Mediation by Protein Kinases C and A of Go-Linked Slow Responses of Enteric Neurons to 5-HT

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Volume 17, Number 3, Issue of February 1, 1997 pp. 1011-1024
Copyright ©1997 Society for Neuroscience

Mediation by Protein Kinases C and A of G_o-Linked Slow Responses of Enteric Neurons to 5-HT

Hui Pan¹, Hoau-Yan Wang², Eitan Friedman², and Michael D. Gershon¹
¹ Department of Anatomy and Cell Biology, Columbia University, College of Physicians and Surgeons, New York, New York 10032, and ² Department of Pharmacology, Allegheny University of the Health Sciences, MCP-Hahnemann School of Medicine, Philadelphia, Pennsylvania 19129

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

5-HT activates the peristaltic reflex and is the neurotransmitter of a subset of myenteric interneurons. Hyperpolarizing afterpotential(AH)/type 2 neurons respond to 5-HT with a long-lived depolarizationthat is caused by the inhibition of a Ca²⁺-activated K⁺ conductance (gK_Ca). This effect is mediated by a G-protein-coupledreceptor, 5-HT_1P. 5-HT_1P agonists specifically activate G $alpha$ _o, theimmunoreactivity of which was found to be highly abundant andmembrane-associated in almost all enteric neurons. Responses ofhyperpolarizing AH/type 2 neurons to 5-HT were inhibited by intracellularinjection of GDP $beta$ S or anti-G $alpha$ _o Fab fragments but were potentiatedand prolonged by intracellular GTP $gamma$ S. Responses to 5-HT were antagonizedby pertussis toxin, downregulation of protein kinase C (PKC) andinhibitors of phosphatidylcholine phospholipase C (PC-PLC), PKC(including pseudosubstrate peptides, chelerythrine, and the $alpha$ / $beta$ isoform-specific inhibitor G_ö 6976),protein kinase A (PKA), and adenylate cyclase. Responses to 5-HTwere mimicked by activators of PKC, and 5-HT induced a concentration-dependentincrease in the membrane-associated PKC activity in isolated myentericganglia. Immunocytochemical studies suggested that the most abundantisoforms of PKC in enteric neurons are $alpha$ and $delta$ . These data suggestthat signal transduction of the 5-HT_1P-mediated slow responseto 5-HT involves activation of PC-PLC by G $alpha$ _o to liberate diacylglycerol,which stimulates PKC (most likely $alpha$ ). PKC probably activates adenylatecyclase, which through cAMP, activates PKA. Activation of bothPKA and PKC lead to closure of gK_Ca.
Key words: enteric nervous system; serotonin; 5-hydroxytryptamine; 5-HT_1P receptor; protein kinase C; protein kinase A; phosphatidylcholine phospholipase C; G_o; G-proteins; signal transduction

INTRODUCTION

Responses of the gut to exogenous 5-HT may be nerve- or muscle-mediated, excitatory, or inhibitory (Mawe and Gershon, 1993;Gershon et al., 1994; Wade et al., 1994). The complexity of theseresponses is attributable to the multiplicity of 5-HT receptorsubtypes in the enteric nervous system (ENS) (Gershon, 1995) andmusculature (Engel et al., 1984). At least five subtypes are presenton nerve, 5-HT_1A (Galligan et al., 1988; Galligan and North, 1991),5-HT_1P (Branchek et al., 1984; Mawe et al., 1986; Mawe and Gershon,1993), 5-HT_2B (unpublished data), 5-HT₃ (Mawe et al., 1986; Derkachet al., 1989), and 5-HT₄ (Clarke et al., 1989; Craig and Clarke,1990; Pan and Galligan, 1994) and two subtypes on muscle, 5-HT_2Aand 5-HT_2B (Engel et al., 1984; Cohen et al., 1985; Foguet etal., 1992a,b; Kursar et al., 1992). Of these receptors, only 5-HT_1Phas been shown to play roles in specific physiological responses.These include the mediation of slow EPSPs in myenteric neurons(Takaki et al., 1985a,b; Mawe et al., 1989; Wade et al., 1991,1994; Galligan, 1995) and the initiation of the peristaltic reflex(Kirchgessner et al., 1992, 1997; Wade et al., 1996).

The response of myenteric neurons that is 5-HT_1P-mediated is known as the slow response (Wood, 1989; Gershon et al., 1994;Galligan, 1995). These responses are most common in hyperpolarizingafterpotential (AH)/type 2 neurons, a cell that is defined bya characteristic Ca²⁺-activated K⁺ conductance (gK_ca). This gK_ca gives rise to a pronounced hyperpolarizingafterpotential (AH) and also contributes to the resting membranepotential (Galligan, 1995). 5-HT inhibits gK_Ca, resulting in aslowly developing but long-lived depolarization, associated withan increase in input resistance and inhibition of the AH (Woodand Mayer, 1979; Grafe et al., 1980; Johnson et al., 1980; Moritaet al., 1982; Hirst et al., 1985; North and Tokimasa, 1987; Galligan,1995). Slow responses to 5-HT are identical to slow EPSPs evokedin the same neurons (Wood and Mayer, 1979), and both are blockedspecifically by N-acetyl-5-hydroxytryptophyl-5-hydroxytryptophanamide (5-HTP-DP) (Takaki et al., 1985a; Mawe et al., 1986), renzapride(Mawe et al., 1989), and anti-idiotypic antibodies that recognize5-HT receptors (Wade et al., 1994). The 5-HT_1P receptor binds5-HT with high affinity (K_D $approx$ 2-3 nM) (Branchek et al., 1984;Gershon et al., 1985; Mawe et al., 1986) and requires that potentialligands be hydroxylated indoles (Branchek et al., 1988; Mawe andGershon, 1993).

5-HT receptor subtypes are defined by their primary structure, transductional properties, and operational characteristics(Humphrey et al., 1993). Although the transductional propertiesof the 5-HT_1P receptor have not previously been fully characterized,following three observations have led to the suggestion that thisreceptor is a member of the heptahelical G-protein-coupled receptorfamily: (1) the binding of ³H-5-HT by the receptor is antagonized by GTP $gamma$ S (Gershon et al.,1991; Fiorica-Howells et al., 1993); (2) intracellular injectionof GTP $gamma$ S potentiates and prolongs slow responses to 5-HT; and(3) similar injections of GDPS inhibit slow responses (Wanget al., 1996). The G-protein to which the 5-HT_1P receptor is coupled,moreover, is likely to be G_o, because G_o is activated specificallywhen enteric neuronal membranes are incubated with 5-HT or 5-hydroxyindalpine(Wang et al., 1996), a 5-HT_1P agonist (Branchek et al., 1988).Activation of G_o by either 5-HT or 5-hydroxyindalpine is antagonizedby 5-HTP-DP (Wang et al., 1996). The current experiments werecarried out to identify the signal transduction pathway responsiblefor 5-HT_1P-mediated slow responses.

MATERIALS AND METHODS
Tissue preparation. Male guinea pigs weighing 250-350 gm were stunned and exsanguinated. A segment of ileum was excised 10-20cm proximal to the ileocecal junction and placed in oxygenated(95% O₂/5% CO₂) Krebs' solution of the following composition (inmM): NaCl 121.3, KCl 5.95, CaCl₂ 2.5, NaHCO₃ 14.3, NaH₂PO₄ 1.34,MgCl₂ 1.2, and glucose 11.5. The Krebs' solution contained nifedipineand scopolamine (1 µM each) to block longitudinal muscle contractionswhile intracellular recordings were obtained. A 1.5 cm segmentof ileum was cut open along the mesenteric border and pinned outflat (mucosal surface up) in a Petri dish lined with a siliconeelastomer. Preparations of longitudinal muscle with adherent myentericplexus (LMMP) were dissected by removing the mucosa, submucosa,and circular muscle with a fine forceps and scissors under microscopiccontrol. A 5 mm² LMMP segment was transferred to a small recording chamber (volume,0.5 ml) that was coated with a silicone elastomer. The LMMP wasstretched lightly and pinned with small stainless steel pins tothe silicone coating of the bottom of the chamber. Preparationswere superfused (3.5 ml/min; 36°C) with Krebs' solution oxygenatedwith a mixture of 95% O₂/5% CO₂.

Intracellular recording. Individual myenteric ganglia were visualized at a magnification of 6.3×. Intracellular recordingswere obtained from neurons using glass microelectrodes filledwith 2 M KCl (tip resistance, 90-160 M $Omega$ ). An amplifier with anactive bridge circuit (Axoclamp 2A, Axon Instruments, Foster City,CA) was used to record the transmembrane potential differenceand to inject current via the recording electrode.

