Positive Modulation of Pepsinogen Secretion by Gastric Acidity After Vagal Cholinergic Stimulation

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Vol. 283, Issue 3, 1043-1050, 1997

Positive Modulation of Pepsinogen Secretion by Gastric Acidity After Vagal Cholinergic Stimulation¹

Corrado Blandizzi, Rocchina Colucci, Diego Carignani, Gloria Lazzeri and Mario Del Tacca

Division of Pharmacology and Chemotherapy, Department of Oncology, University of Pisa, Pisa, Italy

	Abstract

Abstract Introduction Materials & Methods Results Discussion References

Parallel increments of gastric acid and pepsinogen secretion generally occur after the application of cholinergic stimuli.However, it still remains to be established whether the changesin acid output associated with cholinergic stimulation play arole in regulation of the concomitant peptic secretory activity.In the present study, an anesthetized rat model was used for theevaluation of pepsinogen secretion in order to pursue a dual purpose:1) to assess the relative functional relevance of direct and acid-dependentcontrol exerted by cholinergic pathways on pepsinogen output;2) to characterize the mechanisms through which changes in aciditywithin the stomach lumen may affect the peptic secretory activityof gastric mucosa. Bethanechol, 2-deoxy-D-glucose or electricalvagal stimulation caused parallel and atropine-sensitive incrementsof peptic and acid secretions. Omeprazole, a selective inhibitorof gastric H⁺:K⁺-adenosintriphosphatase, blocked the increase in acid but notpepsinogen secretion induced by bethanechol. However, 2-deoxy-D-glucoseor electrical vagal stimulation failed to increase either pepsinogenor acid secretion in omeprazole-pretreated rats. When tested inanimals pretreated with both omeprazole and physostigmine (a drugable to prevent the enzymatic breakdown of vagally released AChthrough the blockade of acetylcholinesterase), 2-deoxy-D-glucoseor electrical vagal stimulation significantly increased pepsinogensecretion without affecting acid secretion. In omeprazole-pretreatedrats, perfusion of the gastric lumen with acid solutions causeda pH-dependent and atropine-sensitive increase in peptic outputonly when applied in combination with electrical vagal stimulation.Functional ablation of capsaicin-sensitive sensory neurons didnot modify the gastric secretory responses induced by bethanecholor electrical vagal stimulation. However, after topical applicationof lidocaine to the gastric mucosal surface, bethanechol stimulatedboth peptic and acid outputs, whereas electrical vagal stimulationonly evoked acid secretion without affecting basal peptic output.The present results indicate that the activation of muscarinicreceptors by vagally released ACh is not sufficient by itselfto stimulate pepsinogen secretion and that a facilitatory actionmediated by acid secretion is necessary to allow an incrementof peptic output in response to vagal cholinergic stimuli. Itis suggested that such facilitatory input is driven to chief cellsby local intramural reflexes that involve capsaicin-insensitiveintrinsic nerves.

	Introduction

Abstract Introduction Materials & Methods Results Discussion References

Vagal cholinergic stimuli and muscarinic receptor agonists evoke parallel increments of gastric acid and pepsinogen secretionsin a variety of experimental models as well as in humans (Hersey,1987; Smith and Torres, 1990; Hirschowitz and Groarke, 1993).However, although a great deal is known about the control of acidsecretion mediated by cholinergic pathways (Hirschowitz and Groarke,1993; Lloyd and Debas, 1994; Welsh et al., 1994), the mechanismsthat account for the in vivo regulation of peptic secretion arestill unclear (Basson et al., 1988; Raufman, 1992). In particular,it is matter of debate whether the changes in acid output associatedwith cholinergic stimulation might play any role in regulationof the concomitant peptic secretory activity (Basson et al., 1988;Smith and Torres, 1990).

Several studies, based on binding, molecular biology and functional techniques, have shown that both gastric chief cells andparietal cells are provided with muscarinic receptors, the activationof which increases intracellular calcium concentration and leadsto subsequent stimulation of pepsinogen and acid secretions, respectively(Raufman, 1992; Hersey, 1994; Soll and Berglindh, 1994). In addition,pharmacological experiments performed on isolated rat stomachdemonstrated that gastric glands receive direct innervation fromcholinergic fibers (Welsh et al., 1994). These findings wouldsuggest that endogenous ACh, released from vagal cholinergic fibers,causes a parallel stimulation of pepsinogen and acid secretionsthrough a simultaneous activation of muscarinic receptors locatedon chief cells and parietal cells, respectively (Hersey, 1994;Soll and Berglindh, 1994). However, both in vivo and in vitrostudies indicated that pepsinogen secretion in response to stimulationof chief cells appears to require a flow of water and acid fromadjacent parietal cells (Hersey, 1987; Sandvik et al., 1987) andthat acidity in the stomach lumen is able to stimulate the pepsinogenoutput from gastric mucosa (Johnson, 1972; Smith and Torres, 1990).This suggests that changes in local hydrogen ion concentrationevoked by cholinergic stimulants might be, at least in part, responsiblefor the parallel variations of the peptic secretory output.

