus via P2X Receptors

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The Journal of Neuroscience, June 15, 2002, 22(12):4767-4775

ATP as a Putative Sensory Mediator: Activation of Intrinsic Sensory Neurons of the Myenteric Plexus via P2X Receptors
Paul P. Bertrand and Joel C. Bornstein
Department of Physiology, University of Melbourne, Parkville, Victoria 3010, Australia

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The mucosal terminals of sensory neurons intrinsic to the wall of the intestine are sensitive to the chemical environmentwithin the lumen. Lumenal stimuli probably release sensory mediatorsfrom the mucosal epithelium, which then activate the nerve terminalsindirectly. Here, we tested the idea that ATP activates intrinsicsensory nerve terminals in a way consistent with its being a sensorymediator.
We made intracellular recordings from intrinsic sensory neurons located in the myenteric plexus [identified as AH neurons,which are neurons with a long-lasting afterhyperpolarization followingthe action potential (AP)], located within 1 mm of intact mucosa.Focal electrical stimulation of the mucosa was used to locateand map regions innervated by each neuron. Application of ATP(1-2 mM in the pressure pipette) to these regions elicited trainsof APs that originated at the sensory terminals. ATP- $gamma$ -S produceda similar response, but $alpha$ , $beta$ -methylene ATP and 2-methylthio-ATPwere only weakly active. The P2 receptor antagonist pyridoxalphosphate-6-azophenyl-2',5'-disulphonicacid (PPADS) (60 µM in the bath) abolished the APs evoked by ATPand ATP- $gamma$ -S but spared similar responses evoked by 5-hydroxytryptamine(5-HT). Another P2 receptor antagonist suramin (100 µM in thebath) did not significantly change the number of APs evoked byATP. Either ATP or $alpha$ , $beta$ -methylene ATP desensitized the ATP-evokedAPs; 50% recovery occurred after ~5 sec. The number of APs evokedby ATP was reduced, but not abolished, by the selective 5-HT₃receptor antagonist granisetron (1 µM in thebath).
ATP was applied to the cell bodies of sensory neurons to investigate whether the cell bodies express the same P2X receptoras the terminals. ATP evoked a fast depolarization associatedwith a reduction in input resistance and a reversal potentialof $-$ 11 mV. This depolarization was potentiated by suramin andblocked byPPADS.
We conclude that activation of an atypical excitatory P2X receptor by ATP triggers AP generation in the mucosal processesof the sensory neurons; endogenous 5-HT release may also contributeto activation of the nerve terminals. A similar P2X receptor existson the cell body of the sensory neuron. Together, these data areconsistent with a role for ATP as a sensory mediator in gastrointestinalchemosensorytransduction.

Key words: ATP; electrophysiology; intestine; sensory neuron; sensory transduction; serotonin

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The chemical environment of the intestinal lumen determines the behavior of this organ. Intestinal transit is enhanced bythe presence of short chain fatty acids within the lumen (Richardsonet al., 1991) but slowed by the presence of many other nutrients(Schemann and Ehrlein, 1986; Spiller, 1994). These behaviors aremediated by neurons of the enteric nervous system present in thegut wall. A population of enteric neurons within the myentericplexus of the guinea pig is sensitive to the chemical environmentof the intestinal lumen and may cause changes in intestinal motorbehavior (Kunze et al., 1995; Bertrand et al., 1997); similarneurons have been identified in the submucosal plexus (Kirchgessneret al., 1992).

The intrinsic chemosensitive sensory neurons (also referred to as intrinsic primary afferent neurons) are classed electrophysiologicallyas AH neurons [neurons with a long-lasting afterhyperpolarization(AHP) following the action potential (AP)], have Dogiel type IImorphology (for review, see Furness et al., 1998), and providea dense innervation to surrounding ganglia and the mucosa (Songet al., 1994; Bertrand et al., 1998; Li and Furness, 1998). Ithas been proposed that the nerve terminals of both the intrinsicafferents and the extrinsic afferents of vagal or spinal originare activated by the release of sensory mediators from specializedsensory cells in the mucosal epithelium rather than respondingdirectly to lumenal stimuli (for review, see Kirkup et al., 2001).Indeed, there is good evidence that 5-hydroxytryptamine (serotonin,5-HT) released from enterochromaffin cells can act through 5-HT₃receptors to excite the mucosal terminals of the myenteric sensoryneurons (Bertrand et al., 2000) or the vagal extrinsic primaryafferent neurons (Hillsley and Grundy, 1998) and can act through5-HT_1P receptors to excite the terminals of the submucosal sensoryneurons (Pan and Gershon, 2000). However, 5-HT is unlikely tobe the only sensory intermediary acting on the mucosal terminalsof the sensory neurons, because depletion of 5-HT from the mucosa,or addition of 5-HT receptor antagonists, does not block all ofthe many reflex actions of the intestine (Gershon, 1991; Sanger,1996). It is more likely that several substances, acting in concert,encode the changing lumenal environment (Kirkup et al., 2001).One such substance may beATP.

ATP and P2X receptors are known to be involved in visceral and cutaneous sensory pathways (Wood and Docherty, 1997; Burnstock,2001). The afferent nerve terminals in these pathways expressP2X2 and P2X3 receptors and respond to application of ATP or itsanalogs (Bland-Ward and Humphrey, 2000). ATP and related purinesare also recognized as neurotransmitters (Ralevic and Burnstock,1998) in the central (Edwards et al., 1992), peripheral (Evanset al., 1992; Silinsky et al., 1992), and enteric (Galligan etal., 2000) nervous systems. This has been most convincingly demonstratedin enteric neurons in which ATP-mediated fast EPSPs have beendescribed (Galligan and Bertrand, 1994) and characterized (LePardand Galligan, 1999) and a role in reflexes defined (Bian et al.,2000; Spencer et al., 2000).