Drugs, chemicals, and antibodies. 5-HT (Sigma Chemical, St. Louis, MO), forskolin (Research Biochemicals International, Natick,MA), histamine (Research Biochemical International), and the PKCactivators phorbol 12,13-dibutyrate (PDBu, Research BiochemicalInternational), ( $-$ )-7-octylindolactam V (LC Laboratories, Woburn,MA), and 1-oleoyl-2-acetyl-rac-glycerol (OAG, Sigma) were appliedto neurons by ejection with pressure from a micropipette (filledwith a 1.0 mM solution) or by addition to the fluid superfusingthe preparations. In six cells used to evaluate the reproducibilityof responses, the ratio of the amplitude of a second responseto 5-HT to that of its predecessor was 0.97 ± 0.05 (p = 0.5669).The interval between trials of 5-HT was at least 5 min to avoiddesensitization of 5-HT receptors. In all experiments, the effectof drugs on responses to 5-HT, histamine, or forskolin was notinvestigated until after reproducible responses to the agonistwere obtained. Membrane-permeable potential antagonists of stepsin signal transduction were added to the superfusing solutions.These included the phosphatidylcholine-phospholipase C (PC-PLC)inhibitor D609 (Kamiya Biomedical, Thousand Oaks, CA); the adenylatecyclase inhibitor 2 $'$ ,5 $'$ -dideoxyadenosine (DDA, Biomol ResearchLaboratory, Plymouth Meeting, PA); and the PKC inhibitors chelerythrine(LC Laboratories), staurosporine (Research Biochemical International),K252a (Kamiya), Gö 6976, an indolcabazole that selectively inhibitsthe PKC isozymes, $alpha$ , $beta$ 1, $beta$ 2, and $gamma$ , but not $delta$ , $epsilon$ , or $zeta$ (Martiny-Baronet al., 1993) (Calbiochem, La Jolla, CA); and a myristolated pseudosubstratesequence from PKC $alpha$ and $beta$ , myr-FARKGALRQ (Biomol). Compounds thatdo not readily cross cell membranes were microinjected into neuronsvia the recording microelectrode. These included GTP $gamma$ S (Sigma),GDP $beta$ S (Sigma), Fab fragments of antibodies to G $alpha$ _o (preparationdescribed below), the PKC $alpha$ , $beta$ pseudosubstrate, RFARKGALRQKNV(PKC_(19-31) (Kemp et al., 1994) (LC Labs, 1.0 mM), and theprotein kinase A (PKA) inhibitor Rp-adenosine 3 $'$ 5 $'$ -cyclic monophosphothiolatetriethylamine cAMPS (Rp-cAMPS, 70 mM, Research Biochemical International).Because pertussis toxin (PTx, Research Biochemical International)penetrates membranes slowly, preparations were incubated for 6hr ± PTx before determining the response to 5-HT.

Antibodies to G $alpha$ _o were obtained from Upstate Biotechnology, Lake Placid, NY. Fab fragments (Mage and Lamoyi, 1987) were preparedby digestion with papain (in an enzyme-to-protein ratio of 1:100)in 500 µl of 20 mM sodium phosphate buffer, pH 7.4, that contained20 µg of antibody to G $alpha$ o, dithiothreitol (1.0 mM), and EDTA (2.0mM). Digestion was allowed to proceed at 37°C for 4-5 hr. Afterincubation, the reaction mixture was cooled to room temperatureand transferred to dialysis tubing and dialyzed against PBS overnight.Protein A-Sepharose 4B beads were then added to the dialyzed mixtureto bind Fc fragments of the antibody. The beads were then removedby centrifugation to provide a final clear solution containingFab fragments that could be loaded into a micropipette.

Immunocytochemistry. Laminar preparations of LMMP or the dissected submucosa (containing the submucosal plexus) were fixedfor 3 hr with 4% formaldehyde (freshly prepared from paraformaldehyde)in 0.1 M sodium phosphate buffer, pH 7.4, at room temperature,and washed three times with PBS. To locate proteins in the tissueby immunocytochemistry, free-floating LMMP or submucosal preparationswere exposed to PBS containing 1.0% Triton X-100 and 10% horseserum for 30 min to permeabilize the tissue and reduce backgroundstaining. G $alpha$ _o immunoreactivity was demonstrated with rabbit polyclonalantibodies (Upstate Biotechnology) at a concentration of 1.0 µg/ml.Preparations were incubated overnight in a humidified chamberat room temperature. Bound antibody was visualized by incubatingtissues for 2 hr with biotinylated affinity-purified goat anti-rabbitIgG secondary antibodies (diluted 1:400; Kirkegaard & Perry, Gaithersburg,MD) at room temperature and then for 2 hr with avidin-FITC (diluted1:200; Vector Laboratories, Burlingame, CA). Calbindin immunoreactivity,which marks 70-80% of neurons classified anatomically as Dogieltype II and physiologically as AH/type 2 (Pompolo and Furness,1988; Furness et al., 1990), was located simultaneously in thesame sections used to visualize G $alpha$ _öimmunoreactivity by double-label immunocytochemistry. To demonstratecalbindin immunoreactivity, preparations were incubated overnightat room temperature with mouse monoclonal antibodies to calbindin(diluted 1:100; Sigma), and bound primary antibodies were locatedwith affinity-purified goat anti-mouse secondary antibodies labeledwith tetramethylrhodamine isothiocyanate (TRITC, diluted 1:100;Kirkegaard and Perry). Double-label immunocytochemistry was madepossible, because primary antibodies were raised in differentspecies and immunoreactivity was visualized with species-specificsecondary antibodies. Specific antibodies to the following isozymesof PKC, $alpha$ , $beta$ 1, $beta$ 2, $gamma$ , $delta$ , $epsilon$ , $zeta$ , $iota$ / $lambda$ , and $eta$ (Jiang et al., 1994),were donated by Dr. Todd Sacktor (State University of New York,Downstate Medical Center). These were all polyclonal rabbit antibodiesand thus were visualized, as described above, with biotinylatedgoat anti-rabbit secondary antibodies, and avidin-FITC. Immunostainedtissues were examined with a Leica DMRB Microscope equipped forvertical fluorescence microscopy. FITC fluorescence was detectedusing a Leica "L-4" filter cube (exciting filter band pass, 470-490nm; dichroic mirror reflection short pass, 510 nm; suppressionfilter bandwidth, 520 nm). TRITC fluorescence was detected usinga Leitz "N-2.1" filter cube (exciting filter band pass, 546/14nm; dichroic mirror reflection short pass, 580 nm; edge wavelength,580 nm). There was no cross-detection between the FITC- and TRITC-selectivedichroic mirror-filter cubes.

Isolation of myenteric ganglia. Ganglia were isolated from dissected LMMP preparations by a modification of the method describedpreviously (Fiorica-Howells et al., 1993). This procedure takesadvantage of the absence of collagen from the interior of themyenteric plexus and the role of glia in providing support forneurons (Gershon et al., 1994). When the LMMP is exposed to collagenase,therefore, the ganglia of the myenteric plexus remain largelyintact, whereas the non-neuronal components of the preparationdissociate and form a suspension of single cells (Yau et al.,1989). When the resulting suspension of dissociated cells andintact ganglia is filtered through a wide-pore (8.0 µm) filter(Nucleopore), the individual cells pass though, whereas the gangliaare trapped on the filter (Fiorica-Howells et al., 1993). Studiesusing desmin immunoreactivity as a muscle marker and neuron-specificenolase as a neuronal marker have verified that the filtered preparationsare highly enriched with ganglia and not contaminated by muscle.

For immunoblotting, the ganglia were scraped from the filters and homogenized in iced buffer [50 mM Tris, pH 7.5, 0.15 M NaCl,1% Triton X-100, 25 µg/ml each of the peptidase inhibitors leupeptinand aprotinin (Sigma), 2 mM EDTA, and 1.0 mM EGTA]. The homogenatewas spun for 10 min in a microcentrifuge, and the proteins inthe resulting supernatant were separated by electrophoresis through10% PAGE. The proteins were then blotted onto nitrocellulose membranesand probed with G-protein-purified rabbit polyclonal antibodiesselective for the $alpha$ , $beta$ , $gamma$ , $delta$ , $epsilon$ , and $zeta$ isozymes of PKC. Immunoreactivebands were demonstrated with goat anti-rabbit secondary antibodiesconjugated to horseradish peroxidase. Horseradish peroxidase activitywas visualized with TMB peroxidase substrate (Kirkegaard & Perry).

