Neuronal Expression of an FMRFamide-Gated Na+ Channel and Its Modulation by Acid pH

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The Journal of Neuroscience, August 1, 2001, 21(15):5559-5567

Neuronal Expression of an FMRFamide-Gated Na⁺ Channel and Its Modulation by Acid pH
Stephen J. Perry, Volko A. Straub, Michael G. Schofield, Julien F. Burke, and Paul R. Benjamin
Sussex Centre for Neuroscience, University of Sussex, Falmer, Brighton, BN1 9QG, United Kingdom

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The molluscan Phe-Met-Arg-Phe-amide (FMRFamide)-gated sodium channels (FaNaCs) show both structural and functional similaritiesto the mammalian acid-sensing ion channels (ASICs). Both channeltypes are related to the epithelial sodium channels and, althoughthe neuropeptide FMRFamide directly gates the FaNaCs, it alsomodulates the proton-gating properties of ASICs. It is not yetknown whether protons can alter the gating properties of the FaNaCs.We chose to examine this possibility at a site of FaNaC expressionin the nervous system of the mollusk Lymnaea stagnalis. We cloneda putative L. stagnalis FaNaC (LsFaNaC) that exhibited a highdegree of sequence identity to the Helix aspersa FaNaC (HaFaNaC,60%), and a weaker homology to the ASICs (ASIC3, 22%). In situhybridization was used to map the LsFaNaC expression pattern inthe brain and to identify the right pedal giant1 (RPeD1) neuronas a site where the properties of the endogenous channel couldbe studied. In RPeD1 neurons isolated in culture, we demonstratedthe presence of an FMRFamide-gated sodium current with featuresexpected for a FaNaC: amiloride sensitivity, sodium selectivity,specificity for FMRFamide and Phe-Leu-Arg-Phe-amide (FLRFamide),and no dependency on G-protein coupling. The sodium current alsoexhibited rapid desensitization in response to repeated FMRFamideapplications. Lowering of the pH of the bathing solution reducedthe amplitude of the FMRFamide-gated inward current, while alsoactivating an additional sustained weak inward current that wasapparently not mediated by the FaNaC. Acidification also preventedthe desensitization of the FMRFamide-induced inward current. Theacid sensitivity of LsFaNaC is consistent with the hypothesisthat FaNaCs share a common ancestry with theASICs.

Key words: Lymnaea; FMRFamide-gated Na⁺ channel; pH sensitivity; ASIC; epithelial Na⁺ channel; amiloride; degenerin; cell culture

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The neuropeptide Phe-Met-Arg-Phe-amide (FMRFamide) and related peptides have diverse physiological effects, such as regulatingheart rate in mollusks (Price et al., 1987), controlling movementin Caenorhabditis elegans (Nelson et al., 1998), and pain modulationin vertebrates (Yang et al., 1985; Waldmann and Lazdunski, 1998).It is believed that in most instances FMRFamide and related neuropeptideswork via G-protein-coupled receptors and second messengers (Higginset al., 1978; Colombaioni et al., 1985; Piomelli et al., 1987;Willoughby et al., 1999a,b). However, in neurons of the snailHelix aspersa it has also been demonstrated that FMRFamide canelicit excitatory effects without activating G-proteins (for review,see Cottrell, 1997). FMRFamide application to these cells directlygated sodium channels with pharmacological properties similarto those of the mammalian epithelial sodium channels (ENaCs):they were highly selective for sodium ions, blocked by amilorideand related drugs, and were insensitive to blockers of other sodiumion channel types. Subsequently, a cDNA encoding an ENaC-relatedchannel was cloned from H. aspersa brain RNA (Lingueglia et al.,1995). Heterologous expression of the channel led to the formationof homotetramers (Coscoy et al., 1998) that responded to bothFMRFamide and Phe-Leu-Arg-Phe-amide (FLRFamide) and hence wasidentified as the H. aspersa FMRFamide-gated sodium channel(HaFaNaC).

Screening of the mammalian CNS for FaNaC homologs identified several new members of the degenerin subgroup of ENaCs that showmore sequence identity to FaNaC than do the prototypical ENaCs(García-Añoveros et al., 1997; Waldmann et al., 1997a,b; Chenet al., 1998). These new mammalian channels were gated by decreasesin extracellular pH [acid-sensing ion channels (ASICs)], and theexpression of some forms in dorsal horn sensory neurons led tothe suggestion that they may be important in nociception resultingfrom acidosis during inflammation (Waldmann and Lazdunski, 1998).Not only were the ASICs somewhat similar in structure to the FaNaCs,but a recent report has demonstrated that many were also modulatedby FMRFamide and the structurally related mammalian peptides neuropeptideFF (NPFF) and neuropeptide AF (NPAF) (Askwith et al., 2000). Preapplicationof the peptides to dorsal root ganglion sensory neurons or tothe heterologously expressed channels increased the duration ofthe acid-induced inward current by reducing the rate of inactivation,often producing sustainedresponses.

