Tachykinergic Neurotransmission Is Enhanced in Small Intestinal Circular Muscle in a Rabbit Model of Inflammation

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

This Article

	Abstract
	Full Text (PDF)
	Submit a response
	Alert me when this article is cited
	Alert me when eLetters are posted
	Alert me if a correction is posted
	Citation Map

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Goldhill, J. M.
	Articles by Piñeiro-Carrero, V. M.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Goldhill, J. M.
	Articles by Piñeiro-Carrero, V. M.

Vol. 282, Issue 3, 1373-1378, 1997

Tachykinergic Neurotransmission Is Enhanced in Small Intestinal Circular Muscle in a Rabbit Model of Inflammation¹

Jon M. Goldhill, Terez Shea-Donohue, Nasima Ali and Victor M. Piñeiro-Carrero

Departments of Medicine and Pediatrics, Uniformed Services University of the Health Sciences, Bethesda, Maryland

	Abstract

Top Abstract Introduction Methods Results Discussion References

Previous electrophysiological studies have shown that tachykinin-mediated excitatory junction potentials are enhanced in aricin model of inflammatory bowel disease. The present study extendsthese findings by investigating the contractile response to stimulationof noncholinergic nerves and tachykinin agonists. According torank order potencies, the rabbit ileal circular muscle was neurokinin(NK)₁ preferring, and the response to these agonists was down-regulatedby acetylcholine and up-regulated by nitric oxide. In ricin-treatedtissue, cholinergic and nitridergic modulation was lost; in thepresence of atropine and N-nitro-L-arginine methyl ester, or tetrodotoxin,the response to NK₁ and NK₂ agonists was enhanced. The noncholinergicresponse to nerve stimulation was predominantly mediated by NK₁receptors, and the enhanced response of ricin-treated tissue toNK₁ agonists probably contributes to the increased response toelectrical field stimulation observed under these conditions.Increased tachykinin response and loss of control of this responseby acetylcholine and nitric oxide are likely to have profoundeffects on intestinal motility and could contribute to some ofthe symptomology of inflammatory bowel disease.

	Introduction

Top Abstract Introduction Methods Results Discussion References

Tachykinins are important excitatory neurotransmitters in the enteric nervous system and are involved in the coordinationof gastrointestinal motility (Bartho et al., 1983; Bartho andHolzer, 1985). This family of peptides includes the products oftwo genes, the PPT I gene, which produces SP and NK-A (Nawa etal., 1983), and the PPT II gene, which produces NK-B (Kotani etal., 1986), a tachykinin that is present in very small quantitiesin the intestinal tract (Tateishi et al., 1990). These tachykininspreferentially bind to NK₁, NK₂ and NK₃ receptors, respectively.Each of these receptors has been localized to circular musclecells in the small intestine (Hellstrom et al., 1994), althoughit is of note that biological effects of NK₃ activation have beenpredominantly attributed to a neural site of action (Croci etal., 1995).

Tachykinins are strongly implicated in IBD, a chronically debilitating condition associated with abnormal intestinal motility,which may contribute to cramping, abdominal pain and diarrhea.Tachykinin levels are increased in the colonic submucosa and mucosaof patients with ulcerative colitis (Goldin et al., 1989, Kochet al., 1987). Immunocytochemical studies have shown increasedtachykinin levels around epithelial cells in the colon of ulcerativecolitis patients and the colonic musculature in Crohn's disease(Mazumdar and Das, 1986). In addition to increased tachykininlevels, up-regulation of tachykinin receptors on intestinal bloodvessels has been reported in ulcerative colitis (Mantyh et al.,1988).

We recently developed an experimental model of IBD produced by the intraluminal administration of the cytotoxic plant lectinricin into the rabbit ileum. Ricin caused mucosal inflammation,epithelial damage and increased myoelectric activity (Sjogrenet al., 1994). These changes represent a general response to acuteinflammation because the hapten trinitrobenzene sulfonic acidevoked similar alterations (Sjogren et al., 1994). In vitro, EFSof enteric nerves resulted in larger noncholinergic EJPs in ricin-treatedcircular muscle than in controls (Goldhill et al., 1995), andthis was suggested to contribute to the increased myoelectricactivity in vivo. SP autodesensitization reversed the increasedresponse to EFS (Goldhill et al., 1995), prompting us to speculatethat altered tachykinin-mediated neurotransmission contributesto altered neuromuscular control during inflammation. We havesuggested that altered neuromuscular control may contribute tothe intestinal cramping and diarrhea associated with IBD.