Previous attempts to discriminate between direct and acid-dependent cholinergic control of pepsinogen secretion were basedmainly on the use of in vitro experimental models (Hersey et al.,1983; Sandvik et al., 1987; Basson et al., 1988). However, undersuch conditions an assessment of the secretory actions mediatedby endogenously released ACh is not usually allowed, and the effectsof hydrogen ions on chief cells cannot be clearly establishedbecause of methodological problems related to the presence ofincubation media (Basson et al., 1988). In addition, data concerningthe putative changes of peptic output induced by gastric lumenacidification after suppression of endogenous acid productionare still lacking.

Therefore, in the present study, an in vivo gastric preparation was used for the evaluation of pepsinogen secretion, underdifferent experimental conditions, to pursue a dual purpose: 1)to assess the relative functional relevance of direct and acid-dependentcontrol exerted by cholinergic pathways on pepsinogen output afterthe activation of muscarinic receptors by endogenous ACh or anexogenously administered muscarinic agonist; 2) to characterizethe mechanisms through which changes in acidity within the stomachlumen may affect the peptic secretory activity of gastric mucosa.

	Materials and Methods

Abstract Introduction Materials & Methods Results Discussion References

Animals

The experiments were carried out on male Wistar rats weighing 200 to 220 g. The animals were fed standard laboratory chowand tap water ad libitum and were not used for at least 1 weekafter their delivery to the laboratory. The animals were housed,six in a cage, in temperature-controlled rooms on a 12-h lightcycle at 22-24°C and 50-60% humidity. Their care and handlingwere in accordance with the provisions of the European EconomicCommunity (EEC) Council Directive 86-609, recognized and adoptedby the Italian government. Twenty-four hours before the experiments,the animals were maintained in single cages provided with wirenet bottoms and were deprived of food. Free access to water wasallowed until 1 h before the experiment.

Perfusion of the Gastric Lumen in Anesthetized Rats

Continuous perfusion of the rat stomach in situ was carried out, following the procedure previously reported (Blandizzi etal., 1995). The animals were anesthetized with urethane (1.2 g/kg)administered i.p., and the trachea was surgically exposed andcannulated by a polyethylene catheter to ensure a patent airway.A polyethylene catheter was introduced into the esophagus andadvanced as far as 5 mm beyond the gastroesophageal junction.After a midline laparotomy, the proximal duodenum was exposedand its wall incised. Then a second polyethylene catheter wasintroduced into the duodenum and pushed forward until its tipwas about 5 mm beyond the pylorus. The stomach lumen was perfusedcontinuously at a rate of 1 ml/min with saline solution (154 mMNaCl) at 37°C (pH = 7.0 ± 0.2) unless otherwise stated, and 15-mineffluent fractions were collected. The effluent samples were usedfor the quantitative evaluation of both pepsinogen and acid secretions.

Evaluation of Pepsinogen and Acid Secretion

Pepsin levels in the gastric effluent were determined as previously reported (Blandizzi et al., 1995). Briefly, 2 ml of 2.5%bovine hemoglobin plus 0.5 ml of 0.3 N HCl and 0.5 ml of gastriceffluent were maintained in separate tubes at 37°C for 10 minand then mixed. Mixtures were incubated for 10 min at 37°C, andthe reaction was stopped by the addition of 5 ml 0.3 N trichloroaceticacid. After agitation and filtration, optical density was measuredat 280 nm by an Uvikon 930 Spectrophotometer (Kontron Instruments,Milan, Italy). The results were compared to a standard curve,which was generated in an identical manner using known amountsof porcine pepsin (1 µg = 3 peptic units), and were expressedas micrograms of pepsin. The acidity in the gastric perfusatewas measured with an autotitrator pH meter (PHM 85, Radiometer,Copenhagen, Denmark) by automatic potentiometric titration topH 7.0 with 0.01 N NaOH and was expressed as µEqH⁺.

After the surgical preparation of animals, basal gastric secretion was allowed to stabilize for 30 min. At the end of thisperiod, we collected two consecutive 15-min effluent fractionsto assess basal secretory values. Both pepsinogen and acid secretionswere then monitored at 15-min intervals for an additional 120min. The peptic and acid outputs obtained during the 120-min periodafter the collection of basal effluent samples were calculatedand expressed as µg of pepsin/120 min and µEqH⁺/120 min, respectively.

Experimental Procedures

Effects of bethanechol, of 2DG and of electrical vagal stimulation under basal secretory conditions. The first set of experiments was carried out on rats with intact vagus nerves. The gastric secretory activity of these animalswas evoked by bethanechol (0.3, 1 and 3 mg/kg), a well-known muscarinicreceptor agonist, or 2DG (200 mg/kg), a centrally acting stimulantof vagal efferent cholinergic pathways (Eisenberg et al., 1966).Both these drugs were administered i.v. as a bolus immediatelyafter the collection of basal effluent samples.