Our preliminary data suggests that the mucosal terminals of myenteric sensory neurons are sensitive to ATP (Bertrand et al.,2000). ATP can also activate the terminals of vagal extrinsicprimary afferent neurons (Kirkup et al., 1999), suggesting thatATP could function as a sensory mediator to enteric sensory neurons.In this study, we test the idea that ATP functions as a sensorymediator within the gastrointestinal tract by activating the terminalsof intrinsic sensory neurons with cell bodies in the myentericplexus.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Tissue preparation. All experiments were performed using guinea pigs of either gender (160-280 gm, Hartley strain, from theUniversity of Melbourne) that were fed a standard laboratory dietuntil the day of the experiment. Animals were stunned by a blowto the head and killed by severing the carotid arteries and spinalcord; procedures were approved by the University of MelbourneAnimal Experimentation Ethics Committee. A 2- to 3-cm-long segmentof ileum, 10-20 cm from the ileocaecal junction, was removed andplaced in oxygenated (95% O₂-5% CO₂) physiological saline solutionof the following composition (in mM): 117 NaCl, 1.2 NaH₂PO₄, 1.2MgSO₄, 2.5 CaCl₂, 4.7 KCl, 25 NaHCO₃, and 11 glucose. The physiologicalsaline also contained nicardipine (3 µM) to relax the smooth muscleand scopolamine (1 µM) to minimize neurogenic movements. The segmentwas cut open along the line of the mesenteric attachment and pinnedmucosal side up in a Petri dish lined with a silicone elastomer(Compound 184; Dow Corning, Midland, MI). The mucosa, submucosa,and circular muscle were removed over half the circumference,leaving the myenteric plexus with attached longitudinal muscleexposed (see Fig. 1). The preparation was then transferred tothe base of a small recording chamber (volume of 1-2 ml), stretched,and pinned flat with 80 µm pins. The preparation was superfusedwith warmed (35-36°C) physiological saline at a flow rate of 3ml/min (for additional details, see Bertrand et al., 1997, 1998,2000).

Electrophysiology. Myenteric ganglia were visualized at 200 to 300× magnification using an inverted microscope (IMT-2; OlympusOptical, Tokyo, Japan) with Nomarski differential interferencecontrast optics. Neurons or muscle were impaled with glass microelectrodes(120-200 M $Omega$ tip resistance, 1 mm outer diameter, 0.5 mm innerdiameter; Clark Electromedical Instruments, Kent, UK) containing1 M KCl (or in previous experiments, 2% biocytin in 1 M KCl) usinga mechanical micromanipulator (MP-1; Narishige, Tokyo, Japan).Voltage recordings were made in bridge mode using an Axoprobeor AxoClamp2A, digitized at 2-20 kHz (Digidata 1200A), recordedon a personal computer using Axoscope 8.0 (all from Axon Instruments,Foster City, CA), and then analyzed with Origin 6.0 (MicrocalSoftware, Northampton, MA). Measurements of the electrophysiologicalproperties of AH neurons commenced 10 min or more after impalement(for classification, see Bornstein et al., 1994). The mucosa wasstimulated with a bipolar electrode (114 µm stainless steel insulatedwith Teflon; MedWire, Mt. Vernon, VT) to generate maps of theregion innervated by single AH neurons that assisted in findingregions sensitive to chemical application (Bertrand et al., 1998).Stimulus pulses from 0.5 to 2.0 mA (typically 1.0 mA) and a 0.5msec duration (Master-8 stimulator, ISO-Flex stimulus isolationunit; both from A.M.P.I., Jerusalem, Israel) were used. All otherprotocols were detailed previously (Bertrand et al., 1997, 1998).

Solutions containing agonist or antagonist. Agonists were made up in a HEPES (10 mM)-buffered saline (120 mM NaCl, pH 7.2)and used on the day of the experiment or frozen in aliquots forlater use. Application of small volumes of saline to the mucosadoes not cause firing in myenteric AH neurons (Kunze et al., 1995;Bertrand et al., 1997). Agonists were applied to the mucosa bypressure ejection (10 psi, 10-100 msec duration; PicospritzerII; General Valve, Fairfield, NJ) from one of two micropipettesmounted on matched micromanipulators and positioned ~0.5 mm abovethe intact mucosa and 2-5 mm from the impaled neuron; micropipetteswere withdrawn from the superfusing solution between trials toguard against leakage of agonist onto the mucosa. The locationof agonist application was visually confirmed under 40× magnification.Agonist was applied to the cell body with the same micropipettesused for application to the mucosa. Pressure application protocolswere described previously (Bertrand and Galligan, 1992).

Antagonists were made up and stored in distilled water at a concentration of 10 mM. Tetrodotoxin (TTX) was an exception; itwas initially dissolved in a small amount of acetic acid and storedat 1 mM. Antagonists were added to physiological saline solutionat a 1000-fold dilution and stored in one or more 50 ml reservoirsthat were connected in-line with the superfusion system. Visualobservations of pyridoxalphosphate-6-azophenyl-2',5'-disulphonicacid (PPADS), which is bright orange in solution, suggested thatsubstantial concentrations of antagonists reached the bath within2 min. The practical time limit that antagonists could be superfusedwas 20-40 min; on reaching the bath, antagonists were allowedto equilibrate with the tissue for 8 min, leaving a window of10-30 min, during which measurements could be taken. Initial measurements,taken after ~5 min equilibration, helped to define the onset ofantagonist action but were not included in the averageddata.