Protein kinase C-mediated protein phosphorylation and translocation. Isolated myenteric ganglia were incubated for 10 minat 37°C in Krebs' solution with 1.0 µM 5-HT, 10.0 µM 5-HT, or1.0 µM PDBu. Reactions were terminated by addition of 0.5 mM EGTAin Ca²⁺- free Krebs' solution. Preparation of tissue fractions and assessmentof PKC activity was performed as described previously (Friedmanand Wang, 1989). All subsequent procedures were carried out at4°C, unless otherwise indicated. Tissues were harvested and homogenizedin 10 vol of buffer A (20.0 mM Tris-HCl, pH 7.5, 0.32 M sucrose,2.0 mM EDTA, 0.5 mM EGTA, 50.0 µg/ml leupeptin, 0.1% 2-mercaptoethanol,and 0.2 mM phenylmethylsulfonyl fluoride), and the homogenatewas centrifuged at 800 × g for 10 min. The supernatant obtainedwas sonicated (Kontes Micro Cell Disrupter) and centrifuged at25,000 × g for 15 min. The resultant supernatant was removed,diluted to 1.0 ml with buffer A, chromatographed on diethylaminoethylcellulose (DE52, Whatman, Maidstone, UK) anion exchange columnsand used as the cytosolic fraction. The pellet was resuspendedin 1.0 ml buffer A with 0.2% Nonidet P-40 and solubilized on icefor 1 hr. The sample was centrifuged at 25,000 × g for 15 min.The resultant supernatant was chromatographed on DE52 columns,and the eluate was used as the membrane extract. Samples wereapplied to 1.0 ml DE52 columns equilibrated in buffer A, and thecolumns were washed with 5.0 ml of buffer A followed by 0.5 mlof 20 mM NaCl in buffer A. Enzyme was eluted with 0.75 ml of 200mM NaCl in buffer A, and the eluate was used immediately for assessingPKC activity.

The standard assay mixture (250 µl) containing 24.0 mM Tris-HCl, pH 7.5, 20.0 mM NaCl, 0.1 mM EGTA, 0.4 mM EDTA, 0.03% 2-mercaptoethanol,60 µg/ml leupeptin, 0.04 mM phenylmethylsulfonyl fluoride, 0.25mg/ml, histone type III-s (Sigma), 1.2 mM CaCl₂, 20 µg/ml phosphatidyl-L-serine,8.0 nM phorbol-12-myristate,13-acetate, 10.0 mM Mg(CH₃CO₂)₂, and0.03 mM [³²P]ATP (500,000 cpm, DuPont, Boston, MA) was preincubated at 30°Cfor 5 min, and the reaction was initiated by the addition of elutedprotein. After 1 min, the reaction was terminated by transferring125 µl onto a 2 × 4 cm phosphocellulose (Whatman P81) strip thatwas subsequently immersed in 75.0 mM phosphoric acid (10.0 mlper strip). The strips were washed three times (2 min per wash)in fresh phosphoric acid and air dried. The strips were then placedin scintillation fluid, and radioactivity was determined by liquidscintillation spectrometry (LKB RACKBETA). PKC activity was definedas the phosphorylation that occurred in the presence of phosphatidyl-L-serineand phorbol-12-myristate,13-acetate and expressed as pmol ³²Pi-incorporated per unit protein of column eluate. Protein wasdetermined by the method of Lowry et al. (Lowry et al., 1951).

RESULTS
5-HT evokes a uniphasic slow depolarization in AH/type 2 neurons when receptors for 5-HT receptor subtypes other than 5-HT_1Pare antagonized

