Angiotensin Inhibits Neurotransmission of Calcitonin Gene-Related Peptide-Containing Vasodilator Nerves in Mesenteric Artery of Spontaneously Hypertensive Rats

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 Google Scholar

Google Scholar

	Articles by Kawasaki, H.
	Articles by Gomita, Y.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Kawasaki, H.
	Articles by Gomita, Y.

Vol. 284, Issue 2, 508-515, February 1998

Angiotensin Inhibits Neurotransmission of Calcitonin Gene-Related Peptide-Containing Vasodilator Nerves in Mesenteric Artery of Spontaneously Hypertensive Rats¹

Hiromu Kawasaki, Makoto Takenaga, Hiroaki Araki, Kojirou Futagami and Yutaka Gomita

Department of Clinical Pharmaceutical Science, Faculty of Pharmaceutical Sciences, Okayama University (H.K.), 1-1-1 Tsushimanaka, Okayama 700 and Department of Hospital Pharmacy, Okayama University Medical School (H.A., K.F., Y.G.), 2-5-1 Shikata-cho, Okayama 700 and the First Department of Internal Medicine, Miyazaki Medical College (M.K.), 5200 Kiyotake, Miyazaki 889-16, Japan

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

The role of angiotensin (Ang) in neurotransmission of calcitonin gene-related peptide (CGRP)-containing vasodilator nervesin perfused mesenteric vascular beds isolated from spontaneouslyhypertensive rats (SHR) (8- and 15-week-old) and age-matched WistarKyoto rats (WKY) was investigated. In both SHR and WKY preparationsprecontracted by continuous perfusion of Krebs' solution containing7 µM methoxamine plus 5 µM guanethidine, periarterial nerve stimulation(PNS; 1 and 2 Hz) produced a frequency-dependent vasodilation,which was abolished by 100 nM tetrodotoxin and 500 nM CGRP(8-37)(CGRP receptor antagonist). The PNS-induced vasodilation in theSHR decreased with age and was smaller than that in the WKY. Theneurogenic vasodilation in the SHR but not WKY was significantlyinhibited by N-acetyltetradecapeptide renin substrate (RS, 100and 500 nM), AngI (50 and 100 nM) and AngII (50 and 100 nM). Theinhibitory effects of RS, AngI and AngII were abolished by theAngII receptor antagonist, [Sar¹,Ile⁸]AngII (500 nM). The effect of RS and AngI was inhibited by captopril(5 µM) and temocapril (500 nM). AngII (100 nM) had no effect onvasodilator response to exogenously infused CGRP (100 pmol). PNS(2 Hz) of perfused mesenteric vascular beds increased the releaseof CGRP-like immunoreactivities (CGRP-LI) in the perfusate, whichwas less in 15-week-old SHR than in age-matched WKY. AngII (100nM) significantly inhibited the neurogenic release of CGRP-LIin the SHR but not in the WKY. These results suggest that exogenousand locally converted AngII, via AngII receptors, modulates theneurotransmission of CGRP-containing vasodilator nerves by inhibitingCGRP release from the nerve.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

The tone of resistance blood vessels is maintained mainly by sympathetic, adrenergic vasoconstrictor nerves, but recent studieshave revealed the NANC vasodilator innervation in blood vesselsand involvement of vasodilator nerves in the regulation of vasculartone (Kawasaki et al., 1988; Toda and Okamura, 1992). We havedemonstrated that the mesenteric resistance blood vessels of therat are innervated by NANC vasodilator nerves in which CGRP, apotent vasodilator neuropeptide, acts as the vasodilator neurotransmitter(Kawasaki et al., 1988, 1990a, 1990b, 1991). In relation to controlof the vascular tone, CGRP-containing vasodilator nerves (CGRPnerves) suppress vasoconstrictor responses to adrenergic nervestimulation through released CGRP, and conversely, adrenergicnerves inhibit the release of CGRP from the nerve to decreaseCGRP nerve function (Kawasaki et al., 1990a,b, 1991). Thus, wehave proposed that CGRP vasodilator nerves along with sympatheticvasoconstrictor nerves regulate the tone of the mesenteric resistanceblood vessels.