It has yet to be investigated whether the FaNaCs expressed in molluscan neurons show sensitivity to acid pH, as might be predictedby analogy to ASICs. To study this we set out to identify neuronsendogenously expressing an FaNaC in the snail Lymnaea stagnalis.Although FaNaCs have been isolated from two molluscan species[Helix aspersa (HaFaNaC) (Lingueglia et al., 1995) and Helisomatrivolvis (HtFaNaC) (Jeziorski et al., 2000)], the expressionof the FaNaC gene in identified neurons has not been demonstrateddirectly in either of them. Here, we describe the cloning of theL. stagnalis FaNaC (LsFaNaC) and its widespread expression throughoutthe brain, including in the readily identifiable giant RPeD1 interneuron.RPeD1 cells were subsequently isolated in culture and used tostudy the peptide and acid sensitivities of the endogenousLsFaNaC.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Experimental subjects and chemicals. Adult specimens of Lymnaea stagnalis were obtained from Blade Biological (Kent, UK).The animals were kept in large holding tanks containing copper-freewater on a 12 hr light/dark cycle and fed lettuce three timesaweek.

All chemicals were purchased from Sigma (Poole, UK) unless otherwisestated.

Cloning of Lymnaea FMRFamide-gated sodium channel. PCR primers identical to nucleotides 84-105 and 1961-1940 of the HaFaNaCopen reading frame (GenBank accession number X92113) were usedto amplify by PCR the entire coding region from the Helix clone(gift of M. Lazdunski). A radiolabeled product was made by replacementof dCTP with $alpha$ [³²P]dCTP in the reaction mix, and this was used as a hybridizationprobe in the screening of 2 million phages of a Lymnaea stagnalisbrain cDNA library (previously described in Vreugdenhil et al.,1988). Three clones were isolated to homogeneity by a furthertwo rounds of screening at high stringency (washes performed with0.2× SSC, 0.1% SDS at 60°C). DNA from the phages was purified,and inserts were sequenced on both strands using dye-terminatorreaction kits following the manufacturer's instructions (Perkin-Elmer,Boston,MA).

In situ hybridization. The protocols for 7 µm tissue section preparation and biotinylated complementary oligonucleotide insitu hybridization were adhered to as previously described (Kellettet al., 1996), using a mixture of 15 different 21-25 mer oligonucleotidesas the probe. Negative control hybridizations using a mixtureof the complementary (sense) oligonucleotide sequences were performedunder identicalconditions.

Gene expression detection by RT-PCR. Total cellular RNA was isolated from various Lymnaea tissues using an RNA preparationkit (Qiagen, Bothell, WA) following the manufacturer's instructions.One microgram of each RNA was used in reverse transcription reactionswith random hexamers and 10 U of Moloney murine leukemia virusreverse transcriptase (Promega, Madison, WI). The samples werethen used as templates in PCR with primers designed to nucleotides3001-3025 and 3891-3865 of the Lymnaea FMRFamide-gated sodiumchannel gene (LsFaNaC; GenBank accession number AF335548) toamplify an 890 bp product. Samples were separated on a 1% agarosegel, and the identity of bands of the correct size was confirmedby hybridization to a radiolabeled PCR product of the entire 3'untranslated region(UTR).

Dissection. All dissections were performed in HEPES-buffered saline containing (in mM): 50 NaCl, 1.6 KCl, 2 MgCl₂, 3.5 CaCl₂,and 10 HEPES, pH 7.9, in distilled water. The CNS, consistingof the circumesophageal ganglionic ring (cerebral, pedal, pleural,parietal, and visceral ganglia) and the buccal ganglia togetherwith a short stretch of esophagus, was isolated from the snail.The preparation was pinned down in a Sylgard-coated dish filledwith HEPES-buffered saline with the dorsal surface facingup.

Isolation and culture of RPeD1 neurons. The cell culture procedure was modified after the protocol of Ridgway et al. (1991).Media used included normal saline (NS), antibiotic saline (ABS),defined medium (DM), and conditioned medium (CM). Normal salineused in cell culture experiments contained the same salt concentrationsas HEPES-buffered saline described above but was made up in culturegrade water (Sigma), whereas ABS also contained gentamycin (150µg/ml). DM was prepared by mixing 100 ml of special L-15 medium(Life Technologies, Paisley, UK), 80 ml of NS, and 120 ml of culturegrade water and by adding glutamine (30 mg), glucose (16.2 mg),and gentamycin (600 µl of 10 mg/ml stock) to the solution. ForCM preparation, isolated brains that had been washed extensivelyin ABS were incubated in DM (two brains per milliliter). After3 d of incubation, the CM was filter sterilized (Millex-GV, 0.22µm; Millipore, Bedford, MA). Aliquots of CM (1 ml) were pipetteddirectly onto culture dishes (Falcon 3001; Becton Dickinson, Rutherford,NJ) coated with poly-L-lysine [15-30 kDa; 1 mg/ml in 15 mM Tris(hydroxymethyl)aminomethane)],and equal amounts of DM were added. The culture dishes were storedat $-$ 20°C and thawed 2-3 hr beforeuse.

The isolation of RPeD1 neurons was performed in a laminar flow cabinet after the isolated nervous system was first incubatedfor 45 min in a protease solution (Sigma type VIII, 1 mg/ml inNS) followed by washing in ABS. Subsequently, the isolated nervoussystem was pinned out in a dissection dish filled with high-osmolarityDM (30 mM glucose in DM). The RPeD1 neuron was visually identifiedaccording to its large size and characteristic position in theright pedal ganglion. Its cell body was exposed by mechanicallydisrupting the inner connective tissue and then removed, togetherwith a short stretch of its main process, by gentle suction witha Sigmacote-coated, fire-polished micropipette (tip diameter,150-200 µm) prepared from 1.5 mm glass tubing (GC150T-10; ClarkElectromedical Instruments, Reading, UK). After isolation, neuronswere transferred onto culture dishes and cultured at 20°C forup to 5d.