The second series of experiments was performed on rats whose vagus nerves were carefully separated from the carotid arteriesand cut at the cervical level 30 min before the collection ofbasal effluent samples began. The effects of bethanechol or 2DGon gastric secretions were reassessed in animals that underwentthis vagotomy procedure. In addition, in a group of vagotomizedanimals, the distal end of the left vagus nerve was placed ona bipolar platinum electrode and immersed in paraffin oil. Inthis case, after the collection of basal effluent samples, thegastric peptic and acid secretions were evoked by continuous electricalstimulation of the left vagus nerve (120 min). The stimulus parameterswere square-wave pulses 0.5 ms in duration, delivered at 5 Hzwith supramaximal intensity (10 V) by means of a Grass S5 stimulator(Grass Instruments, Quincy, MA) (Blandizzi et al., 1992

Effects of bethanechol, of 2DG and of electrical vagal stimulation in animals pretreated with omeprazole. A group of experiments was designed to assess the effects of bethanechol, of 2DG and of electrical vagal stimulation on pepsinogensecretion in the presence of a complete blockade of the acid secretoryfunction of gastric parietal cells. For this purpose, 90 min beforethe collection of basal effluent samples began, animals were pretreatedwith omeprazole (30 mg/kg i.v.), a benzimidazole derivative thatinhibits gastric acid secretion through a selective blockade ofH⁺:K⁺-adenosin-triphosphatase (Fellenius et al., 1981) without interferingwith receptor or signal transduction pathways of gastric secretorycells (Clissold and Campoli-Richards, 1986). The dose of omeprazolewas selected because of its ability to suppress acutely both basaland stimulated gastric acid secretion in anesthetized rats (Blandizziet al., 1995).

Effects of perfusion of the gastric lumen with acid solutions. The influence exerted on pepsinogen secretion by topical application of acid solutions at various pH on the surface of gastricmucosa was studied both under basal conditions and in the presenceof electrical vagal stimulation. In this case, the anesthetizedrats first were pretreated with omeprazole, to suppress endogenousacid production, and then were subjected to bilateral cervicalvagotomy. Perfusion of the gastric lumen was performed with salineup to the collection of basal effluent samples and then was continueduntil the end of the experimental period with one of the followingacid solutions: 0.1 mM HCl plus 153.9 mM NaCl (pH = 4.0); 1 mMHCl plus 153 mM NaCl (pH = 3.0); 10 mM HCl plus 144 NaCl (pH =2.0); 100 mM HCl plus 54 mM NaCl (pH = 1.0).

Effects of bethanechol and of electrical vagal stimulation on animals subjected to systemic capsaicinization or intragastric application of lidocaine. A group of experiments was designed to assess whether bethanechol and whether electrical vagal stimulation was able to affectgastric pepsinogen and acid secretions from vagotomized rats inthe presence of a systemic ablation of capsaicin-sensitive sensorynerve fibers. For this purpose, some animals were given a doseof 125 mg/kg capsaicin s.c., as previously reported by Pabst etal. (1993). Ten days after this treatment, the animals were usedfor the assessment of gastric pepsinogen and acid secretions.One day before the experiment, the efficacy of capsaicin treatmentwas checked by instilling a drop of a capsaicin solution (0.1mg/ml in saline solution) into one eye of each rat. Capsaicin-treatedrats were expected not to react by wiping their eyes, but wheneveran animal responded with wiping, the afflicted eye was immediatelyand extensively rinsed with water.

An additional series of experiments was performed to investigate the effects of bethanechol and of electrical vagal stimulationon both pepsinogen and acid secretions from vagotomized rats aftertopical application of the local anesthetic lidocaine to the gastricmucosal surface. In this case, pre-exposure of the gastric mucosato lidocaine was carried out according to the procedure reportedby Mercer et al. (1994)

with minor modifications. After the collectionof two basal effluent samples, the perfusion was interrupted,and the gastric lumen was gently emptied and then filled with3 ml of 4% lidocaine. Fifteen minutes later the stomach was emptied,rinsed by gently flushing with 6 ml of saline and filled againwith 3 ml of saline. Perfusion of the gastric lumen with salinewas then resumed and continued up to the end of the experimentalperiod. An interval of 5 min was allowed to elapse between therestart of gastric perfusion and either bethanechol injectionor electrical vagal stimulation.

Effects of physostigmine and atropine. In some experiments the enzymatic breakdown of vagally released ACh was prevented in order to promote its accumulation overphysiological concentrations. For this purpose, 5 min before theyreceived 2DG injection or electrical vagal stimulation, some animalswere treated with the acetylcholinesterase inhibitor physostigmine(1 mg/kg i.v.). In those experiments where the involvement ofmuscarinic receptors in the gastric secretory responses was assessed,atropine 1 mg/kg i.v. was always administered 5 min before collectionof the second basal effluent sample ended.