Evidence has accumulated showing that increased total peripheral vascular resistance maintains elevated blood pressure inchronic hypertension (Folkow et al., 1970; Zimmerman, 1983). Theimpaired function of the control systems regulating peripheralresistance has been considered (Zimmerman, 1983; Head, 1989).In studies with SHRs, which are the best animal models for humanessential hypertension, the enhanced activity of sympathetic vasoconstrictornerves has been an important factor in the increased tone of peripheralresistance vessels (Head, 1989; Kawasaki et al., 1982b). Recently,we demonstrated that the CGRP nerve function in SHR decreaseswith age and proposed that malfunction of CGRP vasodilator nervesregulating peripheral vascular resistance plays an important rolein the development and maintenance of hypertension in SHR (Kawasakiet al., 1990c; Kawasaki and Takasaki, 1992). However, the mechanismsunderlying reduced function of CGRP vasodilator nerves in SHRremain unresolved. In a recent pharmacological study, we showedthat chronic treatment of SHR with an ACE inhibitor, but not otherantihypertensive drugs such as a calcium antagonist and beta adrenoceptorantagonist, prevents the decrease in vasodilator responses mediatedby CGRP nerves (Kawasaki, 1992). This finding suggested that therenin-angiotensin system might be involved in the reduced functionof CGRP vasodilator nerves in SHR. The present study was undertakento investigate the role of Ang in neurotransmission of CGRP vasodilatornerves in SHR. We report here that the locally generated AngIIin the blood vessel wall of the SHR caused an inhibition of neurotransmissionsof CGRP nerves.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Blood pressure measurement. Male SHRs at 8 and 15 weeks of age and age-matched normotensive WHYs, purchased from Charles River Japan (Shizuoka, Japan),were anesthetized with an intraperitoneal injection of sodiumpentobarbital (50 mg/kg). The left carotid artery was cannulated,and the arterial pressure was measured with a pressure transducer(model P23ID) and recorded on a polygraph (model RM-6000, NihonKohden).

Perfusion of the mesenteric vascular bed. Under pentobarbital anesthesia, the mesenteric vascular bed was isolated and prepared for perfusion as described previously(Kawasaki et al., 1988, 1990a). The superior mesenteric arterywas cannulated and gently flushed with a modified (see below)Krebs-Ringer bicarbonate solution (Krebs' solution) to eliminateblood from the vascular bed. After removal of the entire intestineand associated vascular bed, the mesenteric vascular bed was separatedfrom the intestine by cutting close to the intestinal wall. Onlyfour main arterial branches from the superior mesenteric trunkrunning to the terminal ileum were perfused. All other branchesof the superior mesenteric artery were tied off. The preparationwas perfused with Krebs' solution at a constant flow rate of 5ml/min with a peristaltic pump (model SJ-1215, ATTO Co., Tokyo,Japan). The preparation was also superfused with the same solutionat a rate of .5 ml/min to prevent drying. Modified Krebs' solutionwith the following composition was used (mM): NaCl, 120.0; KCl,5.0; CaCl₂, 2.4; MgSO₄, 1.2; NaHCO₃, 25.0; 2NaEDTA, 0.027; anddextrose, 11.0 (pH 7.4). The Krebs' solution was bubbled witha mixture of 95% O₂-5% CO₂ before passage through a warming coilmaintained at 37°C. Changes in the perfusion pressure were measuredwith a pressure transducer (model MPU-0.5A).

PNS and bolus injection of CGRP. After allowing the basal perfusion pressure to stabilize, the preparation was contracted with methoxamine at a submaximalconcentration of 7 µM in the presence of 5 µM guanethidine, whichwas added to block adrenergic neurotransmission. The increasedperfusion pressure was allowed to stabilize, and the preparationwas subjected to PNS at 1 and 2 Hz or to bolus infusion of CGRP.PNS was applied for 30 sec through bipolar platinum ring electrodesplaced around the superior mesenteric artery. Rectangular pulsesof 1 msec in duration and supramaximum voltage (50 V) were appliedby an electronic stimulator (model SEN 3301, Nihon Kohden). Inanother preparation, 100 pmol CGRP diluted with Krebs' solutioncontaining methoxamine and guanethidine was infused directly intothe perfusate proximal to the arterial cannula with an infusionpump (model 975, Harvard Apparatus, S. Natick, MA). The volumeof infusion was 100 µl for 10 sec. After control responses tothe first PNS at 2 Hz (S₁) and the first injection of CGRP (I₁)were obtained, the second PNS (S₂) and the second infusion ofCGRP (I₂) were carried out during perfusion with the final concentrationsof AngI, AngII and RS. After switching Krebs' solution containingmethoxamine plus guanethidine without the test drug, the thirdPNS (S₃) and the third infusion (I₃) were carried out as the after-control.

In separate experiments, the Krebs' solution containing methoxamine, guanethidine and the final concentration of AngII receptorantagonist ([Sar¹, Ile⁸]AngII) or ACE inhibitor (captopril or temocapril) was perfusedthroughout the experiment.

To estimate the effects of the drugs tested, the changes in perfusion pressure in response to PNS or bolus infusion of CGRPwere expressed as the ratio between the vasodilation induced byS₂ and by S₁, or the vasodilation induced by I₂ and by I₁, respectively.At the end of each experiment, 100 µM papaverine was perfusedthrough the preparation to produce complete relaxation. Vasodilationwas expressed as a percentage of the maximum relaxation inducedby papaverine.