Recordings were made from cells that were classified as AH/type 2 neurons. Criteria used in classification included (1) thepresence of an AH, and (2) a Ca²⁺ shoulder on the falling phase of the action potential (Gershonet al., 1994; Wood, 1994). A total of 235 AH/type 2 neurons werestudied with a mean resting membrane potential of 73 ± 1 mV andan input resistance of 108 ± 5 M $Omega$ . Except where otherwise stated,the 5-HT_1A antagonist NAN-190 (0.3 µM) and the 5-HT_3/4 dual antagonisttropisetron (1.0 µm) were added to the superfusing medium so thatthe other subtypes of 5-HT receptor to which these cells are knownto respond, would not interfere with 5-HT_1P-mediated responses.Tetrodotoxin (1.0 µM) was also present to confine recordings topostsynaptic events in the impaled neurons. In a series of 81AH/type 2 cells studied under these conditions, 71 responded tothe microejection of 5-HT (Fig. 1). The response was uniphasicunder these conditions and consisted of a prolonged (104 ± 6 sec)membrane depolarization (16 ± 1 mV) associated with an increasein input resistance (mean increase = 102 ± 8%). No response to5-HT was observed in 10 of the 81 neurons; such cells were notstudied further. Superfused 5-HT (1.0 µM) reduced the amplitudeof the AH from 14 ± 1 mV (n = 14) in control preparations to 7± 3 mV (n = 5; p < 0.02). The duration of the AH was also reducedby 5-HT from 13 ± 2 sec in control preparations to 6 ± 2 sec (p< 0.05).
Fig. 1. 5-HT induces a slow depolarization in AH/type 2 cells during which membrane conductance decreases and the AH is inhibited.A, In the presence of the 5-HT_1A antagonist NAN-190 and the 5-HT_3/4antagonist tropisetron, the response to 5-HT is a uniphasic depolarizationassociated with an increase in input resistance. The top tracedepicts the membrane potential, and the bottom trace indicatescurrent injected through the recording pipette. The downward deflectionsin the top trace represent the electrotonic responses to the injectionsof hyperpolarizing current pulses. B, At a faster sweep speed,the pronounced AH (top trace) can be seen after the action potentialin the control record. The addition of 5-HT (1.0 µM) to the superfusingmedium blocks the AH. The bottom trace depicts depolarizing currentinjected through the recording pipette to evoke action potentials.
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The slow response to 5-HT is G_o protein-dependent
The hypothesis that the slow response of AH/type 2 neurons to 5-HT is mediated by a G_o protein was tested. Initial studieswere carried out to determine whether the previous report (Wanget al., 1996) that slow responses to 5-HT are potentiated by theintracellular injection of GTP $gamma$ S and inhibited by GDP $beta$ S couldbe confirmed in preparations in which responses to subtypes of5-HT receptor other than 5-HT_1P were blocked. Subsequent experimentsevaluated the sensitivity of the slow response to inhibition byPTx, which would be expected to antagonize a G_o-mediated response(Casey and Gilman, 1988). Finally, the effects of the intracellularinjection of Fab fragments of antibodies to G $alpha$ _o into AH/type 2neurons were ascertained. To study the effects of the guaninenucleotides on responses to 5-HT, recordings were made with beveledelectrodes loaded with GTP $gamma$ S or GDP $beta$ S. Control recordings wereobtained first and, after stable responses to 5-HT were observed,the cells were injected with the guanine nucleotide by passinga negative DC current and simultaneously applying pressure tothe recording electrode. The amplitude of control responses to5-HT and that of responses to 5-HT recorded 10-15 min after theinjection of GTP $gamma$ S or GDP $beta$ S were measured and their ratios determined(Fig. 2). Intracellular injection of GTP $gamma$ S more than doubled theamplitude of the response to 5-HT (p < 0.05; n = 6); furthermore,after the intracellular injection of GTP $gamma$ S, the depolarizationinduced by the microejection of 5-HT was greatly prolonged andthe membrane potential did not fully return to the resting level.In contrast, intracellular injection of GDP $beta$ S reduced the amplitudeof the response to 5-HT to ~35% of that of the control (Fig. 2)(p < 0.001; n = 6).
Fig. 2. The slow response to 5-HT is inhibited by the intracellular injection of GDP $beta$ S and potentiated by the intracellular injectionof GTP $gamma$ S.
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To study the effects of PTx, we initially tried to obtain control responses to 5-HT and then to maintain impalements longenough, after the addition of PTx (1.0 µg/ml) to the medium, todetermine whether the slow response to 5-HT was affected by thetoxin. Unfortunately, PTx is very slow to take effect when itis applied extracellularly. As a result, very long impalements(4-6 hr) were necessary to investigate the action of PTx. Themembrane properties of AH/type 2 cells, even in control experiments,were found to be unstable during such long impalements; consequently,although responses to 5-HT were found eventually be inhibitedin cells exposed to PTx (Wang et al., 1996), it was difficultto be certain that the inhibition was a specific effect of PTx.To circumvent this problem and to maximize the effectiveness ofexposure to PTx, preparations were incubated with PTx for 6 hrbefore recordings were obtained. Controls were incubated similarly,but PTx was not present in the medium. As an additional control,to evaluate possible nonspecific effects of incubation with PTx,the responses of AH/type 2 neurons to forskolin were studied inthe same cells used to investigate responses to 5-HT. Forskolin,which activates adenylate cyclase, evokes a slow depolarizationsimilar to that elicited by 5-HT, but the response to forskolin(Nemeth et al., 1986; Bertrand and Galligan, 1995) would not beexpected to be PTx-sensitive. The ratios of the amplitude of the5-HT response to that of forskolin were computed for control cellsand cells exposed to PTx. After incubation ± PTx, therefore, AH/type2 cells were identified and their responses to 5-HT and forskolindetermined (Fig. 3). The amplitude of the response to 5-HT wassignificantly lower (p < 0.0001) in cells incubated with PTx (2± 1 mV; n = 8) than in controls (14 ± 1 mV; n = 35). The amplitudeof the response to forskolin was also somewhat lower in cellsincubated with PTx (7 ± 1 mV; n = 8) than in controls (15 ± 1mV; n = 35). The ratio of the amplitudes of responses to 5-HTto those of forskolin (Fig. 3), however, was 1.05 ± 0.09 in controlcells and 0.34 ± 0.07 after exposure to PTx (p < 0.0001). Theresponse of AH/type 2 neurons to 5-HT thus was much more stronglyaffected by exposure to PTx than were the responses of the samecells to forskolin. These observations indicate that the slowresponse to 5-HT is PTx-sensitive.
Fig. 3. Slow responses to 5-HT are inhibited by pertussis toxin (PTx). Preparations were superfused with PTx (1.0 µg/ml) for 6 hr.Control preparations were superfused for an equivalent periodof time but in the absence of PTx. To control for nonspecificeffects of prolonged superfusion, responses of AH/type 2 cellsto 5-HT were compared with the similar responses of the same cellsto forskolin in the presence or absence of PTx. The graph showsthe ratio of the 5-HT to the forskolin response for control andPTx-treated preparations.