Drugs

The following drugs and reagents were used: urethane ethyl carbamate, crystalline porcine pepsin, lyophilized bovine hemoglobin,bethanechol chloride, 2DG, physostigmine sulfate, capsaicin, aminophylline,terbutaline, lidocaine (Sigma, St. Louis, MO), omeprazole (kindlyprovided by Malesci, Florence, Italy) and atropine sulfate (BDHChemicals, Poole, England). Other reagents were of analyticalgrade. Bethanechol, 2DG, atropine, physostigmine and lidocainewere dissolved in saline immediately before use. Omeprazole wasinitially dissolved in polyethyleneglycole (PEG, molecular weight= 400) and then diluted with 7 mM NaHCO₃ to a final concentrationof 50% PEG (v/v). All drugs administered i.v. were injected ina volume of 0.25 ml/rat. Capsaicin was dissolved (12.5 mg/ml)in a vehicle composed by 10% ethanol, 10% Tween 80 and 80% salinesolution (v/v/v). The total dose of capsaicin (125 mg/kg s.c.)was administered under ether anesthesia in four injections overtwo consecutive days (first day: 25 mg/kg in the morning and 25mg/kg in the late afternoon; second day: 25 mg/kg in the morningand 50 mg/kg in the late afternoon). To counteract the respiratoryimpairment associated with the administration of capsaicin, ratsreceived atropine (0.2 mg/kg i.p.), terbutaline (0.2 mg/kg i.p.)and aminophylline (20 mg/kg i.p.) 10 min before the first andthird capsaicin injections.

Statistics

Results are given as mean ± S.E. The significance of differences was evaluated by Student' t test or one-way analysis of variance(ANOVA) followed by post-hoc analysis by Student-Newman-Keuls'test, and P values less than .05 were considered significant;n indicates the number of experiments.

	Results

Abstract Introduction Materials & Methods Results Discussion References

Evaluation of basal pepsinogen and acid secretions. In control animals with intact vagus nerves (n = 6), basal gastric pepsinogen and acid secretions, assessed after a 30-minstabilization, accounted for 59.8 ± 10.1 µg of pepsin/15 min and3.2 ± 0.8 µEqH⁺/15 min, respectively, and these values remained nearly constantuntil the end of the experiments (120 min). In addition, whencontrol animals underwent bilateral cervical vagotomy (n = 6),basal pepsinogen and acid secretions accounted for 54.8 ± 9.1µg of pepsin/15 min and 3.3 ± 0.9 µEqH⁺/15 min, respectively. These values did not differ significantlyfrom those obtained in control rats with intact vagus nerves,and they remained at a steady level throughout the experiment.

In a series of preliminary experiments, both basal pepsinogen and acid outputs were monitored in rats, with or without intactvagus nerves, after pretreatment with omeprazole or atropine (n= 6 for each drug). An almost complete inhibition of basal acidsecretion, but not of peptic output, was detected only in ratsundergoing pretreatment with omeprazole; atropine did not significantlyaffect basal peptic or acid secretory activities (fig. 1).

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Fig. 1. Anesthetized rats with perfused gastric lumen. Effects of omeprazole 30 mg/kg i.v. (OME), of atropine 1 mg/kg i.v. (ATR),of bilateral cervical vagotomy (VAG), of omeprazole 30 mg/kg i.v.plus vagotomy (OME + VAG) and of atropine 1 mg/kg i.v. plus vagotomy(ATR + VAG) on basal pepsinogen (panel A) and acid secretion (panelB). Each column represents the mean value obtained from six animals± SE (vertical bars). *P < .05: significant difference from controlvalues (CON).

Effects of bethanechol on pepsinogen and acid secretions. In animals with intact vagus nerves, bethanechol (0.3, 1 and 3 mg/kg i.v.) caused a dose-dependent and parallel increase inboth pepsinogen and acid secretions, the maximal effects occurringat the dose of 1 mg/kg (fig. 2,A and B). The excitatory responseselicited by bethanechol were not significantly affected by bilateralcervical vagotomy, while they were completely prevented by pretreatmentwith atropine (fig. 2,C and D). When administered to rats pretreatedwith omeprazole, bethanechol failed to stimulate acid secretion,but it was still able to evoke an atropine-sensitive increasein pepsinogen output that did not differ from the increase observedin omeprazole-untreated rats (fig. 2,C and D).

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Fig. 2. Anesthetized rats with perfused gastric lumen. Effects of bethanechol 0.3 (BET-0.3), 1 (BET-1) and 3 (BET-3) mg/kg i.v. (panelsA, B), and of bethanechol 1 mg/kg i.v., administered either alone(BET-1) or in the presence of bilateral cervical vagotomy (BET-1+ VAG), atropine 1 mg/kg i.v. (BET-1 + ATR), omeprazole 30 mg/kgi.v. (BET-1 + OME) and omeprazole 30 mg/kg i.v. plus atropine1 mg/kg i.v. (BET + OME + ATR) (panels C, D), on basal pepsinogen(panels A, C) and acid secretion (panels B, D). Each column representsthe mean value obtained from 8 to 10 animals ± S.E. (verticalbars). *P < .05: significant difference from control values (CON);^aP < .05: significant difference from bethanechol 1 mg/kg alone(BET-1).