Release of CGRP-like immunoreactivity. The mesenteric vascular beds isolated from 15-week-old SHRs and age-matched WKYs were perfused with Krebs' solution containing7 µM methoxamine and 5 µM guanethidine at a constant flow rateof 5 ml/min and superfused with Krebs' solution (0.5 ml/min).The perfusate was collected for 5 min before and after PNS (S₁and S₂) at 2 Hz for 30 sec. The drugs tested were perfused 10min before and throughout PNS (S₂). Each sample was applied toa Sep-PakC₁₈ cartridge (Waters Associates, Milford, MA), and theabsorbed peptide was eluted with 3 ml of 60% acetonitrile in 0.1%trifluoroacetic acid. The eluate was evaporated under a vacuumand stored at $-$ 80°C until a radioimmunoassay for CGRP as describedpreviously (Kawasaki et al., 1990c; Kawasaki and Takasaki, 1992).The samples were preincubated with rabbit anti-human CGRP-II serum(Peninsula Laboratories, Inc., Melmont, CA) at 4°C for 12 hr.Then, the reaction mixture was incubated with (2-[¹²⁵I]iodohistidyl¹⁰)CGRP (human) (Amersham International, Buckinghamshire, UK) foran additional 24 to 36 hr at 4°C. The antibody-bound antigen wasseparated from free antigens by the double-antibody preincubationmethod. The antibodies used cross-reacted 100% with rat and humanCGRP but 0% with substance P, neuropeptide Y and AngII. The lowerdetection limit was 1 fmol/tube for CGRP-LI.

Statistical analysis. All data are presented as the mean ± S.E.M. One-way analysis of variance followed by Dunnett's test or by Tukey's test wasused to determine the significance between values of differentages or different doses. Unpaired Student's t test was used todetermine the significance of differences between two means. Avalue of P < .05 was considered significant.

Drugs. The following drugs were used: AngI (Sigma Chemical Co., St. Louis, MO), AngII (Sigma), N-acetyltetradecapeptide (Sigma),captopril (Sankyo Pharmaceutica, Tokyo, Japan), guanethidine sulfate(Tokyo Kasei, Tokyo, Japan), human CGRP(8-37) (Peptide Institute,Osaka, Japan), methoxamine HCl (Nihon Shinyaku, Kyoto, Japan),rat $alpha$ -CGRP (Peptide Institute), [Sar¹, Ile⁸]AngII (Sigma), temocapril diacid (active form of temocapril,Sankyo) and TTX (Sigma). All drugs, except for temocapril diacidwhich was dissolved in 0.001% NaHCO₃, were dissolved in distilledwater and diluted with Krebs' solution containing 7 µM methoxamineand 5 µM guanethidine, when injected as a bolus or perfused.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

Blood pressure, perfusion pressure and vasoconstriction induced by methoxamine in SHRs and WKYs. As shown in table 1, the mean carotid arterial pressure in SHRs at 15 weeks of age was significantly greater than that at8 weeks of age; no significant difference was found in the WKYblood pressure at any age. The mean carotid arterial pressuresin SHRs at 8 and 15 weeks of age were significantly greater thanthose of the age-matched WKYs. The resting mean perfusion pressureof perfused mesenteric vascular beds was significantly greaterin the 15-week-old SHRs than the 15-week-old WKYs.

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

TABLE 1
Mean blood pressure, mean perfusion pressure, methoxamine-induced vasoconstriction and vasodilation of the mesenteric arteryinduced by PNS in normotensive WKYs and SHRs^a

Neurogenic vasodilator response in SHRs and WKYs. To maintain the active tone of the mesenteric artery, the preparation was contracted by the continuous perfusion of 7 µM methoxaminein the presence of 5 µM guanethidine, which was added to blockadrenergic neurotransmission. As shown in table 1, the methoxamine-inducedincreases in mean perfusion pressure before PNS were significantlygreater in the SHR than in the WKY.

As shown in figure 1A, PNS at 1 and 2 Hz in the SHR preparations with active tone produced a frequency-dependent decreasein perfusion pressure because of vasodilation, which was abolishedby perfusion of TTX (100 nM). The bolus infusion of CGRP (100pmol) also caused a long-lasting vasodilation, which mimickedthe response to PNS (fig. 1B). The perfusion of CGRP(8-37) (500nM), a CGRP receptor antagonist, markedly inhibited the vasodilatorresponse induced by both exogenous CGRP and PNS (fig. 1B), whichindicates that the vasodilator response to PNS is neurogenic andmediated by CGRP vasodilator nerves. Similar results were obtainedin the WKY preparations.

View larger version (19K):
[in this window]
[in a new window]

Fig. 1. Typical records showing vasodilator responses to PNS ( $black-triangle$ ) and bolus infusion of CGRP ( $bullet$ ) and the effects of perfusion of TTX(100 nM) (A) or CGRP receptor antagonist, CGRP(8-37) (500 nM)(B), in the perfused mesenteric vascular beds from 15-week-oldSHRs. The vascular tone was increased by perfusion of methoxamine(7 µM) in the presence of guanethidine (5 µM). PPV, papaverineperfusion.

The PNS-induced (1 and 2 Hz) vasodilator responses in preparations from 8-week-old SHRs were similar in magnitude to the vasodilationin age-matched WKY preparations, but the PNS-induced vasodilationin 15-week-old SHRs was significantly less than that in 8-week-oldSHRs and 15-week-old WKYs (table 1). Only a small reduction inthe PNS-induced vasodilation occurred with age in the WKY preparations(table 1).