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Preliminary studies revealed that AH/type 2 neurons could not consistently be injected through the recording micropipettewith whole antibodies to G $alpha$ _o. Preparations in which injectionswere attempted were fixed and later immunostained with biotinylatedsecondary antibodies and avidin-FITC to determine whether antibodiesto G $alpha$ _o had actually entered cells. In practice, the pipettes filledwith whole antibodies tended to clog, leading to increases inelectrode tip resistance, and antibodies only rarely entered impaledcells in quantities adequate for immunocytochemical detection.Fab fragments were therefore prepared and used for intracellularinjection. In contrast to whole antibodies, the Fab fragmentsconsistently entered injected cells. An initial control was toinject cells with Fab fragments of anti-G $alpha$ s. Although these injectionsdid not inhibit slow responses to 5-HT, the effects of anti-G $alpha$ _oand anti-G $alpha$ s could not be compared in the same cells. To determinewhether injected anti-G $alpha$ _o exerts nonspecific effects, therefore,responses to 5-HT in anti-G $alpha$ _o-injected neurons were studied inthe absence of tropisetron, so that the 5-HT₃-mediated fast responseto 5-HT (Mawe et al., 1986; Derkach et al., 1989) could be measuredsimultaneously with the 5-HT_1P-mediated slow response and usedas a control. Before the injection of anti-G $alpha$ _o Fab fragments,therefore, the response to 5-HT was biphasic instead of monophasic.A rapidly developing transient depolarization (the fast response,which is known to be 5-HT₃-mediated) (Mawe et al., 1986; Wadeet al., 1991) preceded the much more slowly developing and longer-lived5-HT_1P-mediated slow response. A second control was to determinethe effect of injection of anti-G $alpha$ _o Fab fragments on responsesof AH/type 2 neurons to histamine. Histamine evokes a slow depolarizationsimilar to that elicited by 5-HT; however, the response to histamineis thought to be attributable to the activation of adenylate cyclase(Wood, 1994) and, thus, is probably coupled to a G_s protein. Intracellularinjection of anti-G $alpha$ _o Fab fragments was found to substantiallyinhibit the slow response to 5-HT, but these injections had littleor no effect on fast responses to 5-HT of the same neurons (Fig.4A,B) and did not significantly affect slow responses of thesecells to histamine (Fig. 4A, ii). The amplitude of the slow responseto 5-HT was reduced by injection of anti-G $alpha$ _o Fab fragments from13 ± 1 mV to 7 ± 1 mV (n = 23; p < 0.001). In contrast, the meanamplitude of the fast response in the same cells was 14.0 ± 1.8mV before injection and 14.5 ± 2.1 mV (n = 16; p is not significant).These data support the hypothesis that the 5-HT_1P receptor iscoupled to a G_o protein.
Fig. 4. Intracellular injection of anti-G $alpha$ _o Fab fragments inhibits slow responses to 5-HT. A, i, In the absence of tropisetron, 5-HTevokes a biphasic response (control), consisting of a fast 5-HT₃-mediateddepolarization, followed by the 5-HT_1P-mediated slow depolarization.The injection of anti-G $alpha$ _o Fab fragments antagonizes the slow butnot the fast response to 5-HT. ii, Control responses of the sameneuron to 5-HT and histamine are shown. The control response to5-HT is again biphasic; the fast response is very small. An actionpotential is seen during the depolarization. Injection of anti-G $alpha$ _oFab fragments inhibits the slow response to 5-HT far more thanthat to histamine. The mean ratio of the amplitude of slow responsesto histamine after injection of anti-G $alpha$ _o Fab fragments to controlresponses obtained in the same cells (1.3 ± 0.1) was not significantlydifferent from 1 (n = 6; p = 0.0804). B, The effects of intracellularinjection of anti-G $alpha$ _o Fab fragments on fast and slow responsesof AH/type 2 neurons to 5-HT are compared.
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Enteric neurons express G $alpha$ _o immunoreactivity The presence of G $alpha$ _o in enteric neurons and their processes was investigated by immunocytochemistry. G $alpha$ _o immunoreactivity wasobserved to be widely distributed in neurons of both the submucosal(Fig. 5A,B) and myenteric (Fig. 5C) plexuses. The immunoreactivitywas strikingly marginal in these cells and appeared to be concentratedin their plasma membranes (Fig. 5B,C). The cell bodies of neuronsthus appeared as negative images outlined by G $alpha$ _o-immunoreactivemembranes. G $alpha$ _o immunoreactivity was also abundant in the processesof these neurons and thus was seen in interganglionic connectives,as well as in ganglia. Calbindin immunoreactivity, which has beenused as a marker for AH/type 2 neurons and is found in the majorityof these cells (Pompolo and Furness, 1988; Furness et al., 1990)was demonstrated in the same preparations to determine whetherthere was a coincident cellular distribution of the two markers(Fig. 5C,D). All calbindin-immunoreactive neurons (Fig. 5D) wereringed by G $alpha$ _o-immunoreactive membranes (Fig. 5C); however, G $alpha$ _oimmunoreactivity was more widely distributed than that of calbindinand also ringed cells that did not contain calbindin. G $alpha$ _o immunoreactivitywas not observed in the intestinal musculature, but it was abundantin the ganglia and interganglionic connectives of the submucosalplexus (Fig. 5A). In the submucosa, G $alpha$ _o immunoreactivity was notconfined to neural tissue but was also found in the smooth muscleof arteries (Fig. 5A). Within submucosal ganglia, the localizationof G $alpha$ _o immunoreactivity was similar to that seen in the myentericplexus. Again, G $alpha$ _o immunoreactivity was concentrated around neurons,which appeared as negative images (Fig. 5B). Because submucosalneurons were as G $alpha$ _o immunoreactive as myenteric neurons, we evaluatedthe response of submucosal AH neurons to 5-HT. In the presenceof tetrodotoxin (1.0 µM), tropisetron (1.0 µM), and NAN 190 (0.3µM), 5-HT evoked a slow response that was very similar to thatobserved in AH/type 2 neurons of the myenteric plexus (Fig. 5E).
Fig. 5. G $alpha$ _o immunoreactivity is present in most submucosal and myenteric neurons. A, Both ganglia and interganglionic connectivesof the submucosal plexus contain G $alpha$ _o immunoreactivity. Connectivetissue cells of the submucosa do not exhibit G $alpha$ _o immunoreactivity;however, the smooth muscle of submucosal arteries (arrow) andassociated paravascular nerve fibers are also G $alpha$ _o immunoreactive.B, At higher magnification, the G $alpha$ _o immunoreactivity within asubmucosal ganglion can be seen to outline the membranes of componentneurons. C, The G $alpha$ _o immunoreactivity of the neurons of a myentericganglion (visualized with FITC) is also marginal and outlinesneuronal plasma membranes. D, The same section as shown in C,but the filters are set to reveal calbindin immunoreactivity,which is visualized with TRITC. Calbindin-immunoreactive neuronsare ringed by G $alpha$ _o immunoreactivity; however, so too are most ofthe neurons of the ganglion. Scale bars, 30 µm. E, An intracellularrecord obtained from a submucosal AH neuron showing a typical5-HT-evoked slow response associated with an increase in inputresistance.
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Activators of PKC mimic the slow response to 5-HT Because the slow response to 5-HT was found to be associated with the activation of a G_o protein, it seems unlikely that theresponse is directly linked to adenylate cyclase, which is normallyactivated by G_s. The hypothesis that the slow response to 5-HTis PKC-dependent was therefore tested. Each of three differentactivators of PKC mimicked the slow response to 5-HT. When appliedby microejection onto the surface of AH/type 2 neurons, PDBu induceda slow depolarization (Fig. 6A, record 1) with a mean amplitudeof 16 ± 2 mV (n = 8) associated with an increase in input resistanceof 87 ± 15%. The duration of the slow depolarization was extremelylong (>10 min). A similar, but even longer-lasting, response wasevoked by adding PDBu (1.0 µM) to the superfusing medium (Fig.6A, record 2). Almost identical responses were elicited by OAGor ( $-$ )-7-octylindolactam V (data not shown). In addition to theslow depolarization evoked by microejection of PDBu, the AH, whichis inhibited by superfused 5-HT (Figs. 1B, 6B) was also inhibitedby superfusion of PDBu (1.0 µM) or OAG (100 µM) (Fig. 6A, record3, B).
Fig. 6. Activators of PKC mimic slow responses to 5-HT. A, The phorbol ester PDBu evokes a slow depolarization in AH/type 2 neuronsassociated with an increase in input resistance, no matter whetherit is applied by microejection (1) from a pipette positioned closeto the impaled neuron or by superfusion (2) in the ambient medium.Superfusion of PDBu also inhibits the AH (3) that follows theaction potential in these cells. Note that although the effectsof PDBu are qualitatively similar to those of 5-HT, the responseto PDBu is much longer lasting. B, The effects of 5-HT (1.0 µM),OAG (100 µM), and PDBu (1.0 µM) on the amplitude of the AH inAH/type 2 neurons are compared. All three compounds inhibit theAH; PDBu is the most potent.