Effects of 2DG and of electrical vagal stimulation on pepsinogen and acid secretions. In animals with intact vagus nerves, the administration of 2DG (200 mg/kg i.v.) induced significant and simultaneous increasesin pepsinogen and acid outputs (fig. 3,A and B). Both of theseeffects were prevented by bilateral cervical vagotomy as wellas by atropine (fig. 3,A and B). However, in contrast with theresults obtained in the presence of bethanechol, 2DG failed tostimulate either pepsinogen or acid secretion in omeprazole-pretreatedanimals (fig. 3,A and B).

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Fig. 3. Anesthetized rats with perfused gastric lumen. Effects of 2DG 200 mg/kg i.v. (2DG) (panels A, B) or electrical vagal stimulationof the left vagus nerve (EVS: 0.5 ms, 5 Hz, 10 V for 120 min)(panels C, D) on basal pepsinogen (panels A, C) and acid secretion(panels B, D). 2DG was administered either alone or in the presenceof bilateral cervical vagotomy (2DG + VAG), atropine 1 mg/kg i.v.(2DG + ATR), or omeprazole 30 mg/kg i.v. (2DG + OME) (panels A,B). Electrical vagal stimulation was applied either alone or inthe presence of atropine 1 mg/kg i.v. (EVS + ATR) or omeprazole30 mg/kg i.v. (EVS + OME) (panels C, D). Each column representsthe mean value obtained from 8 to 10 animals ± S.E. (verticalbars). *P < .05: significant difference from control values (CON);^a P < .05: significant difference from either 2DG alone (panelsA, B) or EVS alone (panels C, D).

Both pepsinogen and acid outputs increased simultaneously after the application of electrical stimulation to the left vagusnerve, and these effects were completely prevented by atropine.However, analogously to 2DG, electrical vagal stimulation wasalso not able to modify basal pepsinogen or acid secretions afterpretreatment of animals with omeprazole (fig. 3,C and D).

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Fig. 4. Anesthetized rats with perfused gastric lumen and pretreatment with physostigmine. Effects of 2DG 200 mg/kg i.v. (2DG) (panelsA, B) or electrical stimulation of the left vagus nerve (EVS:0.5 ms, 5 Hz, 10 V for 120 min) (panels C, D) on basal pepsinogen(panels A, C) and acid secretion (panels B, D). 2DG was administeredeither alone or in the presence of atropine 1 mg/kg i.v. (2DG+ ATR), omeprazole 30 mg/kg i.v. (2DG + OME) or omeprazole 30mg/kg i.v. plus atropine 1 mg/kg i.v. (2DG + OME + ATR) (panelsA, B). Electrical vagal stimulation was applied either alone orin the presence of atropine 1 mg/kg i.v. (EVS + ATR), omeprazole30 mg/kg i.v. (EVS + OME) or omeprazole 30 mg/kg i.v. plus atropine1 mg/kg i.v. (EVS + OME + ATR) (panels C, D). Each column representsthe mean value obtained from 8 to 10 animals ± S.E. (verticalbars). *P < .05: significant difference from control values (CON);^a P < .05: significant difference from either 2DG alone (panelsA, B) or EVS alone (panels C, D).

In animals where the enzymatic breakdown of ACh was prevented by acute pretreatment with physostigmine, 2DG injection or electricalvagal stimulation evoked atropine-sensitive increases in bothpeptic and acid outputs (fig. 4). However, whereas acid secretionin response to 2DG or vagal stimulation did not differ from thatobtained in physostigmine-untreated rats, the increments in pepticvalues were higher in the presence of physostigmine than in itsabsence (P < .05), and they were similar to those induced by bethanechol1 mg/kg in physostigmine-untreated animals. In addition, whenphysostigmine was administered to animals pretreated with omeprazole,both 2DG and vagal stimulation were still able to induce markedand atropine-sensitive increments in pepsinogen secretion (fig.4,A and C), although they did not exert any stimulant action onacid output (fig. 4,B and D). These peptic responses did not differfrom that obtained after bethanechol injection to omeprazole-pretreatedrats.

Effects of perfusion of the gastric lumen with acid solutions. The influence on pepsinogen secretion exerted by topical intragastric application of solutions with different pH values wasstudied in animals subjected to bilateral cervical vagotomy andpretreatment with omeprazole. Under these conditions, perfusionof the gastric lumen with solutions at pH 4.0, 3.0, 2.0 or 1.0did not modify basal pepsinogen secretion (fig. 5A). However,when gastric perfusion with one of these solutions was carriedout in combination with electrical stimulation of the left vagusnerve, the pepsinogen output increased in a pH-dependent manner,the maximal increment occurring at pH 2.0 (fig. 5B). Pretreatmentwith atropine prevented the peptic response evoked by gastricperfusion with acid solution at pH 2.0 combined with electricalvagal stimulation (fig. 5B).