In the present study, we further investigated the hypothesis that tachykinin-mediated neurotransmission is altered duringintestinal inflammation. Our first aim, therefore, was to determinewhether contractile responses to specific NK₁ and NK₂ agonistswere altered during inflammation. Although it is becoming apparentthat NK₃ receptors play a role in the contraction of intestinalsmooth muscle, this subtype was not studied due to the relativeunavailability of pharmacological tools, especially antagonists.It was unclear from earlier studies (Goldhill et al., 1995) whetherincreased EFS-evoked EJPs resulted in an increased contractileresponse because electrophysiological responses are known to beuncoupled from smooth muscle contraction in inflammation (Goldhillet al., 1994; Snape et al., 1980). Thus, the second aim of thepresent study was to confirm that the noncholinergic contractileresponse of circular muscle strips to EFS was also elevated. Finally,we examined whether this may result from altered tachykinergicresponsiveness by determining the receptor subtypes involved inthe response to EFS.

	Methods

Top Abstract Introduction Methods Results Discussion References

Induction of inflammation. Male New Zealand White rabbits were divided into a control vehicle-treated group and a ricin-treated group. Acute ileitiswas induced with ricin as previously described (Goldhill et al.,1995; Sjogren et al., 1994). Briefly, animals were anesthetizedwith intramuscular xylazine (9 mg/kg) and ketamine (50 mg/kg)and maintained with intravenous pentobarbital (15 mg/ml). A midlineincision was made, a ligated terminal ileal loop (~10 cm in length)was constructed in each animal and 1 ml of ricin (1 mg/ml) orvehicle was injected into the lumen. The loop was removed after5 hr, a time period that allowed development of ileitis, abnormalmyoelectric activity (Sjogren et al., 1994) and increased responseto EFS (Goldhill et al., 1995). Animals were killed with an overdoseof pentobarbital. The loop was opened along its length, gentlyflushed of luminal contents with cold-oxygenated modified KBSand prepared for contractility studies.

Contractility studies. Muscle strips (~1 × 0.4 cm) with mucosa removed were cut in the axis of the circular muscle and attached to isometric tensiontransducers in 10-ml organ baths and continuously bathed withmodified KBS at 37.5 ± 0.5°C. Tissues were allowed to equilibrateat L_i (the length at which no tension could be measured) for 20min. The strips were then progressively stretched to L_o, whichwas determined as the length at which maximum active force wasgenerated in response to acetylcholine (0.5-1 mM). Strips werethen allowed to equilibrate for an additional 20 min before thefollowing studies were performed.

Effect of inflammation on circular muscle response to tachykinins. We investigated the effect of inflammation on the response to NK₁ and NK₂ agonists. The NK₁ agonists used were the naturalagonist SP and its structural analog [SAR]SP. The NK₂ agonistsused were the natural agonist NKA and its structural analog $beta$ -Ala[NKA].Concentration-response curves were constructed on separate musclestrips for each of these agonists in vehicle- and ricin-treatedtissues. Agonists were applied at 10-15-min intervals, with atleast three changes of KBS between concentrations, to preventdesensitization. Studies were performed in the presence or absenceof tetrodotoxin (1 µM) to distinguish between neural and non-neuraleffects of ricin treatment.

Effect of acetylcholine and nitric oxide on the response to tachykinins. Previous electrophysiological studies (Goldhill et al., 1995) showed that increased noncholinergic excitation in ricin-treatedtissue was tempered by muscarinic receptors and/or nitric oxide.Therefore, concentration-response curves to NK₁ and NK₂ agonistswere constructed after the cumulative addition of the muscarinicantagonist atropine (1 µM) and the nitric oxide synthase inhibitorL-NAME (0.1 mM), to investigate whether modulation of tachykininresponse by acetylcholine or nitric oxide was altered during inflammation.These concentrations were the same as those in previous studies(Goldhill et al., 1995).

Effects of ricin treatment on noncholinergic, non-nitridergic responses to EFS. In this series of experiments, muscle strips were passed through a pair of ring electrodes (2-mm diameter) and stimulatedfor 10 sec by square-wave pulses (0.5-msec duration; supramaximalvoltage) at 1 to 10 Hz. Pulses were delivered to the electrodesfrom a Grass S88 stimulator (Grass Instruments, Quincy, MA). Preliminarystudies showed that EFS-evoked changes were maximal at 10 Hz andabolished by the neural blocker, tetrodotoxin (1 µM), demonstratingthat responses were due to neural stimulation. Stimulation wasperformed in the presence of atropine (1 µM) and L-NAME (0.1 mM).These concentrations have been used to abolish cholinergic andnitric oxide-mediated neurotransmission (Goldhill et al., 1995),thus allowing the specific investigation of noncholinergic excitation.Trains of EFS were applied at 20-min intervals to prevent desensitization.