Electrophysiological and pharmacological studies on cultured neurons. For intracellular recordings from isolated RPeD1 neurons,culture dishes containing isolated neurons were placed on thestage of an inverted microscope (Nikon Diaphot) that was equippedwith a custom-built, gravity-fed perfusion system. Cells wererecorded after 1-3 d in culture, and no changes were seen in theelectrical properties of the cells during this period. The culturedishes were perfused with NS at a flow rate of 1-2 ml/min forat least 30 min before the experiment to remove all culture medium.The perfusion was maintained throughout the experiment. RPeD1cell bodies were impaled with one or two microelectrodes pulledfrom 1 mm capillaries (GC100F-10; Clark Electromedical Instruments)and filled with saturated potassium sulfate (tip resistance, 20-30M $Omega$ ). The intracellular signals were amplified using an AXOCLAMP2-Bamplifier (Axon Instruments), output to a storage oscilloscope(5115 Tektronix), and stored on a DAT recorder (Biologic DTR-1801,Biological Science Instruments, Claix, France). Amplified signalswere also digitized using a DigiData 1200 interface (Axon Instruments)and stored on a personal computer. Intracellular recordings wereeither performed in bridge or twin electrode voltage clamp (TEVC)mode of the AXOCLAMP 2B amplifier controlled by pClamp6 software(Axon Instruments) via the DigiData 1200interface.

The effects of FMRFamide (0.1 mM), FLRFamide (0.1 mM), and Ser-Asp-Pro-Phe-Leu-Arg-Phe-amide (SDPFLRFamide) (0.1 mM) weretested by focal application from a micropipette (1 sec pulsesat 6-12 psi) using a Picospritzer (General Valve, Fairfield, NJ).Amiloride, a selective antagonist for peptide gated Na⁺ channels, was applied by including it in the perfusion solutionat a concentration of 0.1 mM. Na⁺ substitution experiments were performed by replacing 90% of theNaCl in NS with N-methyl-D-glucamine (low Na⁺ saline). Pipette solutions for the pressure injection of GDP- $beta$ -Sto test for G-protein-coupled responses contained GDP- $beta$ -S (2 mM),KCl (40 mM), and Fast Green (0.1%) in culture grade distilledwater (Sigma). The solution was injected into the soma of isolatedRPeD1 neurons by applying 500 msec pressure pulses (15 psi) at1 Hz. The injection was stopped when the soma showed a clear greenstaining (this usually occurred within 1 min from the start ofthe injection). The effects of pH on RPeD1 neurons and the FMRFamide-inducedinward current in these neurons were studied by either focal applicationor bath application of saline at pH values of 5.2, 6.0, 6.7, 6.8,and 9.0 in addition to HEPES-buffered saline at pH 7.9. All salinesolutions had the same salt concentration as HEPES-buffered saline,pH 7.9 and pH 6.8, but were buffered with 5 mM 2-(4-morpholino)-ethansulfonicacid (MES), pH 5.2, 6.0, and 6.7, or 5 mM Tris, pH 9.0, insteadofHEPES.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cloning of a Lymnaea homolog of the FMRFamide-gated sodium channel

Screening of 2 million phages from a Lymnaea stagnalis CNS cDNA library, using a radiolabeled PCR product encoding the HaFaNaC,identified three positive clones. Sequencing of the clones revealedthat all three encoded an identical 4872 bp cDNA that showed anoverall 60% identity to the Helix sequence (GenBank accessionnumber X92113). An open reading frame (residues 767-2662) encodinga 71.5 kDa protein (GenBank accession number AF335548) (Fig.1), exhibited 60% identity to the Helix protein and 66% to theHelisoma protein. The open reading frame was flanked by 5' and3' untranslated regions of 766 and 2211 bp, respectively. Comparisonof the open reading frame start point with that of the Helix andHelisoma clones showed that LsFaNaC shares a 31 residue N-terminalextension with HtFaNaC that appears to be absent in HaFaNaC. Furtherscreening of the brain cDNA library by PCR revealed no evidencefor related genes or alternatively spliced mRNAs that could encodevariants of LsFaNaC.

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Figure 1. Comparison of FMRFamide-gated sodium channels (FaNaCs) from Lymnaea stagnalis, Helix aspersa, and Helisoma trivolvis (GenBank accession numbers AF335548, X92113, and AF254118, respectively). Alignment of the protein sequences predicted from translation of open reading frames of cDNA sequences. Amino acids conserved in all three FaNaCs are highlighted in black, and those found in only two are highlighted in gray. Numbering on the right represents equivalent amino acid positions within the clones (taking the published start methionine for X92113 as position 1). Overlining shows positions of predicted transmembrane domains. Amino acids of the mammalian epithelial sodium channel $alpha$ subunit ( $alpha$ ENaC, GenBank accession number NM001038) and ASIC3 (GenBank accession number AF013598) that are conserved in two or more FaNaCs are shown below.