Quantification of agonist-evoked responses. The number of APs and/or proximal process potentials (PPPs) (axonal APs that failedto excite somatic APs) elicited by agonist application to themucosa were counted and are collectively referred to as APs; theresults of two to three such applications were then averaged.The latency to the first AP (latency), the number of APs, theduration over which AP discharge took place (duration), and theaverage (f) and instantaneous (f_INT) firing frequency during APdischarge were measured and used to determine agonist rank-orderpotency (see Fig. 2) and the extent to which antagonists wereeffective in blocking the actions of the agonists (see Figs. 3-5).In some neurons, slow depolarizations, similar to the slow EPSPsevoked in AH neurons by focal electrical stimulation, occurred1-2 sec after mucosal application of agonist. These slow EPSP-likeevents were quantified by measuring the peak amplitude, time-to-peak,and the membrane potential before stimulation. The extent to whichthe excitability or the input resistance of the cell was alteredduring the slow depolarization was determined by passing 500 msecpositive and negative current pulses through the recording electrode.The effects of agonists applied to the cell body of AH neuronswere characterized in the same way as were the slow depolarizations,with the exception that changes in input resistance were assessedusing 50 msec currentpulses.

Chemicals. TTX was purchased from Alomone Labs (Jerusalem, Israel);granisetron was the kind gift of SmithKline Beecham (Middlessex,UK). All other chemicals were purchased from Sigma (St. Louis,MO).

Statistics. Unless otherwise noted, all numbers are given as mean ± SEM. The range, where relevant, is given in parentheses.Student's t test was used to compare data for significant differences,with an $alpha$ of 0.05 taken as the cutoff for significance. All ttests were one-tailed and paired unless noted; Bonferroni's correctionfor multiple comparisons was used whenappropriate.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Electrophysiology

Intracellular recordings were made from 45 myenteric neurons with AH type electrophysiological characteristics. This typeof neuron has been characterized previously as a sensory neuron(Furness et al., 1998) with chemosensitive projections to themucosa (Kunze et al., 1995; Bertrand et al., 1997; Bertrand etal., 2000). Each AH neuron, whose shape was determined in thepresent study, had Dogiel type II morphology and electrophysiologicalcharacteristics that were consistent with previous studies. Allof these neurons responded to a single electrical stimulus (0.5msec pulse duration) applied to the mucosa with one or more APs;these APs could still be elicited when the soma was hyperpolarizedby intracellular current injection, indicating that these AH neuronshad an intact projection to the mucosa. Recordings were also madefrom S neurons (interneurons and motor neurons) and circular musclecells to examine the effects of activation of AH neurons on downstreamcircuits. All neurons or muscle cells studied were within 1 mmof the intact mucosa in the circumferential direction (Fig. 1).

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Figure 1. Illustration of the experimental arrangement and the relation of the epithelium and the AH-sensory nerve terminals. A side view of the preparation used in the present study. From the bottom: LM, the longitudinal muscle; MP, myenteric plexus; CM, circular muscle; SMP, submucosal plexus; EPI, epithelium. Note that the circular muscle, submucosal plexus, and epithelium have been dissected away from the right half of the preparation to allow an intracellular recording electrode (RECORD) to impale myenteric AH neurons [sensory neurons and intrinsic primary afferent neurons (IPAN, at the open circle)]. When the cell body of the AH neuron is close enough to the intact mucosa (<1 mm), there is a good chance that one or more of its projections is intact and innervates the mucosa. ATP and other agonists were applied to the mucosa and to the cell body of AH neurons via short-duration pressure ejection. The serotonin-containing enterochromaffin cells (EC Cell) are evenly spaced among the enterocytes. They represent ~1% of the total population of endothelial cells. The mucosal epithelium is likely to be damaged when maintained in vitro (Damaged EPI).

Effect of ATP applied to the mucosa

Twenty-six of 35 AH neurons responded to mucosal application of ATP (1-2 mM in a HEPES-buffered saline, pH 7.2), with a trainof APs arising from a flat baseline (Fig. 2A). ATP was ineffectivewhen applied to regions from which electrical stimulation didnot evoke APs. The APs were often converted into PPPs by directapplication of hyperpolarizing current passed through the recordingelectrode or by an AHP (see Fig. 5A-D), suggesting that the APsare generated distal to the soma and normally invade the cellbody. The latency to the first AP evoked by ATP (1-2 mM) was 0.7± 0.3 sec, and the bursts consisted of 15 ± 3 APs, which occurredwithin 2.1 ± 0.4 sec of the start of the burst (n = 18). The averagefrequency during the bursts was 10 ± 2 Hz, with instantaneousfrequencies up to 30 Hz at the start of the bursts. ATP appliedto the same area of mucosa typically evoked 10 or more burstsof APs. Seven of the 26 AH neurons also responded to ATP witha slow EPSP-like event. An additional two AH neurons respondedto ATP with a slow EPSP-like event but failed to respond witha burst of APs (data not shown).