Nature of the noncholinergic response to EFS. SP, which preferentially binds to NK₁ receptors, is proposed to mediate noncholinergic excitation in the guinea pig smallintestine (Taylor and Bywater, 1986), but this has not been confirmedin the rabbit. To establish whether NK₁ receptors mediate noncholinergicexcitation in the rabbit ileum, the response to maximal frequencyEFS (10 Hz) was determined after a 20-min pretreatment with atropineand L-NAME and the specific NK₁ antagonist GR 82,334 (10 µM) orin a paired piece of tissue with its vehicle, 0.01 N acetic acid.Previous reports have shown this antagonist to have a maximaland specific effect at this concentration (Hagan et al., 1991),and we have shown it to reduce the contractile response to SP(5 nM) by >70% in rabbit ileal circular muscle under control andinflamed conditions (94 ± 4% vs. 70 ± 19% in control and ricin-treatedtissue respectively; n = 4).

Data analysis. Maximum increases in muscle tone in response to tachykinin addition or EFS were obtained through visual analysis of chartrecorder outputs. Responses to tachykinins are expressed as absolutetension development. EFS data were expressed as a percentage ofthe response to 1 mM acetylcholine added at L_o to reduce the variationof this data. The response to this concentration of acetylcholinewas not altered by ricin in this series of experiments. The responseto EFS (10 Hz) in the presence of GR 82,334 was expressed as apercentage of the response after incubation in vehicle. Valuesare given as mean ± S.E.M. The number of animals (n) is shownin parentheses. Tachykinin concentration responses were fittedto sigmoid curves (GraphPAD, San Diego, CA.), and EC₅₀ values(with 95% CLs) were determined from these curves. Differencesbetween frequency or concentration-response curves were assessedstatistically using multivariate analysis of variance, with adjustmentsmade for multiple comparisons. In cases in which curves were significantlydifferent to one another, maximal responses were compared statisticallyusing Student's t test. The effect of GR 82,334 was assessed statisticallyusing Student's t test. A value of P < .05 was considered significantin each case.

Solutions and drugs. KBS contained (in mM) 118.5 NaCl, 4.75 KCl, 2.54 CaCl₂, 1.19 NaH₂PO₄, 1.19 MgSO₄, 25.0 NaHCO₃ and 11.0 glucose. This solutionwas gassed with 95% O₂/5% CO₂ to give a pH of 7.3 to 7.4. Alldrugs were obtained from Sigma Chemical (St. Louis, MO) unlessotherwise stated. Ricin toxin (Ricinus communis agglutinin₆₀)was dissolved in distilled water at the beginning of every experiment.Atropine sulfate and L-NAME were both dissolved in distilled wateras stock solutions of 10 and 100 mM, respectively. SP, [SAR]SP,NKA and [ $beta$ -Ala]NKA were obtained from Peninsula (Belmont, CA)and dissolved in 0.01 N acetic acid and stored as a stock solutionof 100 µM. GR 82,334 {[D-Pro⁹(spiro- $gamma$ -lactam)Leu¹⁰,Trp¹¹]physalaemin_1-11}; RBI, Natick, MA) was dissolved in 0.01N acetic acid and stored as a stock concentration of 5 mM.

	Results

Top Abstract Introduction Methods Results Discussion References

Response of circular muscle to tachykinins. Under control conditions, the rank order of potency of the tachykinin agonists was SP $sime$ [Sar]SP > NKA $>>$ [ $beta$ -Ala]NKA in bothvehicle- and ricin-treated tissues (table 1), suggesting thatthis tissue is NK₁ preferring. To determine whether alterationsin the response to NK₁ and NK₂ receptor activation occurs duringinflammation, the remainder of the present study was devoted toinvestigation of the contractile response to the specific agonists[Sar]SP and [ $beta$ -Ala]NKA. This avoids interpretational problemsassociated with the use of the natural agonists, SP and NKA, whichdisplay considerable overlap with respect to their binding toNK₁ and NK₂ receptors.

View this table:
[in this window]
[in a new window]

TABLE 1
EC₅₀ values for the responses of control and ricin-treated tissue to tachykinins
Concentration-response curves were constructed for agonists on separate mucosa-free circular muscle strips prepared from vehicle-or ricin-treated (inflamed) tissues. Agonists were applied at10 to 15-min intervals, with three or more changes of KBS betweenconcentrations, to prevent desensitization. Values given are meanEC₅₀ (nM) values with 95% confidence values given in parenthesesfrom $>=$ 6 replicates. Note that all values are for studies performedin the absence of atropine or L-NAME.