Structural predictions from the primary amino acid sequence suggested a protein with two transmembrane spanning domains (residues93-111 and 551-571), a cysteine-rich extracellular loop, and intracellularN- and C-terminal domains. The extracellular loop contained sevenpredicted N-glycosylation signals, five of which were conservedin the Helix protein and two in all members of the superfamily.The loop also contained 15 cysteine residues, 14 of which areconserved in the Helix protein and up to 11 in more distantlyrelated members of the superfamily. The N-terminal domain containedphosphorylation sites for protein kinase C and casein kinase II,as did the C terminus, which also contains a site for proteinkinase A. This structure is topologically identical to that predictedfor all the members of the amiloride-sensitive epithelial sodiumchannels. Comparison of the amino acid sequence to other membersof the superfamily revealed identities of between 15% [mammalianepithelial sodium channels, $alpha$ ENaC (human): GenBank accession numberNM001038] and 22% [mammalian dorsal root acid-sensing ion channel,ASIC 3 (rat): GenBank accession number AF013598] with highesthomology in the region covering the predicted second transmembranedomain (up to 46%).

Expression of LsFaNaC in neuronal and other tissues

Reverse transcription PCR was used to identify Lymnaea tissues where LsFaNaC is expressed (Fig. 2). Reactions performed ontotal RNA isolated from a number of tissues revealed a widespreaddistribution of the channel. Especially high levels of expressionwere detected in the brain, heart, and pedal tissue. Only thebrain and heart have been shown previously to definitely containFMRFamide (Ebberink et al., 1987; Buckett et al., 1990a,b), althoughthere is immunocytochemical evidence for FMRFamergic innervationof the pedal muscle (Schot and Boer, 1982). Low levels of expressionwere detected in the buccal mass, and no expression was detectedin the esophagus.

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Figure 2. Tissue distribution of LsFaNaC expression in Lymnaea. Reverse transcription-PCR reactions that used primers specific for a region within the 3' UTR of the LsFaNaC cDNA were performed on total RNA derived from five tissues. Products of the correct size (890 bp) were separated by gel electrophoresis, transferred to a nylon filter, and visualized by hybridization with a radiolabeled probe of the identical region of the 3' UTR. Products were detected in CNS, buccal mass, heart, and pedal muscle, but not in esophagus. The control reaction was performed in an identical manner to the CNS reaction, except reverse transcriptase enzyme was omitted.

In situ analysis of identified neuron expression

In situ analysis of the distribution of the LsFaNaC gene was performed on the serially sectioned CNS (n = 4). More than 400neurons consistently expressed the gene with staining presentin several previously identified giant neurons (Fig. 3). Prominentamong these was RPeD1, a dopamine-synthesizing member of the respiratorycentral pattern generator network of Lymnaea (Fig. 3A, arrow)(Syed et al., 1990). A bilaterally symmetrically located but smalleridentifiable cell, LPeD1 (Slade et al., 1981), which containsserotonin (Kemenes et al., 1989) was also stained in the oppositeleft pedal ganglia (data not shown) together with large clustersof medial cells of a wide variety of sizes (Fig. 3A). The expressionof LsFaNaC in RPeD1 was consistent with an electrophysiologicalstudy in the closely related snail Helisoma, where the homologouscells GDN (giant dopaminergic neuron) showed fast inward currentsin response to FMRFamide application (Jeziorski et al., 2000).

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Figure 3. Expression of the LsFaNaC in the Lymnaea CNS using in situ hybridization. A, Section through the paired pedal ganglia showing staining of the identified neuron RPeD1 (arrow). B, A cluster of light yellow cells in the right parietal ganglion. C, Expression in a cerebral giant cell (arrow), a modulatory interneuron of the feeding network. Scale bars, 100 µm.

Two serotonin-containing modulatory neurons of the feeding network, the cerebral giant cells (Fig. 3C, arrow) (McCrohan andBenjamin, 1980) were also stained as well as adjacent smallercells in the anterior lobes of the cerebral ganglia. There wereclusters of stained large neurons in the right parietal (Fig.3B) and visceral ganglion. Some of these correspond to the LightYellow Cells that are peptidergic neurons likely to be involvedin ion and water regulation (Boer and Montagnewajer, 1994). Smallernumbers of in situ-positive cells occurred in the left parietal,left, and right pleural ganglia with just two pairs of small unidentifiedcells in the buccal ganglia (data not shown), the main feedingganglia of the snail (Benjamin, 1983). These results showed thatthe LsFaNaC is widely distributed in neurons located in a numberof different types of behavioralnetworks.