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Fig. 5. Anesthetized rats with perfused gastric lumen, bilateral cervical vagotomy and pretreatment with omeprazole. A) Pepsinogensecretion in the presence of intraluminal perfusion with solutionsat pH 7, 4, 3, 2 or 1. B) Pepsinogen secretion in the presenceof electrical stimulation of the left vagus nerve (0.5 ms, 5 Hz,10 V for 120 min) plus intraluminal perfusion with solutions atpH 7, 4, 3, 2 or 1 or with solution at pH 2 after pretreatmentwith atropine 1 mg/kg i.v. (pH 2 + ATR). Each column representsthe mean value obtained from 6 to 8 animals ± S.E. (vertical bars).*P < .05: significant difference from values obtained at pH 7;^a P < .05: significant difference from values obtained at pH 2.

Effects of bethanechol and of electrical vagal stimulation on pepsinogen and acid secretions after pretreatment with capsaicin or lidocaine. The functional ablation of capsaicin-sensitive sensory neurons by systemic pretreatment with capsaicin did not significantlymodify basal gastric secretions and failed also to affect thestimulant actions of bethanechol or electrical vagal stimulationon pepsinogen and acid outputs (fig. 6,A and B).

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Fig. 6. Anesthetized rats with perfused gastric lumen and bilateral cervical vagotomy. Effects of systemic capsaicinization (

) orintragastric application of lidocaine (

) on pepsinogen (A) oracid secretion (B) under basal conditions, treatment with bethanechol1 mg/kg i.v. (BET-1) or electrical stimulation of the left vagusnerve (EVS: 0.5 ms, 5 Hz, 10 V for 120 min). Each column representsthe mean value obtained from 8 animals ± S.E. (vertical bars).*P < .05: significant difference from basal values; ^a P < .05: significant difference from control values (

In animals whose gastric mucosa was exposed to lidocaine, both basal peptic and acid outputs did not differ significantlyfrom those measured in lidocaine-untreated animals. In addition,after topical application of lidocaine to the gastric mucosalsurface, bethanechol increased both pepsinogen and acid secretionsto an extent similar to that induced by the same drug in lidocaine-untreatedrats (fig. 6,A and B). However, under the same conditions, electricalstimulation of the left vagus nerve caused a significant increasein acid secretion without affecting basal pepsinogen output (fig.6,A and B).

	Discussion

Abstract Introduction Materials & Methods Results Discussion References

Current interest in studying the mechanisms underlying the regulation of gastric pepsin secretion arises from recognitionof the relevant role played by this enzyme in the pathophysiologyof various digestive disorders, including peptic ulcer (Samloff,1989; Raufman, 1992) and gastritis associated with Helicobacterpylori infection (Cave and Cave, 1991; Lamers, 1992). As far asthe cholinergic control of pepsinogen secretion is concerned,it is known that a parallel increase in peptic and acid outputsgenerally occurs after the application of cholinergic stimuli(Smith and Torres, 1990; Hirschowitz and Groarke, 1993), but itremains to be established whether peptic hypersecretion dependsmainly on a direct activation of chief cells or on a stimulantaction exerted on these cells by the concomitant increase in acidsecretory output (Basson et al., 1988; Raufman, 1992). In thepresent study, it was possible to dissociate direct from acid-dependentcholinergic regulation of pepsinogen secretion, and we obtainedevidence that the secretory response of chief cells to endogenousACh is driven by the parallel increment of acid output.

The present results showing that, despite a total inhibition of acid output, the basal pepsinogen secretion continued unchangedafter treatment of animals with omeprazole, are in agreement withfindings obtained from fundic mucosal sheets (Basson et al., 1988)and suggest that in the present model, the basal pepsinogen outputis independent of acid secretion. It must be noted also that inthis preparation, the anesthesia with urethane depresses the vagalcholinergic outflow to the stomach (Maggi and Meli, 1986). Accordingly,atropine or bilateral cervical vagotomy did not modify basal pepticand acid outputs, which indicates that the anesthetized animalis not subjected to an endogenous tonic cholinergic control, andtherefore it represents an useful model to test the influenceof applied cholinergic stimuli on gastric secretory functions.It has also been reported that urethane stimulates both synthesisand release of gastric somatostatin (Yang et al., 1990). However,with regard to putative interferences elicited by this peptidein the present study, it should be considered that muscarinicreceptors mediate inhibitory effects on somatostatin secretion(Del Tacca et al., 1987), so the application of cholinergic stimuliwas expected to counterbalance the somatostatin-releasing actionof urethane. In addition, because an increase in gastrin releasemay occur as a consequence of omeprazole administration (Wildeand McTavish, 1994), the presence of a somatostatin backgroundmight have counteracted the possible interference of gastrin inthe excitatory effects evoked by cholinergic stimuli.