Effects of AngI and AngII on neurogenic vasodilator response. As shown in figure 2 and table 2, the perfusion of AngI (50 and 100 nM) and AngII (50 and 100 nM) in both WKY and SHR preparationscaused a transient increase in perfusion pressure because of vasoconstrictionin a concentration-dependent manner. The vasoconstrictor responsesto AngI and AngII were significantly greater in the SHR preparationsthan in the WKY preparations (table 2). No significant differencein the AngI- and AngII-induced vasoconstrictions between 8-week-oldSHRs and 15-week-old SHRs or between 8-week-old WKYs and 15-week-oldWKYs occurred, however (table 2).

View larger version (30K):
[in this window]
[in a new window]

Fig. 2. Typical records showing the effects of AII (100 nM) on vasodilator responses to PNS (2 Hz) in the absence (B) and presence(C) of AII receptor antagonist, [Sar¹,Ile⁸]AII (500 nM), in the perfused mesenteric vascular bed from 15-week-oldspontaneously hypertensive rats (SHR). S₁, S₂ and S₃ indicatethe first, second and third PNS, respectively. AII was perfusedthroughout S₂. The vascular tone was raised by perfusion of methoxamine(7 µM) in the presence of guanethidine (5 µM). A, control responses.PPV, papaverine perfusion.

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

TABLE 2
Vasoconstrictor responses to perfusion of AngI and AngII and RS in the perfused mesenteric vascular bed with active tone producedby methoxamine (5 µM) and guanethidine (7 µM) in WKYs and SHRs^a

In preparations from 8- and 15-week-old SHRs, both AngI (50 and 100 nM) and AngII (50 and 100 nM) caused a concentration-dependentinhibition of the vasodilator response to PNS (figs. 2 and 3).The inhibitory effect of AngI and AngII was much greater in 15-week-oldSHRs than in 8-week-old SHRs. However, in WKY preparations fromboth ages, neither AngI nor AngII inhibited the PNS-induced vasodilation(fig. 3).

View larger version (19K):
[in this window]
[in a new window]

Fig. 3. Effects of angiotensin I (AI) and II (AII) on vasodilator responses to periarterial nerve stimulation (2 Hz) in perfused mesentericvascular beds from 8- and 15-week-old (wks) WKYs (circles) andSHRs (triangles). $open circle$ $triangle$ , control ratio without angiotensins; $bullet$ $black-triangle$ ,ratio in the presence of AI or AII concentrations of 50 and 100nM. *P < .01, **P < .01, compared with control (Dunnett's test).

Effects of AngII receptor antagonist and ACE inhibitors on AngI- and AngII-induced inhibition. In both 15-week-old SHRs and WKYs, vasoconstrictor responses to AngI and AngII were abolished by the AngII antagonist, [Sar¹,Ile⁸]AngII (500 nM), and the AngI-induced vasoconstriction was inhibitedby the ACE inhibitors captopril (5 µM) and temocapril (500 nM)(table 3).

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

TABLE 3
Effects of AngII receptor antagonist ([Sar¹,Ile⁸]AngII, 1 µM) and AngI-converting enzyme inhibitors (captopril, 5 µM; temocapril,500 nM) on vasoconstrictor responses to AngI and AngII and RSin the perfused mesenteric vascular bed with active tone producedby methoxamine (5 µM) and guanethidine (7 µM) in WKYs and SHRs^a

In preparations from 15-week-old SHRs, the inhibitory effects of AngI and AngII on the neurogenic vasodilation were antagonizedby the AngII antagonist, [Sar¹,Ile⁸]AngII (500 nM) (fig. 4), and the effect of AngI was also inhibitedby captopril (5 µM) and temocapril (500 nM). In contrast, in thepreparations from WKYs, the neurogenic vasodilation in responseto PNS was not affected by the AngII antagonist or ACE inhibitors.

View larger version (25K):
[in this window]
[in a new window]

Fig. 4. Effects of the angiotensin (A) receptor antagonist, [Sar¹,Ile⁸]AII (500 nM), and AngI-converting enzyme inhibitors, captopril(Capt, 5 µM) and temocapril (Temcp, 500 nM) on the inhibitoryeffect of AngI (A I) and AngII (A II) in the perfused mesentericvascular beds from 15-week-old (wks) WKYs ( $square$ ) and SHRs ( $black-square$ ). *P< .05,**P < .01, compared with AngI and AngII alone (Dunnett'stest).

Effect of AngI and AngII on CGRP-LI release induced by PNS. In the preparations from 15-week-old SHRs and WKYs, PNS at 2 Hz evoked an increase in CGRP-LI release in the perfusate, whichwas significantly less in the SHRs than in the WKYs (WKY, 0.8373± 0.114 fmol/ml, n = 14; SHR, 0.2877 ± 0.042 fmol/ml, n = 15;P < .01, Student's t test). This release was abolished by TTX(100 nM) and Ca⁺⁺ removal from the medium (data not shown). As shown in table 4,AngI and AngII (100 nM) in SHR but not WKY preparations inhibitedthe release of CGRP induced by PNS. A significant difference fromthe control was found in the inhibition of AngII.

