Abstract
We had shown that bradykinin (BK) generated by cardiac sympathetic nerve endings (i.e., synaptosomes) promotes exocytotic norepinephrine (NE) release in an autocrine mode. Because the synaptosomal preparation may include sensory C-fiber endings, which BK is known to stimulate, sensory nerves could contribute to the proadrenergic effects of BK in the heart. We report that BK is a potent releaser of NE from guinea pig heart synaptosomes (EC50 ∼20 nM), an effect mediated by B2 receptors, and almost completely abolished by prior C-fiber destruction or blockade of calcitonin gene-related peptide and neurokinin-1 receptors. C-fiber destruction also greatly decreased BK-induced NE release from the intact heart, whereas tyramine-induced NE release was unaffected. Furthermore, C-fiber stimulation with capsaicin and activation of calcitonin gene-related peptide and neurokinin-1 receptors initiated NE release from cardiac synaptosomes, indicating that stimulation of sensory neurons in turn activates sympathetic nerve terminals. Thus, BK is likely to release NE in the heart in part by first liberating calcitonin gene-related peptide and Substance P from sensory nerve endings; these neuropeptides then stimulate specific receptors on sympathetic terminals. This action of BK is positively modulated by cyclooxygenase products, attenuated by activation of histamine H3 receptors, and potentiated at a lower pH. The NE-releasing action of BK is likely to be enhanced in myocardial ischemia, when protons accumulate, C fibers become activated, and the production of prostaglandins and BK increases. Because NE is a major arrhythmogenic agent, the activation of this interneuronal signaling system between sensory and adrenergic neurons may contribute to ischemic dysrhythmias and sudden cardiac death.
We had shown that bradykinin (BK) generated by cardiac sympathetic nerve endings (i.e., synaptosomes) promotes exocytotic norepinephrine (NE) release in an autocrine fashion (Seyedi et al., 1997). Because the synaptosomal fraction may also contain sensory C-fiber endings, which BK is known to stimulate (Franco-Cereceda, 1988; Geppetti, 1993;Imamura et al., 1996b; Kopp et al., 1997; Wood and Docherty, 1997), sensory nerves could play a role in the proadrenergic effects of BK in the heart. A BK-initiated interaction between sensory and adrenergic nerves would be important in myocardial ischemia. Indeed, myocardial ischemia is known to be associated with an enhanced release of NE (Schömig, 1990; Imamura et al., 1994, 1996a), BK (Kimura et al., 1973; Matsuki et al., 1987; Lamontagne et al., 1995) and sensory neurotransmitters, such as calcitonin gene-related peptide (CGRP) and Substance P (Franco-Cereceda, 1988, 1989; Milner et al., 1989; Mair et al., 1990).
Accordingly, we investigated whether the presence of intact cardiac C fibers is a prerequisite for the BK-induced release of NE from sympathetic nerve endings and whether this action is affected by specific blockade of sensory transmitter receptors. Furthermore, we assessed possible modulatory mechanisms capable of up- or down-regulating BK-initiated NE release in the heart.
Our findings identify a novel BK-promoted cross-talk system between adrenergic and sensory nerve endings in the heart, whereby BK produced at adrenergic terminals (Seyedi et al., 1997) initiates a paracrine release of CGRP and Substance P from C fibers, and these neuropeptides signal back to adrenergic nerve endings to promote NE release. This action of BK is mediated by B2 receptors, involves a cyclooxygenase-mediated step, is negatively modulated by histamine H3 receptors, and is greatly potentiated at a lower pH.
Materials and Methods
NE Release from Cardiac Synaptosomes.