Electrophysiological characterization of the LsFaNaC

The in situ hybridization study showed that the dopaminergic neuron RPeD1, located in the right pedal ganglion, expressesmRNA for the Lymnaea homolog of the HaFaNaC. This neuron, whichis easy to identify because of its large size, was used for studyingthe LsFaNaC. Isolated RPeD1 neurons in cell culture respond toFMRFamide with an initial fast depolarization followed by a slowhyperpolarization (1 sec pressure pulses; pipette FMRFamide; 0.1mM; n > 30 cells) (Fig. 4A). This was similar to the FMRFamideresponses described previously for RPeD1 in the intact nervoussystem (Skingsley et al., 1993) and in the homologous giant dopaminergicneuron in the pedal ganglia of Helisoma (Jeziorski et al., 2000).The fast depolarizing response was likely to be the response mediatedby the FaNaC. Consistent with this was the weaker response obtainedwith FLRFamide (n = 4 cells) and the absence of a depolarizingresponse to the N-terminally extended peptide SDPFLRFamide (n= 4 cells) applied at the same concentrations (Fig. 4A). Thisagonist selectivity was typical of the HaFaNaC (Cottrell, 1997).FLRFamide and SDPFLRFamide both elicited the hyperpolarizing componentof the response seen with FMRFamide. This hyperpolarizing responseto FMRFamide could be blocked by the injection of the generalG-protein blocker GDP- $beta$ -S into RPeD1 (Fig. 4B) (n = 6 cells),suggesting the presence of a G-protein-coupled receptor. The depolarizingresponse to FMRFamide was not blocked, but in fact was consistentlyenhanced (Fig. 4B), presumably because of the removal of the initialpart of the hyperpolarizing current that had a similar onset tothe LsFaNaC response.

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Figure 4. Responses of isolated RPeD1 neurons to focal application of FMRFamide, FLRFamide, and SDPFLRFamide. A, Responses of a single isolated RPeD1 neuron to focal 1 sec applications of FMRFamide, FLRFamide, and SDPFLRFamide (pipette concentration, 0.1 mM each) recorded under current clamp. B, FMRFamide responses (pipette concentration, 0.1 mM) recorded in a RPeD1 neuron before (control) and after the intracellular injection of the G-protein blocker GDP- $beta$ -S. Note the increase in the FMRFamide-induced depolarization and the block of the delayed hyperpolarizing response after the injection of GDP- $beta$ -S. C1, D1, Voltage dependence of FMRFamide responses (pipette concentration, 0.1 mM) in two different RPeD1 cells recorded under current-clamp conditions. The neuron in C1 showed an exclusively depolarizing response to FMRFamide application, whereas the neuron in D1 displayed a biphasic response that consisted of an initial depolarization followed by a delayed hyperpolarization. The hyperpolarizing component readily reversed when the membrane potential was adjusted to values more negative than $-$ 70 mV. C2, D2, TEVC recording of series of FMRFamide responses in the same two neurons shown in C1 and D1, respectively. In C2, the holding potential was stepped from $-$ 90 to $-$ 20 mV in 10 mV increments, whereas holding potentials in D2 were between $-$ 120 and $-$ 50 mV.

To characterize the LsFaNaC in more detail, FMRFamide responses were recorded in isolated neurons using two-electrode voltageclamp. Brief focal application of FMRFamide caused a fast inwardcurrent with a time course that resembled the fast depolarizationobserved under current clamp. The fast inward current was followedby an outward current at holding potentials more positive than $-$ 70 mV that varied in amplitude between individual neurons (Fig.4, compare D2, C2). The delayed outward current hindered an accuratedetermination of the reversal potential for the fast inward currentin some neurons. However, in RPeD1 neurons with weak or no delayedoutward currents, the fast inward current dominated the responseat the tested holding potentials, allowing the reversal potentialto be determined more accurately (Fig. 4C2). In these cells, theamplitude of the inward current increased linearly at holdingpotentials between $-$ 20 and $-$ 90 mV. Responses were not tested atmore positive holding potentials because of the strong activationof voltage-gated outward currents. The reversal potential wasfound to be +40 ± 7 mV (n = 11 cells) by linear extrapolation(Fig. 4C2, insert).

Evidence that Na⁺ carried the fast inward current was provided by ion substitution experiments under voltage clamp. Replacing90% of the Na⁺ ions in normal saline with N-methyl-D-glucamine (low Na⁺ saline) caused a major reduction in the FMRFamide-induced inwardcurrent (Fig. 5A). The maximum reduction in the amplitude of theinward current was 90% with a mean reduction of 67 ± 6% (n = 6experiments performed on four cells) (Fig. 5B). The use of lowNa⁺ saline also caused a shift in the reversal potential of the fastinward current by 58 mV to $-$ 18 ± 8 mV (n = 4). This value wasidentical to the predicted value based on the reversal potentialin normal saline and the hypothesis that the fast inward currentwas predominantly carried by Na⁺ ions (Lingueglia et al., 1995). Exchanging the low Na⁺ saline for normal saline reversed the reduction in the peak amplitudeof the fast inward current caused by replacement of 90% of theNa⁺ ions (mean recovery, 96 ± 13%).

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Figure 5. Sodium dependence and amiloride block of FMRFamide induced inward currents in isolated RPeD1 neurons. A, Replacing 90% of the extracellular Na⁺ concentration with N-methyl-D-glucamine resulted in the reduction of the peak FMRFamide-induced (pipette concentration, 0.1 mM) inward current recorded under TEVC (holding potential, $-$ 100 mV) from $-$ 0.7 nA (control) to $-$ 0.17 nA (low Na). Returning the extracellular Na⁺ concentration to 50 mM (wash) reversed the effect. B, Summary of six sodium replacement experiments conducted on four cells. Reducing the extracellular Na⁺ concentration significantly reduced the mean peak amplitude of the FMRFamide-induced inward current to 33 ± 6% of the control value (paired t test: p < 0.001). The mean peak amplitude returned to 96 ± 12% of the control value, when the extracellular Na⁺ concentration was raised again to 50 mM. C, Application of amiloride (0.1 mM) decreased the FMRFamide-induced (pipette concentration, 0.1 mM) inward current recorded under TEVC (holding potential, $-$ 100 mV) from $-$ 1.6 nA (control) to $-$ 0.3 nA (amiloride). The block was almost completely reversed after wash-out of amiloride from the bath. D, Summary of three amiloride blocking experiments. Amiloride application blocked a significant proportion of the FMRFamide-induced inward current, reducing the mean peak amplitude to 35 ± 9% of the control value (paired t test; p < 0.05). The amiloride block was reversible, and the mean peak amplitude returned to 92 ± 10% after wash-out of amiloride from the bath. *p $<=$ 0.05; ***p $<=$ 0.001.