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PKC antagonists inhibit slow responses of AH/type 2 neurons to 5-HT The observation that activators of PKC mimic the slow response of AH/type 2 neurons to 5-HT suggests that PKC might be involvedin the transduction of responses mediated by the 5-HT_1P receptor.To determine whether PKC actually does play such a role, the abilityof PKC inhibitors to antagonize slow responses to 5-HT was determined.Superfusion of stau- rosporine (1.0 µM) (data not illustrated)and K-252a (3.0-10 µM) (Fig. 7B,C), both of which inhibit PKC,antagonized slow responses of AH/type 2 neurons to 5-HT. Thesecompounds, however, do not discriminate sufficiently well betweenPKC and other kinases to enable their antagonism of slow responsesto 5-HT to be attributed specifically to inhibition of PKC. Studieswere thus carried out with more selective PKC antagonists. Theseincluded the pseudosubstrate peptide PKC_[19-31]and the membrane permeable PKC inhibitors chelerythrine (3.0 µM),G_ö 6976 (10.0 µM), and myr-FARKGALRQ(40 µM) (Martiny-Baron et al., 1993). Because PKC_[19-31]does not cross cell membranes, it was injected into AH/type 2neurons through the recording micropipette. Superfusion with chelerythrine(Fig. 7A-C), G_ö 6976 (Fig. 7A),or myr-FARKGALRQ (Fig. 7A) and injection of PKC_[19-31](Fig. 7A-C) all inhibited slow responses to 5-HT. For these experiments,control responses to 5-HT were obtained and, when these were stablein amplitude, PKC_[19-31] was injected into cellsor the membrane permeable antagonists were added to the superfusingmedium. The ratio of the amplitude of the response to 5-HT afterthe injection of PKC_[19-31] or superfusion ofchelerythrine to that of the immediate preceding control responsewas determined (Fig. 7C). Each cell thus served as its own control.A ratio of 1.0 would have been obtained if PKC_[19-31]or chelerythrine had failed to antagonize slow responses to 5-HT.In fact, the ratios obtained for both of the specific PKC inhibitorswere significantly less than 1.0 [p < 0.001 for PKC_[19-31](n = 12); p < 0.01 for chelerythrine (n = 8)]. Similarly, a ratioof less than 1.0 was also obtained for the less PKC-specific K252a[p < 0.05 (n = 3)] (Fig. 7C). The membrane-permeable myristolatedpeptide myr-FARKGALRQ also reduced the amplitude of the slow responseto 5-HT from 22.0 ± 2.0 mM to 7.0 ± 2.0 mV; in contrast to theamplitude of slow responses, the amplitude of fast responses to5-HT before addition of myr-FARKGALRQ, 12.5 ± 6.5 mV, was notsignificantly different from that obtained after exposure to thepeptide, 14.5 ± 7.5 mV (n = 3).
Fig. 7. Inhibitors of PKC antagonize slow responses to 5-HT. A, Slow responses to 5-HT of an AH/type 2 neuron are antagonized by theintracellular injection of the PKC pseudosubstrate PKC_[19-31](top trace, left) and by the superfusion of the membrane permeablePKC pseudosubstrate myr-PKC_[19-27] (myr-FARKGALRQ;bottom trace, left). Slow responses are also inhibited by thesuperfusion of chelerythrine (3.0 µM; top trace, right) and bythe selective PKC $alpha$ and $beta$ antagonist G_ö6976 (10 µM; bottom trace, right). B, C, The abilities of PKC_[19-31]chelerythrine and K252a to reduce the amplitude of the 5-HT-inducedslow depolarization of AH/type 2 cells are compared.
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Downregulation of PKC antagonizes slow responses to 5-HT The observations that six different inhibitors of PKC each antagonized the slow response of AH/type 2 neurons to 5-HT supportsthe idea that PKC plays a critical role in the transduction ofresponses mediated by the 5-HT_1P receptor. If so, then the downregulationof PKC would be expected to interfere with slow responses to 5-HT.To downregulate PKC, dissected preparations of LMMP were culturedovernight in the presence of PDBu (10 µM). Control preparationswere cultured similarly, but in the absence of PDBu. The amplitudeof slow responses of AH/type 2 neurons to 5-HT in the preparationsexposed overnight to PDBu was compared with that of slow responsesto 5-HT in the controls. To test the possibility that a decreasein the amplitude of slow responses to 5-HT in cells chronicallyexposed to PDBu might have been attributable to nonspecific effects,responses to forskolin were also obtained from each of the cellsused for testing responses to 5-HT. Responses to forskolin, whichstimulates adenylate cyclase, would not be expected to be dependenton PKC; moreover, the slow depolarizing response of AH/type 2neurons to forskolin (amplitude, 16 ± 1.0 mV; duration, 165 ±9.0 sec, increase in input resistance of 107 ± 11.8%; n = 46)is very similar to the slow response of these cells to 5-HT. Theratio of the amplitudes of the slow responses of each neuron to5-HT to that of the same cells to forskolin was determined. Inpreparations that were not exposed to PDBu, the amplitudes ofslow responses to 5-HT and forskolin were about equal (Fig. 8A)(n = 32); however, in preparations that were treated with PDBu,the amplitudes of the responses of AH/type 2 neurons to 5-HT werequite small and considerably less than those to forskolin (Fig.8B) (n = 11). As a result, the 5-HT to forskolin ratio was significantlyreduced by the chronic exposure of preparations to PDBu (Fig.8C) (p < 0.001). Chronic exposure to PDBu also reduced the durationof slow responses to 5-HT and the associated increase in inputresistance. The ratio of the duration of the 5-HT response tothat of forskolin fell from 0.7 ± 0.1 in untreated preparationsto 0.4 ± 0.1 in those exposed to PDBu (p < 0.05). The ratio ofthe maximal change in input resistance during the 5-HT responseto that during the response to forskolin decreased from 1.3 ±0.2 in untreated preparations to 0.3 ± 0.2 in preparations treatedchronically with PDBu (p < 0.001). These observations indicatethat the slow response of AH/type 2 neurons is inhibited specificallyby downregulation of PKC.
Fig. 8. Downregulation of PKC inhibits the slow response of AH/type 2 neurons to 5-HT. A, In control preparations, the amplitudesof the slow depolarizations evoked by 5-HT and forskolin are approximatelyequal. B, After overnight exposure of preparations to PDBu todownregulate PKC, the 5-HT-induced slow depolarization is reducedin amplitude far more than is the response to forskolin. C, Incontrol preparations, the ratio of the amplitude of the 5-HT tothe forskolin response is about 1; however, this ratio is greatlyreduced as a result of the inhibition of the response to 5-HTafter long-term exposure of preparations to PDBu.
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5-HT activates PKC in isolated myenteric ganglia To test directly whether 5-HT activates PKC in situ, we measured the membrane association of PKC activity ± the exposure ofisolated myenteric ganglia to 5-HT. As a positive control, themembrane association of PKC activity was also followed in preparationsexposed to PDBu. The action of 5-HT was investigated in isolatedganglia to avoid interference from effects 5-HT might exert onsmooth muscle. The isolated ganglia, trapped on filters, wereequilibrated for 5 min at 37°C in oxygenated Krebs' solution,to which was added the 5-HT_1A antagonist NAN-190 (0.3 µM), the5-HT₂ antagonist ketanserin (10 µM), and the 5-HT_3/4 dual antagonisttropisetron (1.0 µM) to block responses to subtypes of 5-HT receptorother than 5-HT_1P. 5-HT (1.0 or 10.0 µM) or PDBu (1.0 µM) werethen applied for 10 min in the continued presence of the cocktailof antagonists. Control preparations were incubated similarlyin the absence of 5-HT. After incubation, all preparations werewashed for 5 min with iced Krebs' solution and transferred toiced buffer for homogenization. PKC activity was measured in boththe membrane and supernatant fractions. Exposure to 5-HT induceda concentration-dependent increase in the membrane associatedPKC activity (Table 1). At 10 µM, the response to 5-HT was ~75%that to PDBu.