Male Hartley guinea pigs (Harlan Bioproducts for Science, Inc., Indianapolis, IN) weighing 250 to 300 g were sacrificed by cervical dislocation under light anesthesia with CO2 vapor in accordance with institutional guidelines. The rib cage was dissected away, and the heart was rapidly excised, freed from fat and connective tissue, and transferred to a Langendorff apparatus (Park et al., 1992). Spontaneously beating hearts were perfused through the aorta for 15 min at constant pressure (40 cm of H2O) with Ringer’s solution at 37°C saturated with 100% O2 (pH 7.5; Park et al., 1992). This procedure ensured that no blood traces remained in the coronary circulation. When indomethacin was used, hearts were perfused with indomethacin (10 μM) for an additional 10 min. In either case, at the end of the perfusion, hearts were minced in ice-cold 0.32 sucrose containing 1 mM EGTA, pH 7.4. Synaptosomes were isolated as previously described (Seyedi et al., 1997). Minced tissue was digested with 40 mg collagenase (type 2; Worthington Biochem. Corp., Freehold, NJ) per 10 ml of HEPES-buffered saline solution (HBS) per gram of wet heart weight for 1 h at 37°C. HBS contained 1 mM pargyline to prevent enzymatic destruction of synaptosomal NE. After low-speed centrifugation (10 min at 120g at 4°C), the resulting pellet was suspended in 10 volumes of 0.32 M sucrose and homogenized with a Teflon/glass homogenizer. The homogenate was spun at 650g for 10 min at 4°C and the pellet rehomogenized and respun. The pellet containing cellular debris was discarded, and the supernatants from the last two spins were combined and equally subdivided into 10 to 12 tubes. Each tube was centrifuged for 20 min at 20,000g at 4°C. This pellet, which contained cardiac synaptosomes, was resuspended in HBS to a final volume of 500 μl in the presence or absence of pharmacological agents for a total of 20 min in a water bath at 37°C. Each suspension functioned as an independent sample and was used only once. In every experiment, one sample was untreated (control, basal NE release), and others were incubated with drugs for 20 min. When antagonists were used, samples were incubated with the antagonist for 20 min before incubation with the agonist. Controls were incubated for an equivalent length of time without drugs. At the end of the incubation period, each sample was centrifuged for 20 min (20,000g at 4°C). The supernatant was assayed for NE content by HPLC with electrochemical detection (Seyedi et al., 1997). The pellet was assayed for protein content by a modified Lowry procedure (Seyedi et al., 1997).
Capsaicin Pretreatment In Vivo.
Guinea pigs were anesthetized with pentobarbital sodium (25 mg/kg i.p.) and artificially ventilated with a rodent respirator (Harvard Apparatus), according to institutional guidelines. Theophylline (100 mg/kg i.p.) was given to counteract respiratory impairment. Capsaicin (total dose, 50 mg/kg s.c.) was administered 6 h before in vitro experimentation; this has been shown to cause a total loss of CGRP-containing nerves within the heart (Imamura et al., 1996b). Control animals received the same treatment except for capsaicin. Hearts from control and capsaicin-treated animals were excised and perfused in the Langendorff apparatus as described above. Most hearts were used for the preparation of synaptosomes. Others were perfused with BK (1 μM) for 20 min to determine whether C-fiber destruction affects the ability of BK to elicit NE release from the intact heart. Destruction of C fibers in capsaicin-pretreated hearts was ascertained by measuring NE overflow in response to a 20-min capsaicin (1 μM) perfusion. NE availability in capsaicin-pretreated hearts was assessed by measuring NE overflow in response to a 20-min tyramine (1 μM) perfusion. NE overflow into the coronary effluent was assayed by HPLC (as described above) before and during perfusions with capsaicin, BK, and tyramine.
Statistics.
Values are expressed as mean percent increases above basal NE release (synaptosomes) or basal NE overflow (isolated hearts) ± S.E. There were no statistically significant differences in basal NE release among the various experiments. Analysis by one-way ANOVA was used, followed by post hoc testing (Dunnett’s test). In two instances (see Figs. 7 and 8), paired and unpaired Student’s t tests were used, respectively. A value ofp < .05 was considered statistically significant. The EC50 for BK-induced NE release was calculated by nonlinear regression curve fitting with the GraphPad Prism program (GraphPad Software, Inc., San Diego, CA).
Drugs and Chemicals.
CGRP, CGRP8–37, and Substance P were purchased from Peninsula Labs., Inc. (Belmont, CA). Capsazepine, Hoe 140, imetit dihydrobromide, and thioperamide maleate were purchased from Research Biochemicals International (Natick, MA). Atropine sulfate, BK, [des-arg9leu8]BK, capsaicin, indomethacin, theophylline, and tyramine hydrochloride were purchased from Sigma-Aldrich Chemical Co. (St. Louis, MO). CP 99,994 was a gift from Pfizer Central Research. Capsaicin was dissolved in 100% ethanol. Capsazepine and indomethacin were dissolved in dimethyl sulfoxide. Further dilutions were made with distilled water; at the concentration used, dimethyl sulfoxide and ethanol did not affect mediator release.