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Figure 2. Responses in AH-sensory neurons to mucosal application of ATP, ATP- $gamma$ -S, $alpha$ , $beta$ -me-ATP or 2-Me-S-ATP. Representative voltage traces from four different AH neurons during application of ATP or ATP analogs to the mucosa; dotted lines indicate RMP. Calibration in C applies to all traces. The total number of APs is shown to the right of each trace. A, Brief application (100 msec; at the filled triangle) of ATP (2 mM) elicited a train of APs that showed a slowing in frequency during the 1.1 sec duration of the discharge; the average instantaneous frequency ( $f$ _INT) was 29 Hz [resting membrane potential (RMP) of $-$ 67 mV]. B, ATP- $gamma$ -S (2 mM) elicited a 3.0-sec-long train of 22 APs (16 APs shown) that fired at a slow, relatively constant frequency (f_INT of 12 Hz; RMP of $-$ 82 mV). C, $alpha$ , $beta$ -methylene ATP (2 mM) failed to elicited any APs in the majority of cases (RMP of $-$ 68 mV). D, 2-Me-S-ATP (2 mM) also failed to elicit any APs under control conditions (n = 3). E, Histogram showing the average number of APs evoked by agonists for two to three repetitions per cell. ATP, n = 18; ATP- $gamma$ -S, n = 7; $alpha$ , $beta$ -methylene ATP, n = 7; 2-Me-S-ATP, n = 3.

Comparison of ATP with 5-HT

5-HT has been shown previously to activate the mucosal terminals of a subset of myenteric sensory neurons (Bertrand et al.,2000). To test whether ATP and 5-HT activate the same populations,14 of the AH neurons that responded to ATP (above) were also testedwith 5-HT (20 µM) applied to the same regions of mucosa. Ten ofthe 14 AH neurons (71%) responded to 5-HT with a short latencyburst of APs. In these 10 AH neurons, near-maximal responses toATP and 5-HT were compared directly. ATP evoked 12 ± 2 APs (latency,0.34 ± 0.11 sec; duration, 6.5 ± 1 sec), whereas 5-HT evoked moreAPs (18 ± 3; p < 0.05; n = 10) with a similar latency (0.31 ±0.12 sec) and a similar duration (6.9 ± 2.2sec).

Effects of purine analogs applied to the mucosa

Different P2X receptors have different affinities for ATP and ATP analogs (Khakh et al., 2001). To characterize the receptorunderlying the responses to ATP, three ATP analogs were appliedto the mucosa with ATP as a direct comparison; these data werethen used to construct an agonist rank-order potency relationship(see below). ATP- $gamma$ -S, when applied at the same concentrationsas ATP, produced similar short-latency trains of APs (Fig. 2B)and/or slow EPSP-like depolarizations (data not shown). ATP- $gamma$ -S(1-2 mM) evoked 27 ± 7 APs (latency, 0.7 ± 0.5 sec; duration,4.3 ± 1.8 sec; n = 7); the average frequency during the burstswas 11 ± 2 Hz, with instantaneous frequencies of up to 20 Hz atthe start of the bursts. Compared with ATP, ATP- $gamma$ -S-evoked trainsof APs were longer in duration and of a lowerfrequency.

$alpha$ , $beta$ -Methylene ATP ( $alpha$ , $beta$ -me-ATP) (Fig. 2C) (see Fig. 6B) and 2-methylthio-ATP (2-Me-S-ATP) (Fig. 2D) were only weakly activewhen applied to the mucosa. $alpha$ , $beta$ -methylene ATP (1-2 mM) elicitedeither a short train of APs in 2 of 11 AH neurons (two and fourAPs; this proportion was significantly less than the proportionof neurons responding to ATP; p < 0.01; $chi$ ² test; df = 1) or a slow EPSP-like event in another 2 of the 11AH neurons. When $alpha$ , $beta$ -me-ATP (1-2 mM) was repeatedly applied (seebelow), it elicited a few APs in an additional two of three AHneurons (see Fig. 6B). Similarly, 2-Me-S-ATP (2 mM) failed toelicit any short-latency bursts of APs in an additional threeAH neurons (Fig. 2D), each of which responded to ATP; in one ofthese neurons, the presence of suramin (100 µM) seemed to reveala small burst of APs in response to 2-Me-S-ATP.

Based on the average number of APs evoked per agonist application (each at ~1 mM), the agonist rank-order potency is as follows:ATP- $gamma$ -S = ATP > $alpha$ , $beta$ -me-ATP = 2-Me-S-ATP, in which "greater than"denotes an ~10-fold greater relationship (Fig. 2E).

Effect of the P2 receptor antagonists PPADS and suramin

To further characterize the receptor underlying the responses to ATP, two nonselective P2 receptor antagonists were used:PPADS and suramin (Khakh et al., 2001). Superfusion of PPADS (60µM), but not suramin (100 µM), into the bath caused a progressivedecrease in the number of ATP-evoked APs from the mucosa in AHneurons (see below). After 10 min, PPADS abolished the train ofAPs and any slow EPSP-like responses but left trains of APs evokedby 5-HT (20 µM; applied to the same region of mucosa) unaffected(Fig. 3). Lower concentrations of PPADS (10 or 30 µM), sufficientto block fast synaptic transmission in myenteric ganglia (Galliganand Bertrand, 1994; Bian et al., 2000) did not depress ATP-evokedAPs during a 30 min incubation (data not shown) (n = 3).

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Figure 3. Effect of the P2 receptor antagonist PPADS on the train of APs evoked by ATP and 5-HT. Representative voltage traces from a single AH neuron; dotted lines indicate RMP. Calibration in C applies to all traces. Left, A, ATP (2 mM, 100 msec; applied at the filled triangle) elicited a 1.8 sec duration train of 14 APs at an average instantaneous frequency (f_INT) of 13 Hz. B, The response was blocked by PPADS (60 µM). C, Twenty-five minutes after washout of PPADS, APs have reappeared, and the response is shorter in duration and of a higher frequency; f_INT of 26 Hz (RMP, control, $-$ 63 mV; PPADS, $-$ 46 mV; recovery, $-$ 59 mV). Right, A, 5-HT (20 µM, 100 msec; applied at the filled triangle) elicited a train of 23 APs; f_INT of 24 Hz. B, The response was not affected during superfusion with PPADS (23 APs; f_INT of 22 Hz) and remained stable during washout of PPADS (C, 29 APs; f_INT of 22 Hz) (RMP, control, $-$ 64 mV; PPADS, $-$ 48 mV; wash, $-$ 56 mV).