Table 1. PKC translocation in myenteric ganglia

PKC activity

Membrane bound Cytosol M/C ratio

(pmol/min/µg protein)

Control 2.09 ± 0.08 2.90 ± 0.11 0.72 ± 0.03

5-HT (1.0 µM) 2.72 ± 0.16^* 2.23 ± 0.06^* 1.22 ± 0.07^*

5-HT (10.0 µM) 3.17 ± 0.19^* 1.96 ± 0.03^* 1.61 ± 0.10^*

PDBu (1.0 µM) 3.86 ± 0.04^* 1.78 ± 0.04^* 2.17 ± 0.05^*

The ability of the PKC $alpha$ / $beta$ pseudosubstrates myr-FARKGALRQ and PKC_[19-31] as well as the $alpha$ / $beta$ isozyme-selectiveG_ö 6976 to antagonize slow responsesto 5-HT suggests that one of the classical isozymes of PKC islikely to be responsible for the effect.

^* P < 0.01, compared with control. Data are mean ± SEM. n = 3-6.

Inhibition of PC-PLC antagonizes slow responses to 5-HT The observations that the slow response of AH/type 2 neurons to 5-HT are dependent on a G_o protein and PKC raise the questionof how G_o, after its activation by the 5-HT_1P receptor, is coupledto PKC. This coupling could be dependent on the activity of aPLC; however, because the slow response to 5-HT is attributableto the inhibition of gK_Ca, it would seem unlikely that the activationof PKC would be linked to a mechanism that would increase intracellularCa²⁺ ([Ca²⁺]_i). The hypothesis was therefore tested that the slow responsedepends not on a phosphatidylinositol-specific isozyme of PLCbut on PC-PLC. The liberation of inositol-1,4,5-trisphosphate(IP₃) by a phosphatidylinositol-specific PLC would be expectedto cause the release of Ca²⁺ from internal stores and thus to increase [Ca²⁺]_i (Exton, 1994). In contrast, the action of PC-PLC would liberatethe PKC activator, DAG, without simultaneously liberating IP₃(Schütze et al., 1992). The effect of D609 (100 µM), a specificinhibitor of PC-PLC (Schütze et al., 1992), on the slow responseof AH/type 2 neurons to 5-HT was therefore tested. Although D609did not affect the membrane potential of AH/type 2 cells, theamplitude of the 5-HT-induced slow depolarization was significantlyreduced by D609 (Fig. 9A,B) (p < 0.001; n = 9).
Fig. 9. An inhibitor of PC-PLC antagonizes slow responses to 5-HT. A, Slow responses to 5-HT are inhibited by the PC-PLC inhibitor,D609. B, The amplitudes of 5-HT-evoked slow depolarizations inthe presence or absence (control) of D609 are compared.
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PKA antagonism inhibits slow responses of AH/type 2 neurons to 5-HT The data outlined above, which suggest that PKC participates in mediating slow responses of AH/type 2 neurons to 5-HT, donot imply that PKC is the only protein kinase that does so. Becausethe downregulation or inhibition of PKC antagonized, but did notabolish, slow responses to 5-HT, it is possible that another proteinkinase contributes to the response. To test the hypothesis thatPKA contributes to the slow response of AH/type 2 cells to 5-HT,the selective PKA inhibitor Rp-cAMPS was injected into AH/type2 neurons through the recording electrode. Responses to 5-HT,applied by microejection to the surfaces of AH/type 2 neurons,were then determined. The ability of injected Rp-cAMPS to effectthe slow depolarization evoked in the same cells by pressure applicationsof the PKC activator PDBu was assessed as an expected negativecontrol. Forskolin and histamine were also studied as expectedpositive controls, because they increase cAMP and thus probablyact via PKA. The resemblance of the response of AH/type 2 neuronsto forskolin has been described above. When applied by microejectionto the surfaces of AH/type 2 neurons, histamine evoked a similarslow depolarization (amplitude, 20 ± 1.2 mV; duration, 93 ± 14.5sec; increase in input resistance, 100 ± 0%; n = 3). As expected,Rp-cAMPS blocked both the responses of AH/type 2 neurons to histamineand those to forskolin (data not shown). Because Rp-cAMPS rapidlydiffused into impaled cells from the recording electrode, evenin the absence of pressure or application of current, it was impossibleto be certain that responses to 5-HT or PDBu obtained before theinjection of Rp-cAMPS were not affected by the compound. The meanamplitudes of the pooled responses to 5-HT (n = 8) or PDBu (n= 4) obtained from neurons after the intracellular injection ofRp-cAMPS were thus compared with the mean amplitudes of the pooledresponses to 5-HT (n = 81) or PDBu (n = 8) obtained from controlneurons. Intracellular injection of Rp-cAMPS significantly (p< 0.001) reduced the amplitude of the slow response of AH/type2 neurons to 5-HT (Fig. 10A,C) but did not affect the amplitudeof the slow response of these cells to PDBu (Fig. 10C). In additionto the reduction in the amplitude of slow responses to 5-HT causedby the intracellular injection of Rp-cAMPS, superfusion of Rp-cAMPSantagonized the ability of 5-HT to inhibit the AH of AH/type 2neurons (Fig. 10B).
Fig. 10. Inhibition of PKA antagonizes slow responses to 5-HT. A, Slow responses to 5-HT of an AH/type 2 neuron are antagonized bythe intracellular injection of the PKA antagonist Rp-cAMPS. B,Under control conditions (top tracings), 5-HT (1.0 µM) inhibitsthe AH that follows the action potential in an AH/type 2 cell.Superfusion of Rp-cAMPS (200 µM; bottom tracings) does not itselfaffect either the action potential or the AH; however, superfusionof Rp-cAMPS prevents the inhibition of the AH by 5-HT. C, Althoughthe slow depolarization of AH/type 2 neurons by 5-HT is inhibitedby the intracellular injection of Rp-cAMPS, the slow depolarizationevoked by PDBu is not affected by Rp-cAMPS.
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Antagonism of adenylate cyclase inhibits slow responses of AH/type 2 neurons to 5-HT The data obtained with Rp-cAMPS are consistent with the idea that PKA, as well as PKC, contributes to the transduction ofresponses mediated by the 5-HT_1P receptor. The participation ofPKA suggests that adenylate cyclase is also likely to play a rolein the response. This hypothesis was tested by determining theeffects of the specific adenylate cyclase inhibitor DDA (0.5 mM)on slow responses of AH/type 2 neurons to 5-HT. The addition ofDDA to the superfusing medium did not affect the membrane potentialbut reduced the amplitude of the 5-HT-induced slow depolarizationfrom 16.0 ± 3.7 mV before the addition of DDA to 4.0 ± 1.5 mVin the presence of the compound (p < 0.05; n = 5). These observationsare consistent with the idea that adenylate cyclase participatesin the transduction of 5-HT_1P-mediated responses.
A variety of isozymes of PKC can be identified in enteric neurons Antibodies to various isozymes of PKC were used to investigate the expression of PKC in the ENS by immunocytochemistry. Westernblots were carried out with proteins extracted from isolated myentericganglia to confirm results obtained by immunocytochemistry. Calbindinimmunoreactivity was located simultaneously with the PKC isozymesto identify probable AH/type 2 neurons in the same preparations.Of the classical (group A) isozymes, only PKC $alpha$ immunoreactivitywas extensively expressed in the enteric plexuses. The distributionof PKC $alpha$ immunoreactivity was similar to that of G $alpha$ _o. As withG $alpha$ _o, the immunoreactivity of PKC $alpha$ was strikingly marginal, formingrings around most myenteric neurons (Fig. 11A). Virtually all ofthe calbindin-immunoreactive neurons (Fig. 11B) were surroundedby such rings of PKC $alpha$ immunoreactivity (compare Fig. 11A and B).In addition, PKC $alpha$ immunoreactivity was abundant in the ganglionicneuropil and was found in processes coursing through interganglionicconnectives. The immunoreactivity of PKC $alpha$ was equally abundantin the submucosal plexus, where it again outlined most neuronsand extended into interganglionic connectives (Fig. 11A, inset).In contrast to PKC $alpha$ , almost no PKC $beta$ 1 or $beta$ 2 immunoreactivitycould be detected in enteric neurons, although smooth muscle containedPKC $beta$ 2 immunoreactivity (data not shown). Of the novel (groupB) isozymes of PKC, only PKC $delta$ immunoreactivity was present inabundance in the ENS. The pattern obtained with antibodies toPKC $delta$ (Fig. 11C) was quite similar to that obtained with antibodiesto PKC $alpha$ . Again, the immunostaining of myenteric neurons was strikinglymarginal and PKC $delta$ immunoreactivity outlined myenteric nerve cellbodies, leaving the bulk of the neuronal cytoplasm unstained.All calbindin-immunoreactive neurons (Fig. 11D) were surroundedby PKC $delta$ immunoreactivity; however, PKC $delta$ immunoreactivity wasnot specifically associated with calbindin-immunoreactive cellsand surrounded almost all of the neurons of the myenteric plexus.PKC $delta$ immunoreactivity was also found in the ganglionic neuropiland in axonal varicosities (Fig. 11C). The abundance of PKC $delta$ immunoreactivitywas only slightly less than that of PKC $alpha$ but was more prominentthan that of $alpha$ in axonal varicosities. No specific immunostainingof the enteric plexuses were obtained with antibodies to anothernovel isozyme, PKC $epsilon$ , although $epsilon$ immunoreactivity was seen inthe smooth muscle (data not shown). Of the atypical isozymes ofPKC that were investigated, $zeta$ , $iota$ / $lambda$ , and $eta$ , none immunostainedenteric neurons. Cells with an appearance and distribution consistentwith that of peritoneal macrophages, however, were immunostainedwith antibodies to PKC $eta$ , which was also observed in circularmuscle. The immunoreactivity of PKC $gamma$ , a classical enzyme, wasobserved in small numbers of myenteric axons, which were distinguishedby very large varicosities (Fig. 11E). Weak PKC $gamma$ immunoreactivitywas also observed in rare neurons (data not shown), which didnot contain calbindin. In addition, small extraganglionic cellsexhibited strong PKC $gamma$ immunoreactivity, which appeared to belocated in intracellular granules (Fig. 11E); these cells did notcontain calbindin (compared F and E). These observations indicatethat only two isozymes of PKC, $alpha$ and $delta$ , are abundant in entericneurons. Data obtained from Western blots of proteins obtainedfrom preparations of isolated myenteric ganglia were consistentwith the observations made by immunocytochemistry; thus, onlyPKC $alpha$ , $gamma$ , and $delta$ immunoreactivities were observed in isolated ganglia(data not shown).
Fig. 11. The immunoreactivities of PKC $alpha$ and PKC $delta$ are prominent in enteric neurons. A, PKC $alpha$ immunoreactivity (visualized with FITC)is concentrated at the margins of neurons in both a myentericand a submucosal ganglion (inset) and thus outline enteric neurons.Axons entering interganglionic connectives (arrows) are also PKC $alpha$ -immunoreactive. B, Calbindin immunoreactivity (visualized withTRITC) is demonstrated in the same section as shown in A. Althoughcalbindin-immunoreactive neurons are outlined by PKC $alpha$ immunoreactivity,so too are virtually all of the neurons of the myenteric plexus.C, PKC $delta$ immunoreactivity (visualized with FITC) is concentratedat the margins of neurons in a myenteric ganglion but does notoutline cells quite as sharply as does the immunoreactivity ofPKC $alpha$ . Axons entering interganglionic connectives are also PKC $delta$ -immunoreactive. D, Calbindin immunoreactivity (visualized withTRITC) is demonstrated in the same section as shown in C. Calbindin-immunoreactiveneurons are outlined by PKC $delta$ immunoreactivity, but again virtuallyall of the neurons of the myenteric plexus are ringed by PKC $delta$ immunoreactivity. E, PKC $gamma$ immunoreactivity is seen in some highlygranular cells (arrows) located outside of myenteric ganglia (aboveor next to the ganglia). In addition, smooth muscle cells containPKC $gamma$ immunoreactivity, which is concentrated in their plasmamembranes. The bright streaks running parallel to the nonimmunoreactivemyenteric ganglion are the immunofluorescence of the membranesof circular muscle cells. Although only the appearance of PKC $gamma$ immunoreactivity in neurons is extremely rare, some very largeaxonal varicosities are PKC $gamma$ -immunoreactive (arrowhead). F, Calbindinimmunoreactivity (visualized with TRITC) is demonstrated in thesame section as shown in E. Note that neither the calbindin-immunoreactiveneuronal cell bodies within the ganglion nor the calbindin-immunoreactiveaxons in the interganglionic connectives are PKC $gamma$ - immunoreactive.The very large PKC $gamma$ -immunoreactive varicosities are not calbindin-immunoreactive(compare with E). Scale bars, 30 µm.
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DISCUSSION
The current studies confirm that the slow response of AH/type 2 neurons [inhibition of gK_Ca (Galligan, 1995)] to 5-HT is linkedto G_o and cooperatively mediated by PKA and PKC. Evidence thatthis response is G_o-linked includes: (1) inhibition by intracellularinjection of GDP $beta$ S and potentiation/prolongation by GTP $gamma$ S; (2)sensitivity to PTx; (3) activation, by 5-HT_1P agonists, of G_o,but not of other G-proteins (Wang et al., 1996); (4) antagonismby intracellular injection of anti-G $alpha$ _o Fab fragments of slow responsesto 5-HT but not to histamine, or antagonism of fast, 5-HT₃-mediatedresponses to 5-HT; and (5) the presence of G $alpha$ _o immunoreactivityon the plasma membranes of many neurons in both plexuses, includingall of those that express the AH/type 2 cell marker calbindin.Evidence that PKC plays a role in mediating slow responses to5-HT includes: (1) mimicry by the PKC activators, PDBu, ( $-$ )-7-octylindolactamV, and OAG; (2) antagonism by PKC inhibitors that have littlein common besides their ability to inhibit PKC, including staurosporine,K-252a, G_ö 6976, chelerythrine,and the pseudosubstrate peptides myr-FARKGALRQ and PKC_[19-31](by intracellular injection), as well as by (3) overnight exposureto PDBu to downregulate PKC; and (4) the concentration-dependentinduction by 5-HT of PKC translocation into membranes in isolatedmyenteric ganglia. Evidence that PKA participates in mediatingslow responses to 5-HT includes: (1) antagonism by the selectivePKA inhibitor Rp-cAMPS of slow responses to 5-HT, histamine, andforskolin, but not those to PDBu; and (2) interference by Rp-cAMPSwith inhibition of the AH by 5-HT.