Putative differences in the peptic response of chief cells to the application of an exogenous cholinergic agonist or to therelease of endogenous ACh were investigated in experiments wheregastric secretion was elicited by bethanechol, 2DG or electricalvagal stimulation, either in the absence or in the presence ofomeprazole. In the absence of omeprazole, these stimulants inducedparallel and atropine-sensitive increments of both peptic andacid outputs, which indicates the involvement of muscarinic receptors.However, quite surprising results were obtained when the samestimuli were applied after blockade of acid secretion by omeprazole.Under these conditions, bethanechol was still able to evoke anatropine-sensitive increase in pepsinogen secretion, whereas neither2DG nor electrical vagal stimulation affected basal peptic output.These findings are compatible with the hypothesis that below athreshold level of muscarinic receptor activation, acid secretionmay exert an excitatory influence on the peptic secretory responseof chief cells to cholinergic stimuli. In particular, the resultsobtained in the presence of omeprazole suggest that a backgroundof acid secretion plays a pivotal role in facilitating peptichypersecretion promoted by endogenous ACh concentrations, whichare likely to lead to submaximal and/or short-lasting occupationof muscarinic receptors. In contrast, according to our data aswell as those yielded by previous in vitro studies (Hersey etal., 1983; Basson et al., 1988), acid secretion does not appearto be necessary to increase the pepsinogen secretion when muscarinicreceptors are activated by pharmacological concentrations of exogenousagonists, such as bethanechol or carbachol, and it rather appearsthat parietal cells and chief cells can be stimulated simultaneouslyby these agents only by virtue of sharing similar receptors (Bassonet al., 1988). In support of this view, in animals where endogenousACh concentrations were raised to pharmacological levels by pretreatmentwith physostigmine, both the injection of 2DG and the stimulationof vagus nerve induced marked and atropine-sensitive incrementsin pepsinogen secretion regardless of whether omeprazole-inducedacid inhibition was present.

In the present study, a series of experiments was designed in the attempt to gain more insight into the mechanisms underlyingthe in vivo interaction between hydrogen ions and chief cells.For this purpose, we took care to suppress endogenous acid productionby pretreatment with omeprazole, and the gastric mucosal surfacewas continuously irrigated with iso-osmotic solutions at pH rangingfrom 4 to 1. Because under these peculiar conditions a pH-dependentand atropine-sensitive increment of pepsinogen output could beachieved only after electrical stimulation of vagus nerve, itis conceivable that hydrogen ions are not able to promote by themselvesa direct stimulation of pepsinogen secretion but that, rather,they facilitate the activation of chief cells in response to therelease of endogenous ACh. This conclusion is in line with ourdata showing that basal pepsinogen secretion remained unchangedafter suppression of acid secretion by omeprazole, and it is consistentwith the findings of previous studies indicating a lack of directstimulant influence by gastric acidity on the secretory functionof chief cells (Puurunen, 1979; Kleveland et al., 1987). Indeed,no significant changes in basal pepsinogen secretion from urethane-anesthetizedrats were observed after perfusion of the gastric lumen with iso-osmoticNaCl solutions containing HCl from 0.01 to 100 mM (Puurunen, 1979).Analogously, intragastric perfusion with 1 mM HCl failed to affectbasal pepsinogen secretion from isolated and vascularly perfusedrat stomach (Kleveland et al., 1987).

It must be noted also that although observations arguing in favor of a direct pepsigogic action exerted by luminal hydrogenions have been previously reported (Johnson, 1972; Smith and Torres,1990), they probably reflected the occurrence of methodologicalbias. For instance, significant increments of pepsinogen secretionwere detected after topical application of acid solutions to thegastric mucosa in humans (Bynum and Johnson, 1975; Smith and Torres,1990), dogs (Johnson, 1972), cats and rabbits (Descroix-Vagneet al., 1993). In all these cases, however, the peptic responsedid not appear clearly to be related to pH changes, but ratherto concomitant gastric distension or osmotic stimulation by testsolutions (Descroix-Vagne et al., 1993). Accordingly, distensionof the stomach wall and osmolarity of the gastric contents arewell recognized as stimulants of pepsin secretion in differentmammalian species, acting by gastrin release or local cholinergicreflexes (Descroix-Vagne et al., 1993; Sengupta and Gebhart, 1994).In addition, when incubated in the presence of acidified media,isolated gastric gland preparations increased their pepsinogenrelease, but under those conditions, chief cells were subjectedto alterations in intracellular pH that occur only after markedback-diffusion of acid through a damaged gastric mucosal barrier(Norris and Hersey, 1983).

There is evidence in the literature to support the view that changes in hydrogen ion concentration might modulate pepsinogensecretion indirectly by interacting with pH-sensitive mucosalchemoreceptors, which in turn would sensitize chief cells to thestimulant action of endogenous cholinergic pathways. Indeed, electrophysiologicalstudies demonstrated the existence of gastric mucosal receptorsthat respond to low pH in various species (Norris and Hersey,1983; Yamamoto et al., 1994a). In addition, the rat stomach isprovided with two distinct populations of sensory fibers, belongingto either capsaicin-sensitive afferent nerves or capsaicin-insensitiveintrinsic neurons, which can affect some gastric functions inresponse to changes in intraluminal pH (Geppetti et al., 1991).