Before addition of PPADS (60 µM), mucosal application of ATP (1 or 2 mM) evoked 13 ± 2 APs (latency, 0.6 ± 0.2 sec; duration,1.4 ± 0.4 sec; n = 6). In the presence of PPADS (60 µM), one AHneuron responded with a single AP, whereas the remaining AH neuronsfailed to respond (p < 0.05; n = 6) (Fig. 3B). Partial recoverywas observed in three AH neurons after 20 min wash (7 ± 1 APs;n =3)

The effects of PPADS on responses to ATP- $gamma$ -S, applied to the mucosa, were also tested for three of the six AH neurons. ATP- $gamma$ -S(1 mM) evoked 14 ± 1.5 APs (latency, AP of 1.2 ± 1.2 sec; duration,1.8 ± 1.2 sec; n = 3), whereas, in the presence of PPADS (60 µM),one AH neuron responded with a burst of 10 APs, and the remainingtwo AH neurons failed to respond (p < 0.05; n =3).

In contrast, PPADS (60 µM) had no effect on the bursts of APs evoked by mucosally applied 5-HT in one AH neuron (whose ATPresponse was blocked) or in two additional AH neurons whose responsesto ATP were not tested (Fig. 3). 5-HT evoked 17 ± 6 APs (latency,0.2 ± 0.1 sec; duration, 2.1 ± 1.4 sec; n = 3), whereas, in thepresence of PPADS (60 µM), it evoked 19 ± 7 APs (latency, 0.2± 0.1 sec; duration, 1.8 ± 0.7 sec; p > 0.05; n =3).

When suramin (100 µM) was superfused into the bath, it was accompanied on three of six occasions by bursts of spontaneousAPs that persisted when the soma was hyperpolarized and, thus,apparently originated in axonal processes rather than the soma.This activity subsided after ~5min.

Before the addition of suramin, ATP (1 mM) evoked 10 ± 1 APs (latency, 0.7 ± 0.3 sec; duration, 1.4 ± 0.7 sec; n = 6), whereas,in the presence of suramin (100 µM), it evoked 11 ± 2 APs (latency,0.6 ± 0.3 sec; duration, 1.6 ± 1.0 sec; p > 0.05; two-tailed ttest; n = 6) (Fig. 4). Overall, there was no significant effectof suramin; however, in two of the six AH neurons, suramin causedan increase in the number of APs in a burst (Fig. 4B), whereasin the other four AH neurons, there was little change from control.

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Figure 4. Effect of the P2 receptor antagonist suramin on the train of APs evoked by ATP. Representative voltage traces from a single AH neuron; the dotted lines indicate RMP. Calibration in C applies to all traces. The total number of APs is shown to the right of each trace. A, ATP (2 mM, 100 msec; applied at the filled triangle) elicited a train of 12 APs at an average instantaneous frequency (f_INT) of 30 Hz for a duration of 0.8 sec. B, The response was not reduced by suramin (100 µM) (17 APs; $f$ _INT of 16 Hz; duration of 2.1 sec). C, Thirty minutes after washout, the response is shorter and of a higher frequency than in suramin (13 APs; f_INT of 30 Hz; duration of 1.0 sec) (RMP, control, $-$ 69 mV; suramin, $-$ 70 mV; recovery, $-$ 65 mV).

Desensitization of the ATP-evoked train of APs

Many P2X receptors rapidly desensitize, and this has been used to distinguish between different subtypes of receptor (Ralevicand Burnstock, 1998). The receptors responsible for the burstof APs evoked by ATP were tested for desensitization. The ATP-evokedburst of APs was suppressed (Fig. 5A-D,F) when either ATP or $alpha$ , $beta$ -methyleneATP was applied to the mucosa a few seconds before a test stimulus;in the case of $alpha$ , $beta$ -methylene ATP, repeated applications were required.When ATP was applied 1 sec after a prepulse of ATP, the secondapplication usually failed to evoke any APs; however, these datawere hard to quantify because the durations of the control burstswere variable. When the interval was extended to 2 sec, the numberof APs evoked by the second application of ATP was reduced from8 ± 1 to 1 ± 1 APs (p < 0.05; n = 5). ATP-evoked APs recoveredfrom desensitization with ATP, with a half-time to recovery of~5 sec. When ATP was applied 1 sec after six prepulses of $alpha$ , $beta$ -methyleneATP, the ATP-evoked burst of APs was reduced from 17 ± 5 to 2± 1 APs (p < 0.05; n = 3).

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Figure 5. ATP can desensitize the train of APs evoked by ATP. A-D, Representative voltage traces from a single AH neuron; the dotted lines indicate RMP. Calibration in B applies to all traces. ATP was applied twice to the mucosa at the vertical lines with a 2, 4, 6, or 8 sec interval (A-D, respectively); the total number of APs is shown to the right of each trace. The diagonal lines indicate a break in the trace of a variable length of time. In control (A-D), ATP evokes a burst of APs consisting of between seven and nine APs. Subsequent APs evoked by the second application of ATP are depressed when the interval is shorter than 8 sec. Note that the long AHP after AP generation does not prevent incoming APs from the distal processes from evoking PPPs. E-G, Calibration in G also applies to E. The total number of ATP-evoked APs is shown to the right of each trace. E, In control, ATP evoked a burst of APs consisting of between seven and nine APs (3 repetitions). F, $alpha$ , $beta$ -me-ATP was then applied six times in rapid succession to the same region of mucosa, and ATP was applied immediately after. G, Two minutes later, the ATP response was fully recovered.