G_o is not commonly linked to the activation of PKC and PKA. Because the selective PC-PLC inhibitor D609 antagonizes slow responsesto 5-HT, it seems likely that the coupling of G_o to PKC is mediatedby PC-PLC. The activity of this enzyme generates DAG, which activatesPKC without simultaneously releasing IP₃ (Schütze et al., 1992),as would a phosphatidylinositol-specific isozyme. Because theslow response to 5-HT involves the inhibition of gK_Ca (Galligan,1995), the liberation of IP₃ would be counterproductive, becauseIP₃ would be expected to increase intracellular Ca²⁺ (Exton, 1994). In fact, the P₂ purinoceptor-induced elevationof intracellular Ca²⁺ is associated with effects, a membrane hyperpolarization anddecreased input resistance, that are the converse of the slowresponse to 5-HT (Palmer et al., 1987a; Christofi et al., 1995).The 5-HT_1P-related activation of PKA is probably stimulated byan adenylate cyclase-mediated elevation of cAMP, because slowresponses are antagonized by the adenylate cyclase inhibitor DDAand 5-HT increases cAMP in isolated myenteric ganglia (Xia etal., 1991, 1994; Fiorica-Howells et al., 1993). Slow responsesto 5-HT are also mimicked by forskolin (Nemeth et al., 1986) andby analogs of cAMP (Zafirov et al., 1985a; Palmer et al., 1986).Despite these observations, available evidence suggests that G_sis not responsible for the 5-HT-induced activation of adenylatecyclase. When applied to isolated myenteric ganglia, 5-HT activatesG $alpha$ _o, but not G $alpha$ _s, (Wang et al., 1996). The adenosine-induced stimulationof G $alpha$ _i does not inhibit slow responses to 5-HT (or slow EPSPs)(Palmer et al., 1987b), but it does block slow responses to forskolin,histamine, vasoactive intestinal peptide, or pituitary adenylatecyclase activating peptide (Zafirov et al., 1985b; Palmer et al.,1987a,b; Christofi and Wood, 1993). Because adenylate cyclasethus appears to be involved in mediating both the G $alpha$ i-resistantslow responses to 5-HT and the G $alpha$ _i-sensitive slow responses toforskolin, histamine, vasoactive intestinal peptide, or pituitaryadenylate cyclase activating peptide, the activation of adenylatecyclase associated with the response to 5-HT must differ fromthat associated with forskolin or compounds that probably actvia receptors linked to G_s. PKC is known to be able to activatetype II adenylate cyclase (Jacobowitz et al., 1993; Yoshimuraand Cooper, 1993); moreover, when adenylate cyclase is activatedby PKC, instead of by G $alpha$ _s or forskolin, it is not inhibited byG $alpha$ _i (Pieroni et al., 1993). These considerations suggest thatthe following signal transduction pathway may be responsible forthe slow response to 5-HT: 5-HT $right-arrow$ 5-HT_1P receptor $right-arrow$ activatesG_o $right-arrow$ activates PC-PLC $right-arrow$ liberates DAG $right-arrow$ stimulates PKC $right-arrow$ activatesadenylate cyclase $right-arrow$ elevates cAMP $right-arrow$ stimulates PKA. Because theslow response to 5-HT is not abolished by inhibitors of PKA orPKC alone but by their combination, PKA and PKC probably eachinhibit gK_Ca. Why PKC inhibitors or downregulation do not eliminatethe slow response to 5-HT is not clear. Conceivably, a Ca²⁺-independent novel or atypical isozyme of PKC, in addition toone of the classical (group A) Ca²⁺-dependent PKC isozymes, becomes activated by 5-HT and is notfully inactivated by PKC inhibitors or downregulation.

Immunocytochemical studies indicated that PKC $alpha$ is present in most of the neurons of both submucosal and myenteric plexuses.In fact, the distribution of the immunoreactivities of G $alpha$ _o andPKC $alpha$ was similar and each was found in virtually every cell thatdisplayed calbindin immunoreactivity, investigated as an AH/type2 cell marker (Furness et al., 1990). In contrast, enteric neuronscontained no PKC $beta$ 1 or $beta$ 2 immunoreactivity and PKC $gamma$ immunoreactivitywas observed only in rare myenteric neurons, none of which werecalbindin immunoreactive. Because many neurons in each plexusand most AH/type 2 neurons exhibit the slow response to 5-HT,PKC $alpha$ is the only classical (group A) isozyme of PKC that is distributedin a manner consistent with a role in transduction of 5-HT_1P-mediatedslow responses. Subject to the limitation that the proteins mighthave been present in forms or quantities that could not be detectedby immunocytochemistry, the $beta$ 1, $beta$ 2, and $gamma$ isozymes thus are unlikelyto be involved in transducing the slow response. The distributionof the immunoreactivity of the novel (group B) isozyme PKC $delta$ ,however, was found to be very similar to that of PKC $alpha$ . Again,many neurons in each plexus and all calbindin-immunoreactive neuronswere PKC $delta$ immunoreactive. PKC $delta$ is thus also a candidate to playa role in the slow response to 5-HT. In contrast, the distributionsof neither PKC $epsilon$ , nor any of the atypical isozymes of PKC, $zeta$ , $iota$ / $lambda$ , and $eta$ , were compatible with roles in 5-HT slow response signaltransduction. These observations suggest that only the $alpha$ and $delta$ PKC isozyme are potential participants in transduction of slowresponses to 5-HT. At least some of the PKC inhibitors that werefound to antagonize slow responses to 5-HT, however, includingG_ö 6976 and the pseudosubstratepeptides FARKGALRQ and PKC_[19-31] are specificfor the $alpha$ and $beta$ isozymes of PKC and have little or no activityagainst PKC $delta$ . The $beta$ PKC isozymes, moreover, are evidently notpresent in enteric neurons; thus, these data suggest that PKC $alpha$ is probably primarily responsible for transducing the 5-HT_1P-mediatedslow response. Although PKC $alpha$ is Ca²⁺-sensitive and intracellular Ca²⁺ is unlikely to increase during slow responses to 5-HT, the constitutivelevel of cytosolic Ca²⁺ may be sufficient to support the activation of PKC $alpha$ by DAG,which increases the affinity of PKC for Ca²⁺ (Nishizuka, 1992; Tanaka and Nishizuka, 1994). Conceivably, localelevations of intracellular Ca²⁺ could occur, which could enhance stimulation of PKC $alpha$ withoutcontributing to gK_Ca.

Many characteristics of slow responses to 5-HT are similar to those that have been reported previously for slow EPSPs. Forexample, slow EPSPs are potentiated by GTP $gamma$ S, mimicked by forskolinand PDBu, and inhibited by D609 and staurosporine (Bertrand andGalligan, 1995). No studies have yet been carried out to determinewhether slow EPSPs are, like slow responses to 5-HT, affectedby GDP $beta$ S, antibodies to G $alpha$ _o, or inhibitors of adenylate cyclaseor PKA. The one difference between slow responses to 5-HT andslow EPSPs is that only slow EPSPs have been reported to be PTx-resistant(Bertrand and Galligan, 1995). When slow EPSPs were studied, however,PTx was applied extracellularly for only 2 hr, whereas in thecurrent investigation, at least 4 hr of exposure was found tobe required before PTx inhibited slow responses to 5-HT. It ispossible, therefore, that slow EPSPs might actually be PTx-sensitivebut not observed to be so, because insufficient time was allowedfor PTx to become effective. Both the slow response to 5-HT andslow EPSPs are resistant to inhibition by adenosine (Palmer etal., 1987b). The resistance of slow EPSPs to inhibition by adenosineimplies that they are, like slow responses to 5-HT, G $alpha$ _i-resistant.Thus it seems unlikely that any receptor that induces a slow EPSPcould be coupled by a G_s protein to adenylate cyclase; nevertheless,because 5-HT is only one of the transmitters that mediate slowEPSPs (Bornstein et al., 1984), the observation that PTx did notinhibit slow EPSPs (Bertrand and Galligan, 1995) could also beexplained by the existence of subsets of slow EPSPs transducedby different transmitters using receptors coupled to differentG-proteins. Given the many other identities between slow EPSPsand slow responses to 5-HT, however, it seems premature to postulatesubsets of slow EPSPs triggered by different G-proteins.

FOOTNOTES

Received July 3, 1996; revised Oct. 21, 1996; accepted Nov. 22, 1996.

This work was supported by National Institutes of Health Grant NS12969. H.P. is a fellow of the Pharmaceutical ManufacturersAssociation Foundation.

Correspondence should be addressed to Dr. Hui Pan, Department of Anatomy and Cell Biology, Columbia University (P&S 12-513),630 West 168th Street, New York, NY 10032.

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