Bath application of amiloride (0.1 mM) to the Lymnaea neuron also caused a 65 ± 16% reduction in the fast inward current evokedby FMRFamide pulses in isolated RPeD1 neurons (n = 3 cells) (Fig.5C,D). The block of the inward current was almost completely reversed(mean recovery, 93 ± 10%) after washout of the amiloride solution(Fig. 5D).

Modulation of the FMRFamide response by acidic pH

The molecular and electrophysiological characterization of the LsFaNaC clearly demonstrated that it is a member of the Degenerin/ENaCfamily (DEG/ENaC) family of channels that also includes the H⁺-gated ASIC channels that are expressed in sensory neurons ofthe mammalian dorsal root ganglia. The molecular relationshipbetween these channels raised the question of whether protonsalso gate the LsFaNaC. The application of 1 sec pulses of NS bufferedat pH 5.2 caused a very small inward current (mean amplitude, $-$ 0.04 ± 0.01 nA; n = 4 cells) in isolated RPeD1 neurons in cellculture, which was considerably weaker than FMRFamide responsesin the same neuron (Fig. 6A). However, the pH 5.2-induced currentwas unlikely to be mediated by the LsFaNaC, because its reversalpotential ( $-$ 39 ± 2 mV; n = 4 cells) was significantly more negativethan that of the FMRFamide-induced current (+40 mV, see above).Furthermore, the I-V relationship for the pH 5.2-induced inwardcurrent showed some rectifying behavior at holding potentialsmore negative than $-$ 40 mV (Fig. 6B), which was not seen in theI-V relationship for the FMRFamide-induced inward current.

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Figure 6. Effect of pH 5.2 acidification on FMRFamide-induced inward current in isolated RPeD1 neurons. A, Response of a RPeD1 neuron to focal application of a 1 sec pulse of saline at pH 5.2 recorded under TEVC (trace labeled pH 5.2; holding potential, $-$ 100 mV). The pH 5.2 pulse caused a very weak transient inward current. A record of an FMRFamide-induced inward current (1 sec pulse; pipette concentration, 0.1 mM) in the same neuron is shown for comparison. B, Mean I-V plot for the pH 5.2-induced inward current in four RPeD1 cells recorded under TEVC. C, Series of FMRFamide-induced inward currents (pipette concentration, 0.1 mM; holding potential, $-$ 100 mV) recorded in a RPeD1 neuron while bathed in saline buffered at pH 7.9 or pH 5.2. D, Summary of the effects of bath pH on the amplitude of FMRFamide-induced inward currents in RPeD1 neurons. Statistical analysis revealed that the reduction by acidification to pH 5.2 was significant compared with values at pH 6.7, 6.8, and 7.9 [ANOVA: F_(5,39) = 8.982, p < 0.001; followed by pairwise comparisons using post hoc Tukey honestly significant difference (HSD) tests giving p values $<=$ 0.001]. The differences between all other pairs of pH values were not statistically significant (Tukey HSD tests: p values between 0.08 and 0.99).

Despite the lack of evidence for direct H⁺-gating of the LsFaNaC, altering the pH of the medium had significant modulatoryeffects on the FMRFamide-activated currents in isolated RPeD1neurons. This was demonstrated by comparing the responses to 1sec FMRFamide pulses in saline buffered at pH 7.9 (normal saline)with FMRFamide-induced currents in salines buffered at pH 5.2,6.0, 6.7, 6.8, and 9.0. Acidification of the medium to pH 5.2had the most dramatic effect and reversibly reduced the peak amplitudeof the FMRFamide-induced inward current to 57 ± 8% (n = 11 cells)of its control value at pH 7.9 (Fig. 6C,D). Saline at pH 6.0 hada weaker blocking effect, reducing the peak amplitude to 74 ±8% (n = 5 cells), whereas pH 6.7 and pH 6.8 medium had no apparenteffect on the FMRFamide-gated current (98 ± 6% and 96 ± 6%; n= 6 cells each) (Fig. 6D). A reduction in the peak amplitude ofthe FMRFamide-gated current to 75 ± 9% (n = 6 cells) of its controlvalue was also observed when the medium was adjusted to an alkalinevalue of pH 9.0.

The most dramatic effect of acidification of the medium, however, was a reduction in the desensitizing effects of repeatedapplications of FMRFamide (Fig. 7). At normal pH (7.9), desensitizationwas strong at intervals of 15 sec between successive 1 sec pulsesof FMRFamide in a six pulse train, less at 30 sec, and not significantat 60 sec intervals (Fig. 7A). Most of the reduction in responseoccurred between the first and second applications of FMRFamide(Fig. 7C). After acidification of the medium to pH 5.2, no reductionin the amplitude of the response could be detected at 30 sec intervals,and at 15 sec the desensitization was significantly reduced whencompared with FMRFamide applications at 15 sec intervals at pH7.9 (Fig. 7B,C).