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

TABLE 4
Effect of AngII on release of CGRP-LI (fmol/ml) induced by PNS in perfused mesenteric vascular beds with active tone in SHRsand WKYs^a

Effect of AngII on vasodilator response to bolus infusion of exogenous CGRP. In preparations from 15-week-old SHRs and WKYs, a bolus infusion of exogenous CGRP (100 pmol) caused a long-lasting reductionin perfusion pressure because of vasodilation, which was antagonizedby CGRP(8-37) (fig. 1B). The control I₂/I₁ ratios in SHR and WKYpreparations were 0.974 ± 0.062 (n = 6) and 1.002 ± 0.025 (n =6), respectively. The perfusion of AngII (100 nM) did not affectthe vasodilator response to bolus infusion of exogenous CGRP:I₂/I₁ ratio in SHR (n = 6) and WKY (n = 6) preparations, 1.0071± 0.070 and 0.967 ± 0.051, respectively.

Effect of RS on neurogenic vasodilation induced by PNS. As shown in figure 5 and table 2, the perfusion of RS (100 and 500 nM) in WKY and SHR preparations caused a transient increasein perfusion pressure, because of vasoconstriction, in a concentration-dependentmanner. The vasoconstrictor responses to RS were significantlygreater in SHR than in WKY (table 2), but no significant differencein the RS-induced vasoconstriction between 8-week-old SHRs and15-week-old SHRs or between 8-week-old WKYs and 15-week-old WKYsoccurred (table 2). In preparations from 15-week-old SHRs andWKYs, the vasoconstrictor response to 500 nM RS was abolishedby [Sar¹,Ile⁸]AngII (500 nM) and inhibited by ACE inhibitors (5 µM captopriland 500 nM temocapril), more so in WKYs than in SHRs (table 3).

View larger version (29K):
[in this window]
[in a new window]

Fig. 5. Typical records showing the effect of RS (500 nM) on vasodilator responses to PNS ( $black-triangle$ , 2 Hz) in the absence (B) and presence(C) of the AngII (A II) receptor antagonist, [Sar¹,Ile⁸]AII (1 µM), in the perfused mesenteric vascular bed from 15-week-oldSHRs. S₁, S₂ and S3 indicate the first, second and third PNS,respectively. RS was perfused throughout S₂. The vascular tonewas increased by continuous perfusion of methoxamine (7 µM) inthe presence of guanethidine (5 µM). A, control responses; PPV,papaverine perfusion.

In preparations from 15- but not 8-week-old SHRs, RS (100 and 500 nM) caused a significant inhibition of the vasodilator responseto PNS (figs. 5 and 6). The inhibitory effect of RS was much greaterin the 15-week-old SHRs than in the 8-week-old SHRs. In WKY preparationsof both ages, however, RS did not inhibit the PNS-induced vasodilation(fig. 6).

View larger version (20K):
[in this window]
[in a new window]

Fig. 6. Effect of RS on vasodilator responses to PNS (2 Hz) in perfused mesenteric vascular beds from 8- and 15-week-old (wks) WKYs(circles) and SHRs (triangles). $open circle$ $triangle$ , control ratio without RS; $bullet$ $black-triangle$ , ratio in the presence of RS at concentrations of 100 and 500nM. **P < .01, compared with control (Dunnett's test).

In 15-week-old SHRs but not in WKYs, the inhibitory effect of RS on PNS-induced vasodilation was antagonized by the AngIIantagonist and ACE inhibitors (fig. 7).

View larger version (20K):
[in this window]
[in a new window]

Fig. 7. Effects of the AngII (A II) receptor antagonist, [Sar¹,Ile⁸]AII (500 nM), and ACE inhibitors, captopril (Capt, 5 µM) and temocapril(Temcp, 500 nM) on the inhibitory effect of RS in the perfusedmesenteric vascular beds from 15-week-old (wks) WKYs ( $square$ ) and SHRs( $black-square$ ). *P < .05, **P < .01, compared with RS alone (Dunnett's test).

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

The present study demonstrated that frequency-dependent vasodilator responses to PNS in the mesenteric arteries isolated fromboth SHRs and WKYs were abolished by the neurotoxin TTX and theCGRP receptor antagonist CGRP(8-37), which indicates that theresponses are neurogenic and mediated by endogenous CGRP whichis released by CGRP nerves. These results agree with previousreports (Kawasaki et al., 1990c), and confirm the earlier findingsthat neurogenic vasodilation in response to CGRP nerve stimulationin aged SHRs is less than in age-matched WKYs and decreases withage, and that the neurogenic release of CGRP-LI evoked by PNSin aged SHRs was significantly less than that in age-matched WKYs(Kawasaki et al., 1990c; Kawasaki and Takasaki, 1992). Thus, thepresent results support our proposal that the function of CGRPnerves in SHRs decreases with age.