Effect of granisetron, a 5-HT₃ receptor antagonist

Trains of APs evoked by ATP or 5-HT had similar latencies, comparable numbers of APs, and occurred in a similar populationof AH neurons (see above). We tested the idea that the responseto ATP is attributable to the release of endogenous 5-HT frommucosal enterochromaffin cells (Fig. 6). In control, ATP (1 mM;n = 4) or ATP- $gamma$ -S (1 mM; n = 2) evoked 18 ± 4 APs (latency, 0.3± 0.1 sec; duration, 3.1 ± 0.6 sec; n = 6), whereas, in the presenceof granisetron (1 µM), they evoked 10 ± 3 APs (latency, 0.7 ±0.3 sec; duration, 1.3 ± 0.3 sec). This decrease in the numberof APs, from 18 to 10 (45%), was found to be significant (p <0.05; n = 6). In four of the same neurons, 5-HT evoked 19 ± 8APs (latency, 0.2 ± 0.1 sec; duration, 5.0 ± 3.5 sec; n = 4);these bursts were completely blocked in the presence of granisetron.These data suggest that the actions of endogenously released 5-HTare also blocked by granisetron and, thus, that the granisetron-resistantresponse to ATP is not mediated by 5-HT.

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Figure 6. Effect of granisetron on trains of APs evoked by ATP and 5-HT. Representative voltage traces from a single AH neuron; the dotted lines indicate RMP. Calibration in C applies to all traces. The total number of APs is shown to the right of each trace. Left, A, ATP (1 mM, 100 msec; applied at the filled triangle) elicited a train of 10 APs at an average instantaneous frequency (f_INT) of 12 Hz for a duration of 2.1 sec. B, Granisetron (1 µM) caused a significant reduction in the number of APs (8 APs; f_INT of 13 Hz; duration of 0.6 sec; RMP of $-$ 77 mV). C, The train of APs recovered after washout of granisetron (9 APs; f_INT of 11 Hz; duration of 0.8 sec). Right, A, 5-HT (20 µM, 100 msec; applied at the filled triangle) elicited a train (15 APs; f_INT of 11 Hz; duration of 3.9 sec). B, Granisetron (1 µM) fully blocked this response. C, Twenty-five minutes after washout of granisetron, the number of APs had increased (8 APs; f_INT of 10 Hz; duration of 3.1 sec). Note that the long AHP after AP generation in C does not prevent incoming APs from the distal processes from evoking PPPs.

Effects on enteric microcircuitry

S neurons (interneurons and motor neurons) located within the same ganglia as were the AH neurons were also studied. In 9of 12 S neurons of unknown functional class, ATP or ATP- $gamma$ -S (1mM), applied to a region of mucosa directly circumferential tothe impaled neuron, caused a sustained burst of fast EPSPs thatconsisted of 25 or more distinct peaks (Fig. 7A). When hexamethonium(300 µM) was added to the bath, most of these fast EPSPs wereblocked (n = 3) (data not shown), indicating that ATP is actingat upstream neurons rather than at the cell body of the S neuron.Five of these 12 S neurons were also tested with 5-HT (20 µM)applied to the same region of mucosa, and all responded with asimilar burst of fast EPSPs (data not shown). In 5 of 12 S neurons,ATP applied to the mucosa evoked a slow EPSP-like depolarizationwith (n = 2) or without (n = 3) a burst of fast EPSPs (Fig. 7A).

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Figure 7. Effect of ATP applied to the mucosa on myenteric S neurons and circular muscle. ATP (1 mM) was applied to mucosa directly circumferential from the impalement. Calibrations in A applies to all traces. A, Representative voltage traces from two S neurons; the dotted lines indicate RMP. Top, ATP evoked a burst of fast EPSPs, two of which reach threshold for AP generation. Bottom, ATP evoked a slow EPSP-like depolarization that evoked many APs. B, Voltage traces from a single circular muscle cell. Top, Electrical stimulation of the mucosa, directly circumferential to the recording site, evoked a biphasic inhibitory junction potential (RMP of $-$ 48 mV). Bottom, Application of ATP to the same site on the mucosa evoked a biphasic inhibitory event, similar to that evoked electrically (RMP of $-$ 55 mV). ES, Electrical stimulation.

When circular smooth muscle cells were impaled, ATP (1 mM) applied to a region of mucosa directly circumferential to the impaledcell evoked a hyperpolarization, followed by a depolarization(n = 8) or a prolonged hyperpolarization (n = 2) in cells from10 separate preparations (Fig. 7B). The hyperpolarizations weresimilar in amplitude to inhibitory junction potentials evokedby electrical stimulation of the mucosa and were blocked by additionof TTX (1 µM; n = 3) (data not shown), suggesting that ATP didnot act directly on the smooth muscle. ATP- $gamma$ -S (1 mM) evoked similarhyperpolarizations in the circular muscle cells in an additionalthree preparations. No cholinergic excitatory junction potentialswere recorded in these experiments because the muscarinic receptorantagonist scopolamine (1 µM) was present in the bathingsolution.

Effect of ATP applied to the neuronal soma

To investigate whether AH neurons express the same P2X receptor on the cell body as on the terminal, ATP (1-2 mM) was appliedto the cell bodies of 16 AH neurons, including four that had respondedto mucosal application of ATP. Twelve of the AH neurons (includingthree that had responded to mucosal application) responded toATP with a large somatic depolarization (12 ± 3 mV at $-$ 65 mV)that had a short latency (~100 msec) and initiated somatic APs(Fig. 8A); in 4 of the 12 AH neurons, only the first applicationof ATP evoked a depolarization. When ATP was applied under directvisual control to either ganglionic or interganglionic regions,it caused movements of the underlying longitudinal muscle butdid not affect AH neurons.