Because capsaicin-sensitive nerves of the GI mucosa have been implicated in the control of various digestive functions (Sharkeyet al., 1991; Pabst et al., 1993), we attempted first to ascertainwhether capsaicin-sensitive fibers might be involved in the sensitizingaction exerted by hydrogen ions on chief cells. The present data,which show that bethanechol or vagal stimulation was still ableto induce simultaneous increments of acid and peptic outputs afterpretreatment with capsaicin, indicate that systemic capsaicinizationdid not influence the functional status of chief cells and suggestthat capsaicin-sensitive sensory nerves are not implicated inthe mechanisms linking pepsinogen secretion to changes in hydrogenion concentration. In accordance with these findings, Sharkeyet al. (1991) showed that in urethane-anesthetized rats subjectedto vagal stimulation at 4 Hz, the gastric secretory response istotally independent of the activation of capsaicin-sensitive afferentfibers.

In the present study, different results from those obtained after systemic capsaicinization were obtained when gastric mucosawas acutely exposed to lidocaine in order to induce a local surfaceanesthesia. Lidocaine-pretreatment did not impair the abilityof parietal or chief cells to respond to secretory inputs, asdemonstrated by the significant and parallel increase in bothacid and pepsinogen secretions after bethanechol administration.However, under the same conditions, vagal stimulation evoked acidsecretion but did not affect basal peptic output, which suggeststhat mucosal afferent fibers, probably belonging to capsaicin-insensitiveintrinsic neurons, drive an acid-mediated facilitatory input tochief cells, allowing a peptic secretory output in response tothe activation of muscarinic receptors by endogenous ACh. In supportof this view, previous studies indicated that capsaicin-insensitiveintrinsic neurons of rat stomach can be activated by low pH levelsto promote a reflex increase in mucosal blood flow (Geppetti etal., 1991).

Although the existence of a local intramural reflex linking pepsinogen output to changes in acid secretion may represent apossible explanation for our findings, two points remain to beclarified: 1) how gastric intrinsic neurons can detect pH variationsand 2) how these neurons can transmit their information to chiefcells. With regard to the first point, it is hard to believe thatunder normal conditions, hydrogen ions can penetrate the gastricepithelium to reach the free endings of intrinsic sensory fibers,and it is generally considered that such nerve terminals may beconnected to special sensory structures sensitive to acidic pH(Yamamoto et al., 1994a). Accordingly, enteroendocrine or enterochromaffincells of the mucosal epithelium are currently regarded as possibletransducer elements for pH variations (Sengupta and Gebhart, 1994;Yamamoto et al., 1994a), and it has been postulated that, onceactivated by gastric acidification, these cells release a specificfactor that, in turn, stimulates local sensory nerve terminals(Yamamoto et al., 1994b). As far as the second issue is concerned,the activation of a local acid-dependent reflex might theoreticallyresult either in an enhancement of ACh release from cholinergicterminals or in the release (or co-release) of a distinct transmitteracting on chief cells to facilitate the pepsigogic action of ACh.However, further investigations are needed to clarify this issue.

In conclusion, the present results suggest that the activation of muscarinic receptors on chief cells by vagally releasedACh is not sufficient to increase peptic output and that an acid-mediatedfacilitatory action is necessary to allow pepsinogen hypersecretionin response to stimulation by endogenous cholinergic pathways.According to our findings, it may be proposed that such acid-dependentfacilitatory input is driven to chief cells by a local gastricintramural reflex that involves capsaicin-insensitive intrinsicneurons. Overall, the hypothesis emerging from these findingswould reconcile the conflicting results of previous reports thathave indicated, on the one hand, a close parallel between acidand peptic hypersecretory responses to cholinergic stimulationin vivo and, on the other, the ability of chief cells to be activatedby muscarinic agonists in vitro independently of acid secretion.

	Acknowledgments

The experiments were carried out with the technical assistance of Mr. Bruno Stacchini.

	Footnotes

Accepted for publication August 26, 1997.

Received for publication March 31, 1997.

¹ The present work was supported in part by the Italian Ministry of University and Scientific Research (40% + 60% funds).

Send reprint requests to: Prof. Mario Del Tacca, M.D., Division of Pharmacology and Chemotherapy, Department of Oncology, University of Pisa, Via Roma, 55, I-56126 Pisa, Italy.

	Abbreviation

2DG, 2-deoxy-D-glucose.

	References

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Positive Modulation of Pepsinogen Secretion by Gastric Acidity After Vagal Cholinergic Stimulation1

Positive Modulation of Pepsinogen Secretion by Gastric Acidity After Vagal Cholinergic Stimulation¹