Results
Release of Synaptosomal NE by BK and Capsaicin.
Incubation of the cardiac synaptosomal fraction with 1 to 100 nM BK caused a concentration-dependent NE release that reached a maximum of ∼32% above basal level (EC50 ∼20 nM; Fig.1). The concentration-response curve was not modified in the presence of atropine (1 μM; Fig. 1). The BK B2-receptor antagonist HOE 140 (3 nM; ≈pA2) caused a marked downward shift in the BK concentration-response curve. In contrast, the B1-receptor antagonist [des-arg9leu8]BK (1 μM; 2.5 × pA2) failed to shift the BK concentration-response curve (Fig. 1).
Incubation of the synaptosomal fraction with the sensory neuron excitotoxin capsaicin (100 nM) elicited an ∼45% increase in NE release above basal level (Fig. 2). This effect was reduced by ∼60% in the presence of the capsaicin-receptor antagonist capsazepine (10 μM). When synaptosomes were isolated from hearts of guinea pigs pretreated in vivo with capsaicin (50 mg/kg, 6 h earlier) to destroy sensory C fibers (Imamura et al., 1996b), NE release in response to a subsequent incubation with capsaicin was reduced by ∼60% as compared with cardiac synaptosomes from sham-treated animals (Fig. 3A). Similarly, capsaicin pretreatment in vivo reduced the response of cardiac synaptosomes to BK by ∼75% (Fig. 3B).
Release of Synaptosomal NE by CGRP and Substance P.
Incubation of the synaptosomal fraction with capsaicin or BK in the presence of antagonists of the sensory neuropeptide transmitters CGRP and Substance P greatly diminished the effects of capsaicin and BK. The CGRP-receptor antagonist CGRP8–37 (1 μM; pKi, 6.5–8.0; Bell and McDermott, 1996) decreased the NE-releasing effects of capsaicin and BK by 50 to 60% (n = 6 + 6, p < .01). The Substance P/tachykinin neurokinin-1 (NK1)-receptor antagonist CP 99,994 (100 nM; pKi, 7.3–9.3; Regoli et al., 1994) decreased the NE-releasing effects of capsaicin and BK by ∼60% (n = 6 + 6, p < .01). As shown in Fig.4, A and B, when these neuropeptide-receptor antagonists were used in combination, at 5- and 10-fold greater concentrations (i.e., CGRP8–37 5 μM and CP 99,994 1 μM), the blockade of the NE-releasing effect of capsaicin and BK remained at a 60 to 65% level.
CGRP (100 nM) and Substance P (1 μM) each induced NE release from cardiac synaptosomes. As shown in Fig. 4, C and D, CGRP and Substance P caused an ∼40% and ∼30% increase in NE release above basal levels, respectively. The NE-releasing effect of CGRP was antagonized by the CGRP-receptor blocker CGRP8–37 (1 μM), whereas the NE-releasing effect of Substance P was antagonized by the Substance P-receptor blocker CP 99,994 (100 nM; Fig. 4, C and D).
Modulation of BK- and Capsaicin-Induced Release of NE from Cardiac Synaptosomes.
Inhibition of cyclooxygenase with indomethacin (10 μM) reduced the NE-releasing effect of capsaicin and BK. As shown in Fig. 5, after pretreatment with indomethacin, synaptosomes released ∼70% less NE than untreated controls in response to either capsaicin or BK.
The histamine H3-receptor agonist imetit (100 nM) diminished the amounts of NE released by capsaicin and BK. In synaptosomes incubated with imetit, capsaicin- and BK-induced NE release was reduced in each case by ∼40%. The effects of imetit were blocked by the histamine H3-receptor antagonist thioperamide (300 nM; Fig. 6).