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Figure 8. Effect of ATP applied to the cell body of myenteric AH-sensory neurons. Representative voltage traces from two AH neurons (A, B); the dotted lines indicate RMP. A, ATP was applied to mucosa with an increasing duration in milliseconds (numbers to the left of the trace). The top calibration bar applies to the top two traces; the bottom calibration applies to all traces. A', Summary data from three AH neurons in which ATP evoked depolarizations that did not generate APs. B, ATP was applied to the cell body under control conditions and during superfusion with PPADS (60 µM), which blocked, and suramin (100 µM), which potentiated, the depolarization.

The somatic depolarization was associated with a decrease in input resistance and was increased in amplitude by increasingthe duration of ATP ejection (10 msec, 3 ± 2 mV; 20 msec, 8 ±3 mV; 50 msec, 14 ± 5 mV; 100 msec, 19 ± 4 mV; n = 5) (Fig. 8B).Hyperpolarizing the cell up to $-$ 90 mV also resulted in an increasein the amplitude of the somatic depolarization; the reversal potentialfor the depolarization was estimated to be $-$ 11 ± 13 mV from datataken at holding potentials between $-$ 20 and $-$ 80 mV (n = 4). TTX(1 µM) did not alter the size or duration of the depolarizationin three AH neurons in which the somatic depolarization did notinitiate APs. PPADS (60 µM), superfused into the bath, blockedthe response to ATP (2 mM, 50 msec) (control, 15 mV; PPADS, 2mV; wash, 17 mV; n = 4), whereas suramin (100 µM) doubled theamplitude of the depolarization (control, 7 mV; suramin, 15 mV;wash, 6 mV; n = 8). Both PPADS and suramin blocked the ATP-evokedmovements of the longitudinal muscle (seeabove).

In 5 of these 12 AH neurons, the somatic depolarization was followed by a hyperpolarization. This hyperpolarization was associatedwith a decrease in the membrane resistance, and its amplitudewas increased during depolarization of the cell (Fig. 8B, endof trace); this response was not dependent on AP generation andwas similar to that reported by Katayama and Morita (1989).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this study, we found that local application of ATP to the mucosal epithelium of the intestine generates APs in the mucosalprocesses of intrinsic sensory neurons innervating that region.These APs then propagate back to the cell bodies of the sensoryneurons in the myenteric plexus. This effect is mimicked by aP2X receptor agonist and blocked by a P2 receptor antagonist.An additional finding is that the same P2X receptor appears tobe expressed on both the terminals and the cell bodies of thesensoryneurons.

ATP activates the mucosal terminals of enteric sensory neurons

The following observations support our conclusion that ATP activates the sensory neurons by an action on the mucosal nerveterminals. Application of ATP to the cell body and to the mucosagenerate distinctly different responses: ATP acting at the cellbody produces a large depolarization capable of evoking somaticAPs, whereas mucosal application causes APs arising from a flatbaseline. Somatic APs evoked by mucosal application of ATP areconverted to PPPs by somatic hyperpolarization, whereas thoseevoked by somatic application of ATP are blocked by such a hyperpolarization.This indicates APs attributable to mucosal application were generatedat a site distant from thesoma.

ATP evoked APs from the mucosa only when applied to relatively small regions. When electrical stimuli were applied to thesesame regions, an antidromically conducted AP with a 3-7 msec latencywas always found; this suggests a site of initiation several millimetersfrom the soma, consistent with the position of the stimulatingelectrode. These regions of mucosa were well correlated with areasfrom which 5-HT or electrical stimulation evoked trains of APs(Bertrand et al., 1998). This suggests that, when ATP is appliedto the mucosa, it interacts with specialized regions of mucosathat contain the terminals of sensoryneurons.

We did not find any evidence that 5-HT stimulated the release of ATP, although we did find evidence that ATP causes the releaseof endogenous 5-HT. The selective 5-HT₃ receptor antagonist granisetronconsistently reduced the number of APs in a train evoked by ATPin a reversible manner, whereas the responses to 5-HT were blocked.These data, combined with results from our previous study (Bertrandet al., 2000), suggest that the actions of endogenously released5-HT would also be blocked by granisetron and, thus, that thegranisetron-resistant response to ATP is not mediated by 5-HT.Thus, 5-HT, released by ATP, activates the same sensory nerveterminals as ATP itself, suggesting that 5-HT₃ receptors and P2Xreceptors are colocalized on the same sensory nerveterminals.

Similar receptors are on the cell bodies of enteric sensory neurons

P2X receptors mediate fast synaptic transmission to descending interneurons and inhibitory motor neurons of the enteric nervoussystem (Johnson et al., 1999; LePard and Galligan, 1999; Bianet al., 2000). This is, however, the first study to show P2X-likedepolarizations in identified sensory neurons. In the presentstudy, we applied high concentrations of ATP to the cell bodiesof AH-sensory neurons and found depolarizations associated witha reduction in membrane resistance. Of these neurons, three offour AH neurons responded to mucosal application of ATP with atrain of APs; thus, they appeared to express the same receptorat the nerve terminal at the cell body. In almost half of theAH neurons tested, the depolarization was followed by a longer-lastinghyperpolarization associated with a decrease in membrane resistanceand was increased in amplitude during depolarization of the cell.This hyperpolarization was similar to that seen previously byKatayama and Morita (1989) who did not, however, find a fast P2X-likedepolarization of AH neurons as was demonstratedhere.