In the present study, both AngI and AngII inhibited the neurogenic vasodilator response to PNS in SHRs but not in WKYs. Theinhibitory effect of AngI and AngII was abolished by the AngIIreceptor antagonist, [Sar¹,Ile⁸]AngII, which indicates that the effect is mediated by AngII receptors.The effect of AngI was also inhibited by the ACE inhibitors captopriland temocapril, which suggests that AngII locally converted fromAngI in the mesenteric vasculature is involved in this effectin vitro. Additionally, RS attenuated the neurogenic vasodilationin response to the PNS of the SHR preparations, which was antagonizedby the AngII receptor antagonist and by ACE inhibitors. Thus,AngII locally converted in the vasculature is responsible forthe inhibitory effect of RS.

Evidence for the presence of a local renin-angiotensin system in the blood vessel wall is compelling (Mizuno et al., 1988;Dzau, 1989; Ziogas and Story, 1991; Hilgers et al., 1991). Sucha local system in the vasculature could synthesize and releaseAngII, which exerts local autocrine-paracrine influences on thevascular function (Malik and Nasjletti, 1976; Kawasaki et al.,1984). This concept supports the present suggestion that AngIand RS act through AngII, which is locally converted in the mesentericvasculature.

The results of the present study show that AngII caused a decrease in the neurogenic release of CGRP-LI in response to PNSof the SHR preparations but not the WKY preparations. However,AngII had no significant effect on vasodilator responses to exogenouslyapplied CGRP in the SHR preparations. These results strongly suggestthat AngII acts on a presynaptic site of CGRP nerves to decreasethe neurogenic release of CGRP. It is widely accepted that AngIIincreases the release of neurotransmitter to enhance the autonomicneurotransmission, especially in the vasculature. However, severalreports have shown that AngII has the capacity to inhibit theautonomic neurotransmission by decreasing the release of transmitterin the rabbit ear artery (Ronai, 1990), pig renal artery (Fergusonand Randall, 1989) and rabbit vas deferens (Trachte, 1988). Additionally,AngII has been reported to inhibit the release of acetylcholinein the human and rat cerebral cortex (Barnes et al., 1989, 1990).The release of endogenous dopamine in the pig renal artery seemedlikely to play a part in this inhibition (Ferguson and Randall,1989). In the rabbit ear artery (Ronai, 1990), a PG-mediated mechanismhas been proposed because AngII stimulates the synthesis of PGI₂and PGE₂ (Dusting et al., 1981). However, in the rabbit vas deferens,PGs did not mediate the inhibitory effect of AngII on the autonomicneurotransmission (Trachte, 1988). Furthermore, PGs such as PGE₁but not PGI₂ have been reported to enhance the CGRP release fromthe capsaicin-sensitive nerves (Franco-Cereceda, 1989). Takentogether, these findings suggest that the PG-mediated mechanismis unlikely to play a major role in the inhibitory effect of AngIIon the neurotransmission of CGRP nerves. It is conceivable thatAngII acts directly on a presynaptic site of action (probablyAngII receptors) in the CGRP nerve to inhibit the release of CGRP.

The present results also show that the inhibitory effect of AngII on the neurotransmission of CGRP nerves was specific tothe SHR preparations and became clear with age. This finding raisesthe hypothesis that SHRs have an altered function and sensitivityto AngII receptors, which are probably present on the CGRP nervesin the resistance blood vessel; or the CGRP nerves of SHRs becomenewly endowed with such presynaptic AngII receptors as the SHRsage. Such an altered sensitivity to AngII receptors in the adrenergicneurotransmission has been shown by the finding that the facilitatoreffect of AngII is enhanced in the mesenteric vasculature of SHRs(Kawasaki et al., 1982a).

Previous studies demonstrated that the CGRP nerves inhibit the adrenergic nerve-mediated vasoconstriction via direct vasodilationof CGRP released (Kawasaki et al., 1990a), whereas the adrenergicnerves decrease the release of CGRP from the CGRP nerves to inhibitCGRP nerve-mediated function (Kawasaki et al., 1990b, 1991). Moreover,we have observed that the CGRP nerve-mediated function in theSHR mesenteric vasculature decreases with age (Kawasaki et al.,1990c; Kawasaki and Takasaki, 1992). The current findings thatRS, AngI and AngII attenuate the neurotransmission of CGRP nervesin the SHRs suggest that the vascular AngII, which is locallyconverted in the resistance blood vessel, contributes to the decreasedfunction of CGRP nerves. This notion is supported by the previousfinding that long-term treatment of SHRs with the ACE inhibitorprevents the decreased vasodilation mediated by CGRP nerves (Kawasaki,1992).