Acidosis greatly potentiated the NE-releasing effect of BK. As shown in Fig. 7, a reduction in pH from 7.4 to 7.0, 6.5, and 5.5 caused a progressive leftward and upward shift of the concentration-response curve for the BK-induced NE release. Thus, at pH levels between 7.0 and 5.5, the effect of any given BK concentration was ∼20 to 90% greater than at pH 7.4. Basal NE release was unaffected by lowering the pH from 7.4 to 6.5 (basal NE release was 1.50 ± 0.06, 1.53 ± 0.06, and 1.59 ± 0.06 pmol/mg protein at pH 7.4, 7.0, and 6.5, respectively; n = 8–20; not significant). In contrast, at pH 5.5, basal NE release was ∼40% greater than at pH 7.4 (p < .01); addition of BK further increased NE release by ∼50%.
BK-Enhanced NE Overflow from Isolated Guinea Pig Hearts: Modification by Capsaicin Pretreatment.
We next determined whether C-fiber destruction affects the ability of BK to elicit NE release from the intact heart. As shown in Fig. 8A, the overflow of NE from isolated guinea pig hearts increased by 48% during a 20-min perfusion with BK (1 μM). In contrast, in hearts from capsaicin-pretreated animals, NE overflow increased only by 17% in response to BK (p < .001, by unpaired Student’st test; Fig. 8A). Not shown in Fig. 8 is that NE overflow increased by 45.8 ± 12.2% in response to a 20-min perfusion with capsaicin (1 μM) but only by 10.5 ± 5.0% in capsaicin-pretreated hearts (p < .05;n = 4 + 4). In contrast, the increase in NE overflow elicited by a 20-min perfusion with tyramine (1 μM) was unaffected by capsaicin pretreatment (Fig. 8B), indicating that the diminished BK and/or capsaicin response in capsaicin-pretreated hearts was not caused by a loss in NE availability.
Discussion
Our findings demonstrate that stimulation of cardiac sensory C fibers with BK elicits the release of NE from sympathetic nerve endings, an action attenuated by prior C-fiber destruction or by CGRP- and Substance P-receptor antagonists. This suggests that BK, at least in part, initiates the release of CGRP and Substance P from C fibers; these neuropeptides subsequently act on adrenergic nerve endings to promote NE release. This action of BK is mediated by B2 receptors; positively and negatively modulated by cyclooxygenase products and histamine H3receptors, respectively; and greatly potentiated at a lower pH.
We had previously reported that BK promotes NE release from adrenergic nerve endings in a preparation of cardiac synaptosomes (Seyedi et al., 1997). This synaptosomal fraction is likely to contain other types of nerve endings, such as cholinergic terminals and unmyelinated sensory C fibers. Inasmuch as atropine does not modify the NE-releasing effects of BK (Seyedi et al., 1997; see also Fig. 1), cholinergic nerves are not likely to contribute to these effects. In contrast, sensory C fibers are known to be highly sensitive to BK (Franco-Cereceda, 1988;Geppetti, 1993; Wood and Docherty, 1997). Thus, we questioned whether the cardiac sympathomimetic effects of BK might be initiated in part by an action on sensory nerves, subsequently relayed to adrenergic terminals.
First, we established that, in addition to its proexocytotic effects (Kurz et al., 1997; Seyedi et al., 1997; Chulak et al., 1998), BK elicits the release of endogenous NE from cardiac adrenergic nerves even in the absence of K+-induced depolarization. We found this action to be as potent (EC50 ∼20 nM) as the proexocytotic effect of BK (EC50 ∼17 nM; Seyedi et al., 1997) and mediated by B2receptors. In fact, B2 receptors have been consistently found to mediate the proadrenergic effects of BK (McDonald et al., 1994; Minshall et al., 1994; Chulak et al., 1995, 1998; Poxton, 1995; Dendorfer et al., 1996; Boehm and Huck, 1997; Rump et al., 1997;Seyedi et al., 1997).
Next, we sought to demonstrate that chemical stimulation of cardiac sensory C fibers results in NE release from adrenergic terminals. For this we used capsaicin, a highly specific sensory neuron excitotoxin and vanilloid-receptor agonist (Caterina et al., 1997; Wood and Docherty, 1997). We found that incubation of the cardiac synaptosomal fraction with capsaicin caused the release of endogenous NE, and this effect was inhibited by the vanilloid-receptor blocker capsazepine (Bevan et al., 1992; Caterina et al., 1997; Wood and Docherty, 1997). Moreover, prior destruction of sensory C fibers by pretreatment with capsaicin in vivo (Imamura et al., 1996b), greatly reduced NE release in response to a subsequent capsaicin administration to the intact heart and cardiac synaptosomes. This is the first demonstration that stimulation of cardiac sensory neurons in turn activates sympathetic nerve terminals.