Effect of acetylcholine and nitric oxide on the response of vehicle-treated tissue to tachykinins. The addition of atropine significantly altered the response of vehicle-treated tissue to the selective NK₁ agonist [Sar]SP(P < .05) (fig. 1a). This did not correspond to a change in potency(3.0 nM, 95% CL = 2.5-3.6 vs. 3.2 nM, 95% CL = 1.8-5.6 nM; n $>=$ 6 in absence and presence of atropine respectively), but the maximalresponse was significantly increased (P > .05). These increasesin responsiveness were reversed by further addition of the nitricoxide synthase inhibitor L-NAME, so the response to NK₁ stimulationin the presence of atropine and L-NAME was not significantly differentthan that in the absence of drugs (fig. 1a). In contrast to [Sar]SP,the response to [ $beta$ -Ala]NKA was unaffected by atropine or L-NAME(fig. 1c).

View larger version (22K):
[in this window]
[in a new window]

Fig. 1. Concentration-response curves to [Sar]SP in vehicle-treated (A) or ricin-treated tissue (B) and to [ $beta$ -Ala]NK A in vehicle-treated(C) or ricin-treated tissue (D). Responses were determined undercontrol conditions ( $bullet$ , n $>=$ 6), in the presence of atropine (1µM) ( $black-diamond$ , n $>=$ 6) and in the presence of atropine (1 µM) and L-NAME(0.1 mM) ( $black-square$ , n $>=$ 6), in vehicle- and ricin-treated tissue. Theseseries of concentration-response curves were compared statisticallyusing a multivariate analysis of variance. * P < .01 vs. controlconditions in vehicle-treated tissue; $dagger$ P < .05 vs. vehicle-treatedtissue in the presence of atropine and L-NAME.

Effect of ricin treatment on cholinergic and nitridergic control of tachykinin response. After ricin treatment, neither atropine nor atropine and L-NAME significantly (P > .05) altered the concentration responseto [Sar]SP or [ $beta$ -Ala]NKA (figs. 1, b and d).

Effect of ricin treatment on noncholinergic, non-nitridergic response to tachykinins. In the presence, but not the absence, of atropine and L-NAME, ricin treatment significantly altered the response to both [Sar]SPand [ $beta$ -Ala]NKA (fig. 2). In both cases, this effect correspondedto a small but not significant increase in the maximum responseand an increase in potency. Ricin decreased the EC₅₀ value of[Sar]SP from 5.4 nM (95% CL = 5.2-5.4 nM) to 1.9 nM (95% CL =1.6-2.3 nM) and that of [ $beta$ -Ala]NKA from 114.8 nM (95% CL = 112.2-114.8nM) to 58.9 nM (95% CL = 58.5-59.3 nM). To confirm that this increasedresponsiveness was not related to activation of noncholinergic,non-nitridergic nerves the response of vehicle- and ricin-treatedto both [Sar]SP and [ $beta$ -Ala]NKA was compared in the presence oftetrodotoxin. Figure 3 shows that under these conditions, ricin-treatedtissue was still hyperresponsive to tachykinergic stimulation.As in the presence of atropine and L-NAME, after neural blockade,ricin-treated tissue was more sensitive than vehicle-treated tissueto [Sar]SP [0.19 nM (95% CL = 0.16-0.23 nM) vs. 3.09 nM (95% CL= 1.68-5.89 nM), respectively] and to [ $beta$ -Ala]NKA/[Sar]SP [6.49nM (95% CL = 4.79-8.91 nM) vs. 53.70 nM (95% CL = 52.48-54.95nM), respectively].

View larger version (16K):
[in this window]
[in a new window]

Fig. 2. Concentration-response curves to [Sar]SP and [ $beta$ -Ala]NKA in vehicle-treated tissue ( $bullet$ , n $>=$ 6),and in ricin-treated tissue ( $open circle$ ,n $>=$ 6). Each of the response curves were performed in the presenceof atropine (1 µM) and L-NAME (1 mM). These pairs of concentration-responsecurves were compared statistically using a multivariate analysisof variance. $dagger$ P < .05 vs. vehicle-treated tissue. It should benoted that the data are the same as those in figure 1 but replottedto facilitate direct comparison between vehicle- and ricin-treatedtissue.