Although increased levels of renin, which is synthesized in the blood vessel wall and partly taken up from the plasma (Inagamiet al., 1991; Mizuno et al., 1986), have been reported in SHRblood vessels (Naruse and Inagami, 1982), recent studies havepresented little evidence for increased production of AngII inthe blood vessels of SHRs (Nakamura et al., 1986). On the contrary,the decreased mRNA level of angiotensinogen in periarterial adipocytestaken from SHRs suggested the reduced production of AngII (Naftilanet al., 1988). However, there is evidence that sensitivity toAngII receptors can be enhanced in the mesenteric artery of theSHR (Kawasaki et al., 1982a, 1984; Li and Jackson, 1989). In fact,the present experiments showed that the SHR vasoconstrictor responsesto perfusion of AngI and AngII were significantly greater thanthose in WKY preparations. In addition to this mechanism, thecurrent finding that AngII has the ability to inhibit the functionof vasodilator nerves only in SHRs suggests that the vascularrenin-angiotensin system could induce increased vascular tonewithout an elevated concentration of AngII in the blood vesselwall.

In conclusion, the exogenous and locally converted AngII in the SHR mesenteric artery has the ability to inhibit the neurotransmissionof CGRP vasodilator nerves. The present results suggest that thereduced function of CGRP nerves by the vascular renin-angiotensinsystem plays an important role in the development and maintenanceof chronic hypertension.

	Footnotes

Accepted for publication October 22, 1997.

Received for publication April 29, 1997.

¹ This study was supported in part by Grants-in-Aid 08672611 and 09672326 for Scientific Research from the Ministry of Education,Science and Culture of Japan.

Send reprint requests to: Hiromu Kawasaki, Ph.D., Department of Clinical Pharmaceutical Science, Faculty of Pharmaceutical Sciences, Okayama University, 1-1-1 Tsushimanaka, Okayama 700, Japan.

	Abbreviations

ACE, angiotensin converting enzyme; Ang, angiotensin; CGRP, calcitonin gene-related peptide; CGRP-LI, calcitonin gene-related peptide-like immunoreactivities; NANC, nonadrenergic noncholinergic; PG, prostaglandin; PNS, periarterial nerve stimulation; RS, N-acetyltetradecapeptide renin substrate; SHR, spontaneously hypertensive rat; TTX, tetrodotoxin; WKY, Wistar Kyoto rat.