Most important, we found that, analogous to capsaicin, nearly complete destruction of sensory C fibers markedly decreased the NE-releasing activity of BK, both in the intact heart and in the synaptosomal fraction. This decreased BK response was not caused by NE depletion. Indeed, we found that tyramine released the same amount of NE from control and capsaicin-pretreated hearts. These findings clearly indicate that sensory nerve terminals play an important role in the sympathomimetic effects of BK in the heart.
To identify the chemical signals by which sensory terminals may communicate with adrenergic fibers, we used two neuropeptide-receptor antagonists, CGRP8–37 and compound CP 99,994, that specifically block the effects of CGRP and Substance P withKis in the high and low nanomolar range, respectively (Regoli et al., 1994; Bell and McDermott, 1996). We found that the administration of exogenous CGRP and Substance P elicited the release of synaptosomal NE and that these effects were inhibited by CGRP8–37 and CP 99,994, respectively. Furthermore, we found that the NE-releasing effects of capsaicin and BK were markedly reduced by blockade of CGRP and Substance P receptors. This suggests that BK ultimately releases NE in the heart by first liberating CGRP and Substance P from sensory nerve endings; these neuropeptides then stimulate specific receptors on sympathetic nerve endings. Indeed, BK is known to release CGRP from capsaicin-sensitive nerves in guinea pig atria (Geppetti et al., 1990). We found that the NE-releasing effect of BK was not further reduced when CGRP8–37 and CP 99,994 were used in combination at 5- and 10-fold greater concentrations. Similarly, a small portion of the NE-releasing effect of BK persisted even after destruction of C fibers. Thus, BK appears to act for the most part on sensory C fibers and to a lesser extent directly on sympathetic nerve endings.
Prostaglandins are known to enhance the actions of BK on sensory nerves. Indeed, sensory neurons are endowed with cyclooxygenase activity, and indomethacin attenuates the BK-stimulated release of CGRP and Substance P from sensory neurons in culture (Vasko et al., 1994) and of CGRP from guinea pig atria (Geppetti et al., 1990). Furthermore, the BK-induced release of Substance P in the kidney is a prostaglandin-dependent phenomenon (Kopp et al., 1997), and the cyclooxygenase system contributes to enhanced BK responsiveness of chemosensitive nerve endings in heart failure (Schultz et al., 1997). Accordingly, we assessed whether endogenous prostaglandins play a role in the C-fiber-dependent sympathomimetic effects of BK in the heart. We found that pretreatment of isolated guinea pig hearts with indomethacin markedly reduced the ability of BK to release NE from the synaptosomal fraction. Analogous to BK, the NE-releasing effect of capsaicin was also significantly decreased. Thus, the C-fiber-initiated release of NE from cardiac sympathetic nerve terminals comprises a cyclooxygenase-dependent step. Conceivably, cyclooxygenase products could augment the release of neuropeptide transmitters from activated sensory fibers (Vasko et al., 1994). Also, prostaglandin-induced posttranslational modifications could increase the sensitivity of the vanilloid and B2 receptors and associated channels (Wood and Docherty, 1997).
We had previously characterized the function of inhibitory histamine H3 receptors on cardiac sensory C fibers (Imamura et al., 1996b). These receptors, activated by histamine released by CGRP from adjacent cardiac mast cells, play a major role in a regulatory negative-feedback loop that modulates neurotransmitter release from sensory nerve endings. Thus, we questioned whether this regulatory system may also modulate the sympathomimetic effect of BK in the heart. Our findings suggest that this may be the case. Indeed, the selective histamine H3-receptor agonist imetit attenuated the release of synaptosomal NE elicited by C-fiber stimulation with BK or capsaicin, and this effect was prevented by blockade of histamine H3 receptors with thioperamide. Although this demonstrates the presence of inhibitory histamine H3 receptors, it does not distinguish between receptors located on sensory (Imamura et al., 1996b) and adrenergic (Imamura et al., 1995) nerve endings in the heart, because histamine H3-receptor stimulation at either or both locations would ultimately result in a decreased NE release. Inasmuch as CGRP released from sensory endings in the heart elicits the release of histamine from local mast cells (Imamura et al., 1996b), it is likely that histamine H3 receptors become activated when C fibers are stimulated by BK, so that the release of CGRP and thus NE would be curtailed. Nevertheless, we could not directly test this hypothesis because histamine H3 receptors in the synaptosomal preparation would not be expected to be endogenously activated, given the absence of intact mast cells.