View larger version (16K):
[in this window]
[in a new window]

Fig. 3. Concentration-response curves to [Sar]SP and [ $beta$ -Ala]NKA in vehicle-treated tissue ( $bullet$ , n $>=$ 6) and ricin-treated tissue ( $open circle$ ,n $>=$ 6). Each of the response curves were performed in the presenceof tetrodotoxin (1 µM). These pairs of concentration-responsecurves were compared statistically using a multivariate analysisof variance. $dagger$ P < .05 vs. vehicle-treated tissue.

Response to EFS. In the presence of atropine and L-NAME, EFS evoked a frequency-dependant contractile response, reaching a maximum at 10 Hz(fig. 4). The addition of the NK₁ antagonist GR 82,334 reducedthe maximal response of vehicle-treated tissue to EFS by 81.5± 11.69% (n = 4; P < .01), showing that NK₁ receptors play a majorrole in the noncholinergic response to EFS.

View larger version (13K):
[in this window]
[in a new window]

Fig. 4. Effect of EFS on the response of vehicle-treated tissue ( $bullet$ , n = 5) and ricin-treated tissue ( $open circle$ , n = 7). EFS was performedfor 10 sec (0.5-msec pulse width, supramaximal voltage) in thepresence of atropine (1 µM) and L-NAME (.1 mM). These pairs offrequency-response curves were compared statistically using amultivariate analysis of variance. * P < .05 vs. vehicle-treatedtissue.

Effect of ricin on the response to EFS. Because the responsiveness to NK₁ specific agonists is enhanced during inflammation, and these receptors mediate a large portionof the response to EFS, it was reasonable to speculate that ricinwould increase the response to EFS. The present study shows thisto be the case (fig. 4), thus extending our earlier electrophysiologicalstudies that showed that in the presence of atropine and L-NAME,the myoelectric response to EFS was increased by ricin (Goldhillet al., 1995).

	Discussion

Top Abstract Introduction Methods Results Discussion References

In a previous electrophysiological study, we reported that acute inflammation increased the magnitude of EFS-evoked noncholinergicEJPs (Goldhill et al., 1995) and speculated that this may contributeto cramping and abdominal pain during intestinal inflammation.Because this effect was reversed by SP autodesensitization, itwas suggested that an altered response to or release of tachykininscontributes to this phenomenon. Data from the present study supportthis hypothesis, demonstrating that acute inflammation increasesthe response to NK₁ and NK₂ agonists under noncholinergic conditions,that the rabbit circular muscle is NK₁ preferring and that thesereceptors play a major role in mediating the response to EFS.The enhanced response to NK₁ agonists may therefore contributeto the increased contractile response to EFS also seen under thesecondition in the present study.

SP and NKA are derived from the same PPT I gene (Nawa et al., 1983) which explains why both of these peptides are found inthe same synaptic vesicles (Deacon et al., 1987). SP and NKA bindpreferentially to NK₁ than NK₂ receptors; however, there is considerableinterspecies differences with respect to the balance between thesesubtypes. The circular muscle of the human, dog and rat smallintestine show NK₂ selectivity (Hellstrom et al., 1994; Maggiet al., 1992; Muller et al., 1988), and the guinea pig, NK₁ selectivity(Maggi et al., 1994). In the course of the present study, theresponsiveness of healthy rabbit circular muscle to the tachykininswas characterized, and we report that the rank order of potenciesfor the various tachykinin agonists is similar to that of theguinea pig small intestinal circular muscle (Maggi et al., 1994).

The mechanism of action of SP is well understood in the guinea pig ileum. Contractile effects of SP on longitudinal muscleare mediated, in part, by cholinergic nerves (Regoli et al., 1984)because the effects of SP are inhibited by atropine. In contrast,the NK₁-mediated response to EFS is reduced by acetylcholine,suggesting presynaptic inhibition (Wiklund et al., 1993). Tachykinergicneurotransmission is also regulated by nitric oxide. The mostcommonly reported effect of nitric oxide is to reduce tachykininneurotransmission (Wiklund et al., 1993), although under certainconditions, nitric oxide appears to contract intestinal smoothmuscle by releasing tachykinins (Bartho and Lefebvre, 1994). Regulationof tachykinin neurotransmission in rabbit ileal circular musclehas not been previously described. The effect of atropine andL-NAME on the response to [Sar]SP suggests that under healthyconditions, acetylcholine reduces tachykinergic contraction, whereasnitric oxide enhances contraction. The mechanisms of these effectsare beyond the scope of this study. In contrast, one of the mostimportant findings of the present study is that these regulatorymechanism appears to be lost during inflammation.