	References

Top Abstract Introduction Materials & Methods Results Discussion References

Barnes JM, Barnes NM, Costall B, Horovitz ZP, Ironside JW, Naylor RJ and Williams TJ (1990) AngiotensinIIinhibits acetylcholine release from human temporal cortex: Implicationsfor cognition. Brain Res 507: 341-343[Medline].
Barnes JM, Barnes NM, Costall B, Horovitz ZP and Naylor RJ (1989) AngiotensinIIinhibits the release of [³H]acetylcholine from rat entorhinal cortex `in vivo.' BrainRes 491: 136-143[Medline].
Dusting GJ, Mullins EM and Nolan RD (1981) Prostacyclin(PGI₂) release accompanying angiotensin conversion in rat mesentericvasculature. Eur J Pharmacol 70: 129-137[Medline].
Dzau VJ (1989) Multiple pathways of angiotensin productionin the blood vessel wall: Evidence, possibilities and hypotheses. JHypertens 7: 933-936[Medline].
Ferguson DR and Randall MD (1989) Neurotransmissionin pig renal artery: The action of angiotensinII and dopamine. BrJ Pharmacol 96: 279-282[Medline].
Folkow B, Hallback M, Lundgren Y and Weiss L (1970) Structurallybased increase in flow resistance in spontaneously hypertensiverats. Acta Physiol Scand 79: 373-378[Medline].
Franco-Cereceda A (1989) Prostaglandins and CGRP releasefrom cardiac sensory nerves. Naunyn-Schmiedeberg'sArch Pharmacol 340: 180-184[Medline].
Head RJ (1989) Hypernoradrenergic innervation: its relationshipto functional and hyperplastic changes in the vascular of thespontaneously hypertensive rat. BloodVessels 26: 1-20[Medline].
Hilgers KF, Mann JFE, Hilgenfeldt U and Ganten D (1991) Vascularproduction and regulation of angiotensin. BloodVessels 28: 201-209[Medline].
Inagami T, Murakami T, Higuchi K and Nakajo S (1991) Rolesof renal and vascular renin in spontaneous hypertension and switchingof the mechanism upon nephrectomy: Lack of hypotensive effectsof inhibition of renin, converting enzyme, and angiotensin IIreceptor blocker after bilateral nephrectomy. AmJ Hypertens 4: 15S-22S[Medline].
Kawasaki H (1992) Effects of chronic administrationof antihypertensive drugs on vasodilation mediated by calcitoningene-related peptide-containing vasodilator nerves in spontaneouslyhypertensive rats. Clin ExpPharmacol Physiol 19: 569-573[Medline].
Kawasaki H, Cline WH, Jr and Su C (1982a) Enhancedangiotensin-mediated facilitation of adrenergic neurotransmissionin spontaneously hypertensive rats. JPharmacol Exp Ther 221: 112-116[Abstract/Free Full Text].
Kawasaki H, Cline WH, Jr and Su C (1982b) Enhancedpresynaptic beta-adrenoceptor-mediated modulation of vascularadrenergic neurotransmission in spontaneously hypertensive rats. JPharmacol Exp Ther 223: 721-728[Free Full Text].
Kawasaki H, Cline WH, Jr and Su C (1984) Involvementof the vascular renin-angiotensin system in beta adrenergic receptor-mediatedfacilitation of vascular neurotransmission in spontaneously hypertensiverats. J Pharmacol Exp Ther 231: 23-32[Abstract/Free Full Text].
Kawasaki H, Nuki C, Saito A and Takasaki K (1990a) Roleof calcitonin gene-related peptide-containing nerves in the vascularadrenergic neurotransmission. JPharmacol Exp Ther 252: 403-409[Abstract/Free Full Text].
Kawasaki H, Nuki C, Saito A and Takasaki K (1991) NPYmodulates neurotransmission of CGRP-containing vasodilator nervesin rat mesenteric arteries. AmJ Physiol 261: H683-H690[Abstract/Free Full Text].
Kawasaki H, Nuki C and Takasaki K (1990b) Adrenergicmodulation of calcitonin gene-related peptide (CGRP)-containingnerve-mediated vasodilation in the rat mesenteric resistance vessel. BrainRes 506: 287-290[Medline].
Kawasaki H, Saito A and Takasaki K (1990c) Age-relateddecrease of calcitonin gene-related peptide-containing vasodilatorinnervation in the mesenteric resistance vessel of the spontaneouslyhypertensive rat. Circ Res 67: 733-743[Abstract/Free Full Text].
Kawasaki H and Takasaki K (1992) Age-relateddecrease of neurogenic release of calcitonin gene-related peptidefrom perivascular nerves in spontaneously hypertensive rats. ClinExp Hyper A 14: 989-1001.
Kawasaki H, Takasaki K, Saito A and Goto K (1988) Calcitoningene-related peptide acts as a vasodilator neurotransmitter inmesenteric resistance vessels of the rat. Nature 335: 164-167[Medline].
Li P and Jackson EK (1989) Enhancedslow-pressor response to angiotensin II in spontaneously hypertensiverats. J Pharmacol Exp Ther 251: 909-921[Abstract/Free Full Text].
Malik KU and Nasjletti A (1976) Facilitationof adrenergic transmission by locally generated angiotensinIIin rat mesenteric arteries. CircRes 38: 26-30[Abstract/Free Full Text].
Mizuno K, Nakamura M, Higashimori K and Inagami T (1988) Localgeneration and release of angiotensinII in peripheral vasculartissue. Hypertension 11: 223-229[Abstract/Free Full Text].
Mizuno K, Watari H, Tani M and Fukuchi S (1986) Activeand inactive renin-like enzymes in the arterial wall of the spontaneouslyhypertensive rats. Clin ExpHypertens A 7: 1707-1717.
Naftilan AJ, Ryan TJ, Pratt RE and Dzau V (1988) Angiotensinogengene expression in the vascular wall is abnormal in the genetichypertensive rat. Clin Res 36: 430A.
Nakamura M, Jackson EK and Inagami T (1986) Role of vascular angiotensin II released by 144 $beta$ -adrenergic stimulationin rat. J Cardiovasc Pharmacol 8:suppl.10, S1-S5.
Naruse M and Inagami T (1982) Antibody-sensitiverenin of adrenal and resistance vessels is markedly elevated inspontaneously hypertensive rats. ClinSci 63: 187s-189s.
Ronai AZ (1990) Inhibition of neurotransmission by angiotensinIand II in rabbit isolated ear artery. EurJ Pharmacol 179: 281-286[Medline].
Toda N and Okamura T (1992) Mechanismof neurally induced monkey mesenteric artery relaxation and contraction. Hypertension 19: 161-166[Abstract/Free Full Text].
Trachte GJ (1988) Prostaglandins do not mediate theinhibitory effects of angiotensin II and III on autonomic neurotransmissionin the rabbit vas deferens. Prostaglandins 36: 215-228[Medline].
Zimmerman BG (1983) Peripheral neurogenic factors inacute and chronic alterations of arterial pressure. CircRes 53: 121-130[Free Full Text].
Ziogas J and Story DF (1991) AngiotensinIIgeneration in the rat vena cava: Stimulation of local synthesisby $beta$ -adrenoceptor activation. Naunyn-Schmiedeberg'sArch Pharmacol 343: 31-36[Medline].

0022-3565/98/2842-0508$03.00/0
THE JOURNAL OF PHARMACOLOGY AND EXPERIMENTAL THERAPEUTICS
Copyright © 1998 by The American Society for Pharmacology and Experimental Therapeutics

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 Google Scholar

Google Scholar

Articles by Kawasaki, H.

Articles by Gomita, Y.

Search for Related Content

PubMed

PubMed Citation

Articles by Kawasaki, H.

Articles by Gomita, Y.

Angiotensin Inhibits Neurotransmission of Calcitonin Gene-Related Peptide-Containing Vasodilator Nerves in Mesenteric Artery of Spontaneously Hypertensive Rats1

Angiotensin Inhibits Neurotransmission of Calcitonin Gene-Related Peptide-Containing Vasodilator Nerves in Mesenteric Artery of Spontaneously Hypertensive Rats¹