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Figure 7. Desensitization of FMRFamide-induced inward currents in RPeD1 neurons by repeated applications at 60, 30, and 15 sec intervals in bath media at pH 7.9 and pH 5.2. A, B, Sample records of series of inward currents (holding potential, $-$ 100 mV) induced in the same RPeD1 neuron by six repeated FMRFamide pulses (1 sec, pipette concentration, 0.1 mM) at intervals of 60, 30, and 15 sec in bath media buffered at pH 7.9 (A) and pH 5.2 (B). Note the substantial desensitization at 15 sec intervals and to a lesser extent at 30 sec intervals in pH 7.9. In contrast, desensitization was weak at 15 sec intervals and absent at 30 sec intervals in pH 5.2. C, Summary of the desensitization data obtained from six individual RPeD1 neurons. Each neuron was tested for desensitization in response to series of six FMRFamide pulses applied at 60, 30, and 15 sec intervals in bath media at pH 7.9 and pH 5.2. The graphs clearly illustrate the difference in desensitization observed in pH 7.9 and pH 5.2. Pairwise comparison between mean peak amplitude values at 15 sec application intervals showed that these values for trials 2-6 were significantly larger in pH 5.2 than in pH 7.9 (t tests; p values 0.001-0.004). Similarly, at 30 sec application intervals, these values were significantly larger in pH 5.2 than in pH 7.9 for trials 3-6 (t test; p values 0.03-0.05). The small differences in desensitization at 60 sec application intervals in pH 5.2 and pH 7.9 were not significant. *p $<=$ 0.05; **p $<=$ 0.01; ***p $<=$ 0.001.

A second set of experiments was performed to study the effect of a wider range of pH changes on the level of desensitizationto repeated FMRFamide pulses. The same protocol that producedthe maximum desensitization in the previous experiment in HEPES-bufferedsaline at pH 7.9 (i.e., a train of six FMRFamide pulses at 15sec intervals) was applied, whereas the bath medium was exchangedfor salines buffered at pH 6.8 (HEPES-buffered), pH 5.2, 6.0,and 6.7 (all MES-buffered), and pH 9.0 (Tris-buffered). At pH7.9, the response to repeated FMRFamide pulses again showed rapiddesensitization, and the peak amplitude of the sixth FMRFamide-inducedinward current was reduced to 43 ± 9% (n = 6 cells) of the correspondingfirst response in the series (Fig. 8). The level of desensitizationwas statistically similar at bath pH values of 9.0, 6.8, 6.7,and 6.0 with responses to the sixth FMRFamide application beingreduced to between 28 ± 6% (pH 6.8; n = 6 cells) and 46 ± 9% (pH6.0; n = 5 cells) of their corresponding control values (Fig.8). A significant reduction in desensitization was observed onlywhen the bath medium was acidified to pH 5.2. Under these conditions,the amplitude of the last response within a series of six FMRFamidepulses was still 85 ± 9% (n = 6 cells) of the first response (Fig.8), which is comparable with the result of the previous experiment(Fig. 7B).

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Figure 8. Effects of various bath pH values on desensitization in isolated RPeD1 neurons. Isolated RPeD1 neurons were exposed to series of six FMRFamide pulses (pipette concentration, 0.1 mM, 1 sec) at 15 sec intervals, and the induced inward currents were measured under TEVC (holding potential, $-$ 100 mV) in bath media buffered at pH 5.2, 6.0, and 6.7 (MES-buffered), 6.8 and 7.9 (HEPES-buffered), and pH 9.0 (Tris-buffered). The amplitude of the sixth response in each series was expressed as a percentage of the first response, and the mean values for each experiment were plotted against the pH. A statistical analysis revealed that acidification of the bath medium to pH 5.2 significantly reduced desensitization of the FMRFamide-induced inward current compared with all other pH values tested (ANOVA: F_(5,29) = 8.684, p < 0.001, followed by post hoc Tukey HSD tests for pairwise comparison; p $<=$ 0.01 for all pairs; **p $<=$ 0.01, ***p $<=$ 0.001). These tests also showed that none of the differences between the desensitization levels at pH 6.0, 6.7, 6.8, 7.9, and 9.0 were significant (Tukey HSD tests; p values > 0.5).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Comparison of the structure of LsFaNaC with other members of the ENaC superfamily of sodium channels revealed many commonfeatures. The structure of all the channels was predicted to bethat of a protein with two membrane-spanning domains with boththe N- and C-terminal domains located within the cell. The mostconservation of sequence between all the ENaCs was found in thetransmembrane domains, especially the second domain that is knownto form the pore of the channel. Mutations within this regionlead to altered or lost ion selectivity and amiloride sensitivity(Lingueglia et al., 1995). LsFaNaC shows 93 and 98% sequence identitywith HaFaNaC and HtFaNaC, respectively, in these regions and upto 46% identity with the more distantly related ENaCs, indicatingthat LsFaNaC was indeed a member of this channel superfamily.In both LsFaNaC and HtFaNaC the intracellular N-terminal domaincontained a 31 residue extended sequence lacking in HaFaNaC. WhereasJeziorski et al. (2000) reported that alternative splicing occurswithin this region of HtFaNaC, they concluded that the likelysite of translational initiation is that predicted by comparisonto the sequence of HaFaNaC. Conservation of this N-terminal extensionin LsFaNaC, however, would suggest that in both Lymnaea and Helisomathe channel used an alternative start codon. Because this sequencealso contains potential phosphorylation sites for several serine-threonineprotein kinases, such alternative translational initiation mayresult in differences in regulation of thechannels.