The tachykinins have previously been implicated in functional alterations observed during inflammation. Mucosal/submucosallevels of SP are increased in the colon of ulcerative colitis(Goldin et al., 1989; Koch et al., 1987). SP levels are also increasedby ~60% in the muscle layer of the ileum from Crohn's diseasepatients (Koch et al., 1987). Moreover, NK₁ receptor numbers arealso reported to be increased in IBD (Mantyh et al., 1988). Ina guinea pig model of IBD, trinitrobenzene sulphonic acid increasedthe density of SP staining in the small intestinal myenteric plexus(Miller et al., 1993). Despite considerable evidence that NK₁receptors are involved in the pathophysiology of intestinal inflammation,the present study is the first to show that tachykinergic controlof contraction is altered during inflammation. This alterationoccurs at two levels. First, as described above, the interactionsbetween nitric oxide and acetylcholine, and NK₁ excitation areabsent during inflammation, and thus the regulation of tachykinergicneurotransmission may be lost under these conditions. Second,we have shown that under noncholinergic conditions, or in thepresence of TTX, the contractile responses to both [Sar]SP andthe NK₂ agonist [ $beta$ -Ala]NKA, are increased during inflammation.It is of note that although evidence is starting to accumulatethat implicates the NK₃ receptor in the control of intestinalsmooth muscle, changes in NK₃ responsiveness were not investigatedin the present series of experiments and therefore deserve futurestudy. The mechanism by which increased responsiveness to tachykininsoccurs is unclear but appears to involve an increase in sensitivityas the response curves to both [Sar]SP and [ $beta$ -Ala]NKA were shiftedto the left. It is not clear whether this reflects increased receptorsensitivity or postreceptor modification, and binding studiesare required to resolve this issue. Whatever the exact mechanism,changes in the receptor/second-messenger system are nonneuralin nature as differences between vehicle- and ricin-treated tissuewere observed in the presence of tetrodotoxin. Alternatively,increased tachykinin sensitivity could result from down-regulationof the neutral endopeptidase, the enzyme responsible for tachykininbreakdown. This has previously been demonstrated in the rat smallintestine after Trichinella spiralis infection (Hwang et al.,1993). This explanation, however, cannot fully explain the presentdata as [ $beta$ -Ala]NKA is insensitive to enzyme metabolism (Patacchiniet al., 1989).

In the guinea pig ileum, in the presence of atropine and nitric oxide synthase inhibition the response to EFS was abolishedby the NK₁ antagonist CP 99,345, suggesting that NK₁ receptorsmediate most of the noncholinergic excitatory response to nervestimulation (Wiklund et al., 1993). The same appears to be truein the rabbit ileum, as in the present study we show that GR82,334almost abolished the response to EFS. Because the noncholinergicresponse to EFS is predominantly NK₁ mediated and NK₁-mediatedexcitation is enhanced under noncholinergic, non-nitridergic conditionsduring inflammation, the response to EFS should be enhanced underthese conditions if transmitter release in unimpaired. It wasnecessary to test this hypothesis directly- however, as it haspreviously been shown that transmitter release is impaired inTrichinella-infected rats (Collins et al., 1989). Even if thisis the case in ricin-evoked inflammation, we show in the presentstudy that in agreement with our previous electrophysiologicaldata (Goldhill et al., 1995), the contractile response to EFSis enhanced during inflammation.

In summary, we demonstrated that (1) inflammation abolishes cholinergic down-regulation and nitridergic up-regulation of theNK₁ response, and (2) inflammation increases circular muscle responsivenessto NK₁ and NK₂ agonists, which could contribute to the heightenedresponse to noncholinergic nerve stimulation. Consequently, wespeculate that the response to those stimuli that evoke tachykinin-mediatedcontractions alone will be augmented during inflammation. Also,the loss of cholinergic and nitridergic modulation of tachykinergicneurotransmission would be expected to result in an altered responseto stimuli that corelease acetylcholine and/or nitric oxide withthe tachykinins. However, before specific defects can be moreaccurately predicted, a greater understanding of neural pathwaysand their response to different stimuli is necessary. What isclear, however, is that such changes are likely to impair theability of the intestine to adapt to its ever-changing luminalconditions during inflammation and is likely to contribute tothe altered intestinal function observed under these conditions.

	Footnotes

Accepted for publication May 14, 1997.

Received for publication September 6, 1996.

¹ This work was funded by grants to T. Shea Donohue (G183EP).

Send reprint requests to: Dr. Jon M. Goldhill, Synthelabo Recherche, 10 Rue des Carrieres, 92505 Rueil-Malmaison, France.