ATP acts at a novel P2X receptor subtype

Several lines of evidence suggest that ATP activates the mucosal processes of AH neurons through a P2X receptor rather thana P2Y receptor or a P1 adenosine receptor. First, agonists activeat P2X receptors ATP and ATP- $gamma$ -S reliably elicited responses,whereas the P2Y-selective agonist 2-methylthio-ATP did not. Interestingly, $alpha$ , $beta$ -methylene ATP, which is also a P2X agonist, was only weaklyactive. Second, PPADS, a P2 receptor antagonist, blocked bothATP- and ATP- $gamma$ -S-elicited responses. Another P2 receptor antagonist,suramin, was not effective but appeared to potentiate some ATP-evokedresponses; suramin is known to block the ectonucleotidases thatcause degradation of ATP to adenosine (Ralevic and Burnstock,1998). Third, either ATP or $alpha$ , $beta$ -methylene ATP could be used todesensitize the ATP-evoked response. Finally, only relativelyhigh concentrations of ATP were effective, and the response hada short latency, suggesting a low-affinity, ligand-gated receptorsuch as the P2Xreceptor.

Barajas-Lopez et al. (1996), working with cultured myenteric neurons of unknown functional class (although they were likelyto be AH-sensory neurons), demonstrated a fast P2X-mediated currentwith several similarities in pharmacology to the receptor describedhere. For example, $alpha$ , $beta$ -methylene ATP was only a weak agonist atboth receptors, and both were insensitive to blockade bysuramin.

Together, these data suggest that ATP acts on intrinsic sensory neurons through a P2X receptor with a pharmacology not seenfor the homomeric receptors studied thus far (Burnstock and Wood,1996). Lack of a correlation with known P2X receptor types isnot unusual for native receptors, which are likely to be assembledfrom several different subunit types (Lewis et al., 1995; Torreset al., 1999; Patel et al., 2001). Recent evidence suggests thatguinea pig pelvic neurons express a P2X receptor with characteristicsnot seen in rat pelvic neurons but similar to that reported here(Zhong et al., 2001). Our findings extend this observation tothe enteric nervous system of the guinea pig and suggest thatguinea pigs may express a P2X receptor subtype with characteristicsnot seen in rat or human receptors identified to date. We concludethat myenteric AH neurons express a novel subtype of P2X receptor,the study of which should be facilitated by its presence on boththe soma andterminals.

ATP may act as a sensory mediator

In this study, we present two converging lines of evidence that ATP acts as a sensory mediator in gastrointestinal sensorytransduction: demonstration that the intrinsic sensory nerve terminalsexpress functional excitatory P2X receptors and that ATP can excitelocal reflex pathways mediating inhibition in the circular muscle.The data also suggest that enterochromaffin cells in the guineapig ileum possess excitatory P2X receptors that mediate an increasein 5-HT release (Racké et al., 1996) and that a large proportionof the sensory neurons activated by ATP are also activated by5-HT. Thus, ATP may act either directly or indirectly to excitethe mucosal terminals of intrinsic sensoryneurons.

Mucosal ATP also excites local interneurons and motor neurons and, because these neurons do not project to the mucosa, thisis presumably secondary to the activation of intrinsic sensoryneurons. The monosynaptic and polysynaptic reflexes that are initiatedcontrol the excitability of the neighboring circular muscle. ATP-evokedreflexes appear to be similar to those that would be initiatedby physiological, or pathophysiological, activation of the sensorynerve terminals by an abrupt change in the chemical environmentof the lumen, as when contents are first pushed into a new region,by distortion of the villi or by the arrival of an inflammatoryagent. This then raises the question as to what may release ATPand fromwhere.

In preliminary experiments, we found that blockade of P2X receptors in the lumen with PPADS (60 µM) had little effect on thethreshold for initiation of peristaltic reflexes by increasedluminal pressure (P. P. Bertrand, unpublished observations). Thissuggests that stretching the intestinal wall does not releasesufficient ATP to excite the mucosal P2X receptors, which contrastswith the bladder (Vlaskovska et al., 2001). This stimulus is unlikelyto excite enteroendocrine cells in the mucosa, however, so thepossibility that these cells mediate sensory transduction viaATP remains open. Interestingly, it has been suggested that theserotonin storing enterochromaffin cells do not contain ATP (Tamirand Gershon, 1990), although other types of enteroendocrine cellsmay. An alternative source of ATP would be the mast cells thatare prominent in the intestinal mucosa. Activation of these cellsmarkedly enhances intestinal motility and secretion (Cooke, 1994),making them a prime candidate for release of pathophysiologicalsensory mediators. Thus, it may be that ATP is a mediator of chemosensoryinformation or nociception in the intestine, as has been moregenerally suggested (Burnstock, 2001).

Conclusions

We found that the mucosal processes of intrinsic sensory neurons in the guinea pig small intestine generate APs in responseto ATP acting via excitatory P2X receptors. ATP released withinthe mucosa may, thus, initiate or enhance reflexes in the guineapig small intestine. ATP may be a sensory mediator in the guineapig ileum and in other gastrointestinaltissues.

  FOOTNOTES

Received Dec. 18, 2001; revised Feb. 15, 2002; accepted Feb. 15, 2002.

This work was supported by National Health and Medical Research Council (Australia) Grant 114103 and Fellowship 007703 (toP.P.B.). We thank Prof. John Furness and Prof. Marcello Costafor helpfulcomments.

Correspondence should be addressed to Dr. Paul P. Bertrand, Department of Physiology, University of Melbourne, Parkville,Victoria 3010, Australia. E-mail: p.bertrand{at}unimelb.edu.au.

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