In situ hybridization allowed the identification of many neurons expressing LsFaNaC, including the giant dopaminergic neuronRPeD1. Previous work had shown that this neuron displays a fastdepolarizing response to FMRFamide application, as would be predictedfor a neuron expressing an FMRFamide-gated Na⁺ channel (Skingsley et al., 1993). In cell culture, applicationof FMRFamide induced an inward current in isolated RPeD1 neuronsthat showed the characteristics of a current that is mediatedby a member of the DEG/ENaC superfamily (i.e., reversal potentialclose to the estimated Na⁺ reversal potential, high selectivity of the channel for Na⁺ ions, block byamiloride).

A very similar current was described recently in the giant dopaminergic neuron (GDN) in Helisoma (Jeziorski et al., 2000),which is homologous to the RPeD1 neuron in Lymnaea (Harris andCottrell, 1995). The same authors also conducted a detailed comparisonbetween the neuronal FMRFamide-induced currents in GDN neuronsin the isolated nervous system and FMRFamide-induced currentsin oocytes expressing the HtFaNaC. They found only minor differencesand concluded that the heterologously expressed channel trulyresembles the neuronal channel present in GDN, although they providedno direct evidence for the expression of the HtFaNaC gene in GDNneurons. Considering the strong sequence homology between HtFaNaCand LsFaNaC and the homology between GDN (Helisoma) and RPeD1(Lymnaea), it would be reasonable to expect very similar resultsfor the heterologous expression of theLsFaNaC.

The molecular relationship between ASICs in mammals and FaNaCs in mollusks prompted us to study the effects of pH changeson FaNaCs. Although acidification of the medium appeared to beunable to directly open the LsFaNaC, it had considerable effectson the characteristics of the FMRFamide-induced current. First,acidification of the medium caused a pH-dependent block of theFMRFamide-gated inward current at pH < 6.0. Some blocking effectswere also observed when the medium was adjusted to an alkalinevalue of pH 9.0. These results are consistent with effects describedfor the heterologously expressed HaFaNaC (Price and Price, 2000)and more generally with structurally diverse channel types inwhich changes in extracellular pH can have widely varying outcomes(Hille, 1992; Pasternack et al., 1992; Traynelis, 1998; McLatchieand Bevan, 2001; Shah et al., 2001). Second, acidification topH 5.2 reduced the desensitization of the response of LsFaNaCto repeated applications of FMRFamide. This is of particular interestbecause it has been reported recently that application of FMRFamideto the mammalian ASICs substantially reduces their inactivationrate in response to acidification of the medium. This modulationof the ASICs was interpreted as evidence that the peptide-bindingsite has been at least partially conserved between FaNaC and theASICs (Askwith et al., 2000). Taking this into account, togetherwith the structural similarity of FaNaCs and ASICs and our demonstrationthat the rate of desensitization of LsFaNaC is modulated by pHchanges, it would suggest that not only is the peptide-bindingsite likely to be conserved between FaNaCs and ASICs, but alsothe proton-sensing site. It has been proposed that the weaklyconserved region immediately following the last cysteine in theextracellular domain of FaNaC may represent the peptide-bindingsite, because this region is absent from the other, peptide-insensitivefamily members (Jeziorski et al., 2000). In light of the recentdiscovery that ASICs bind FMRFamide and from our results thatdemonstrate pH modulation of LsFaNaC, it would seem that regionsconserved between the FaNaCs and the ASICs may in fact be sitesof FMRFamide binding or acid sensing. Such regions should be divergentor nonexistent in those channels, which are not affected by FMRFamideor acid treatment. A comparison of all three FaNaCs with ASIC3and $alpha$ ENaC reveals that such a region exists, just before TM2 (residues477-519 in LsFaNaC). In this 43 residue region of near sequenceidentity within the FaNaCs there is considerably more sequencehomology to ASIC3 than there is to $alpha$ ENaC. Mutational analysisof this region and other potential sites should allow the siteof ligand binding to be determined. Such a study would elucidatewhether acid modulation of the LsFaNaC and acid-gating in ASICsare in fact caused by a conserved, structurally related site orwhether the effects are mediated by nonrelatedsites.

  FOOTNOTES

Received April 25, 2001; revised April 25, 2001; accepted May 17, 2001.

This work was supported by a grant from the Biotechnology and Biological Sciences Research Council to P.R.B.
S.J.P. and V.A.S. contributed equally to thiswork.

Correspondence should be addressed to V. A. Straub, Sussex Centre for Neuroscience, University of Sussex, Falmer, BrightonBN1 9QG, UK. E-mail: V.Straub{at}sussex.ac.uk.

S. J. Perry's present address: Department of Medicine, Duke University Medical Center, Durham, NC27710.

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