	Abbreviations

CL, confidence interval; NK, neurokinin; L-NAME, N-nitro-L-arginine methyl ester; IBD, inflammatory bowel disease; SP, substance P; EFS, electric field stimulation; EJP, excitatory junction potential; KBS, Krebs-bicarbonate-saline; PPT, preprotachykinin; [SAR]SP, [Sar⁹,Met¹¹(O₂)]substance P; $beta$ -Ala[NKA], [ $beta$ -Ala⁸]neurokinin A; L-NAME, N-nitro-L-arginine methyl ester.

	References

Top Abstract Introduction Methods Results Discussion References

Bartho, L., Holzer, P., Lembeck, F. and Szolcsanyi, J.: Evidence that the contractile response of the guinea pig ileum to capsaicin is due to the release of substance P. J. Physiol. 332: 157-167, 1983.[Abstract/Free Full Text]
Bartho, L. and Holzer, P.: Search for a physiological role of substance P in gastrointestinal motility. Neuroscience 16: 1-32, 1985[Medline].
Bartho, L. and Lefebvre, R.: Nitric oxide induces acetylcholine-mediated contractions in the guinea-pig small intestine. Arch. Pharmacol. 350: 582-584, 1994.
Collins, S. M., Blennerhassett, P. A., Blennerhasset, M. G. and Vermillion, D. L.: Impaired acetylcholine release from the myenteric plexus of Trichinella-infected rats. Am. J. Physiol. 257: G898-G903, 1989[Abstract/Free Full Text].
Croci, T., Landi, M., Emonds-Alt, X., Le Fur, G. and Manara, L.: Neuronal NK3-receptors in guinea-pig ileum and taenia caeci: In vitro characterization by their first non-peptide antagonist, SR142801. Pharmacol. Lett. 57: 361-366, 1995.
Deacon, C. F., Agoston, D. V., Nau, R. and Conlon, J. M.: Conversion of neuropeptide K to neurokinin A and vesicular colocalization of neurokinin A and substance P in neurons of the guinea pig intestine. J. Neurochem. 48: 141-146, 1987[Medline].
Goldhill, J. M., Percy, W. H., Donovan, V., Joseph, I., Zhao, L. and Burakoff, R.: In vivo muscle activity and epithelial function in the rabbit distal colon during experimental colitis. Neurogastroenterol. Motil. 6: 289-294, 1994.
Goldhill, J. M., Sanders, K., Shea-Donohue, T. and Sjogren, R.: In vitro changes in neural control of muscle function in experimental ileitis. Am. J. Physiol. 268: G823-G830, 1995[Abstract/Free Full Text].
Goldin, E., Karmeli, F., Selinger, Z. and Rachmilewitz, D.: Colonic substance P levels are increased in ulcerative colitis and decreased in chronic severe constipation. Dig. Dis. Sci. 34: 754-757, 1989[Medline].
Hagan, R. M., Ireland, S. J., Bailey, F., McBride, C., Jordan, C. C. and Ward, P.: A spirolactam conformationally-restrained analogue of physalaemin which is a peptidase-resistant, selective neurokinin NK1 receptor antagonist. Br. J. Pharmacol. 102: 168P, 1991.
Hellstrom, P. M., Murthy, K. S., Grider, J. R. and Makhlouf, G. M.: Coexistence of three tachykinin receptors coupled to Ca⁺⁺ signalling pathways in intestinal smooth muscle cells. J. Pharmacol. Exp. Ther. 270: 236-243, 1994[Abstract/Free Full Text].
Hwang, L., Leichter, R., Okamoto, A., Payan, D., Collins, S. M. and Bunnett, N.: Downregulation of neutral endopeptidase (EC3.4.24.11) in the inflamed rat intestine. Am. J. Physiol. 264: G735-G743, 1993[Abstract/Free Full Text].
Kotani, H., Hoshimaru, M., Nawa, H. and Nakanishi, S.: Structure and gene organization of bovine neuromedin K precursor. Proc. Natl. Acad. Sci. USA 83: 7074-7078, 1986[Abstract/Free Full Text].
Koch, T. R., Carney, J. A. and Go, V. L. W.: Distribution and quantitation of gut neuropeptides in normal intestine and inflammatory bowel diseases. Dig. Dis. Sci. 32: 369-376, 1987[Medline].
Maggi, C. A., Giuliani, S., Patacchinin, R., Santicioli, P., Theodorsson, E., Barbanti, G., Turinin, D. and Giachetti, A.: Tachykinin antagonists inhibit nerve-mediated contractions in the circular muscle of the human ileum. Gastroenterology 102: 88-96, 1992[Medline].
Maggi, C. A., Patacchini, R., Meini, S., Quartara, L., Sisto, A., Potier, E., Giuliani, S. and Giachetti, A.: Comparison of tachykinin NK1 and NK2 receptors in the circular muscle of the guinea-pig ileum and proximal colon. Br. J. Pharmacol. 112: 150-160, 1994[Medline].
Mantyh, C. R., Gates, T. S., Zimmerman, R. P., Welton, M. L., Passaro, E. P., Vigia, S. R., Maggio, J. E., Kruger, L. and Mantyh, P. W.: Receptor binding sites for substance P, but not substance K or neuromedin K, are expressed in high concentrations by arterioles, venules, and lymph nodules in surgical specimens obtained from patients with ulcerative colitis and Crohn disease. Proc. Natl. Acad. Sci. USA 85: 3235-3239, 1988[Abstract/Free Full Text].
Mazumdar, S. and Das, K. M.: Immunocytochemical localization of vasoactive intestinal peptide and substance P in the colon from normal subjects and patients with inflammatory bowel disease. Am. J. Gastroenterol. 87: 176-181, 1992[Medline].
Miller, M. J. S., Sadowska-Krowicka, H., Jeng, A. Y., Chotinaruemol, S., Wong, M., Clark, D. A., Ho, W. and Sharkey, K. A.: Substance P levels in experimental ileitis in guinea pigs: Effects of misoprostol. Am. J. Physiol. 265: G321-G330, 1993[Abstract/Free Full Text].
Muller, M. J., Sato, H., Bowker, P. and Daniel, E. E.: Receptors for tachykinins in canine intestinal circular muscle. J. Pharmacol. Exp. Ther. 246: 739-744, 1988[Abstract/Free Full Text].
Nawa, H., Hirose, T., Takashima, H., Inayama, S. and Nakanishi, S.: Nucleotide sequences of cloned cDNAs for two types of bovine substance P precursor. Nature. 306: 32-36, 1983[Medline].
Patacchini, R., Maggi, C. A., Rovero, P., Regoli, D. and Meli, A.: Effect of thiorpan on tachykinin-induced potentiation on nerve mediated contraction of the rat isolated vas deferens. J. Pharmacol. Exp. Ther. 250: 678-681, 1989[Abstract/Free Full Text].
Regoli, D., D'orlean-Juste, P., Escher, E. and Mizrahi, J.: Receptors for substance P. I. The pharmacological preparations. Eur. J. Pharmacol. 97: 161-170, 1984[Medline].
Sjogren, R. W., Colleton, C. and Shea-Donohue, T.: Intestinal myoelectric response in two different models of acute enteric inflammation. Am. J. Physiol. 30: G329-G337, 1994.
Snape, W. J., Matarazzo, S. and Cohen, S.: Abnormal gastrocolonic response in patients with ulcerative colitis. Gut 21: 392-396, 1980[Abstract/Free Full Text].
Tateishi, K., Kishimoto, S., Kobayash, H., Kobuke, K. and Matsuoka, Y.: Distribution and localization of neurokinin A-like immunoreactivity and neurokinin B-like immunoreactivity in rat peripheral tissue. Regul. Peptides 30: 193-200, 1990[Medline].
Taylor, G. S. and Bywater, R. A. R.: Antagonism of non-cholinergic excitatory junction potentials in the guinea-pig ileum by a substance P analogue antagonist. Neurosci. Letts. 63: 23-26, 1986[Medline].
Wiklund, C. U., Wiklund, P. and Gustafsson, L. E.: Modulation of neuroeffector transmission by endogenous nitric oxide: A role for acetylcholine receptor-activated nitric oxide formation, as indicated by measurments of nitric oxide/nitrite release. Eur. J. Pharmacol. 240: 235-242, 1993[Medline].

This article has been cited by other articles:

K. Venkova, J. M. Palmer, and B. G.-V. Meerveld
Nematode-Induced Jejunal Inflammation in the Ferret Causes Long-Term Changes in Excitatory Neuromuscular Responses
J. Pharmacol. Exp. Ther., July 1, 1999; 290(1): 96 - 103.
[Abstract] [Full Text]

This Article

Abstract

Full Text (PDF)

Submit a response

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Similar articles in this journal

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Google Scholar

Google Scholar

Articles by Goldhill, J. M.

Articles by Piñeiro-Carrero, V. M.

Search for Related Content

PubMed

PubMed Citation

Articles by Goldhill, J. M.

Articles by Piñeiro-Carrero, V. M.

Tachykinergic Neurotransmission Is Enhanced in Small Intestinal Circular Muscle in a Rabbit Model of Inflammation1

Tachykinergic Neurotransmission Is Enhanced in Small Intestinal Circular Muscle in a Rabbit Model of Inflammation¹