Myocardial ischemia is associated with activation of C fibers and CGRP release, probably via an increase in cation conductance (Franco-Cereceda, 1988; Franco-Cereceda and Lundberg, 1992; Wood and Docherty, 1997). This most likely occurs because tissue pH decreases in myocardial ischemia as CO2 and protons accumulate (Ichihara et al., 1991; Opie, 1991), and protons are known to activate vanilloid-gated ion channels (Wood and Docherty, 1997). Because both BK production (Kimura et al., 1973; Matsuki et al., 1987; Lamontagne et al., 1995) and NE release (Schömig, 1990; Imamura et al., 1994,1996a) are enhanced in myocardial ischemia, a lower tissue pH could potentiate the BK-initiated, C-fiber-mediated NE release. Our findings favor this hypothesis. In fact, at pH 5.5 and 6.5 (comparable to tissue pH values found in myocardial ischemia; Hirche et al., 1980; Ichihara et al., 1991; Opie, 1991), much less BK was needed to produce an increase in NE release equal to that observed at pH 7.4. Accordingly, a lower tissue pH could be mechanistically important in the BK-induced promotion of NE release in ischemia-reperfusion models (Hatta et al., 1999). Because protons increase the release of neuropeptides and prostaglandins (Franco-Cereceda and Lundberg, 1992; Wood and Docherty, 1997) and prostaglandins in turn augment peptide release (Franco-Cereceda et al., 1994), both of these factors could be involved in the pH-mediated potentiation of BK-initiated NE release. In addition to the effect of lower pH on C fibers, our data would also be consistent with a direct effect of lower pH on sympathetic nerve terminals. However, the fact that acidosis does not influence the nicotine-induced and electrically stimulated release of NE from isolated hearts (Dart and Riemersma, 1989; Kruger et al., 1995) would seem to exclude this possibility.
In conclusion (see Fig. 9), our data suggest that BK initiates the antidromic release of CGRP and Substance P by activating B2 receptors on afferent sensory C fibers (Maggi, 1995); these neuropeptides subsequently act on CGRP and NK1 receptors at adrenergic endings and promote NE release. In addition, but probably to a smaller extent, BK releases NE by directly stimulating B2 receptors at adrenergic terminals (Seyedi et al., 1997). Because BK can be generated by cardiac sympathetic nerve endings (Seyedi et al., 1997), our findings identify a novel paracrine cross talk between adrenergic and sensory nerve endings in the heart, whereby BK formed at sympathetic endings activates sensory fibers that in turn stimulate sympathetic endings via neuropeptide release. Histamine released from local mast cells by CGRP (Imamura et al., 1996b) acts at inhibitory histamine H3 receptors located at both adrenergic (Imamura et al., 1995) and sensory (Imamura et al., 1996b) nerve endings as part of a BK-initiated negative-feedback loop that ultimately limits NE release. In contrast, cyclooxygenase products appear to augment the sympathomimetic action of BK in the heart. Because the effect of BK is potentiated at a lowered pH, the NE-releasing action of BK is likely to be greatly enhanced in the setting of myocardial ischemia, where protons accumulate (Hirche et al., 1980; Ichihara et al., 1991; Opie, 1991), C fibers become activated (Franco-Cereceda, 1988; Milner et al., 1989; Franco-Cereceda and Lundberg, 1992; Wood and Docherty, 1997), and the production of prostaglandins (Berger et al., 1976, 1977; Kraemer et al., 1976) and BK (Kimura et al., 1973; Matsuki et al., 1987; Lamontagne et al., 1995) increases. Because NE is a major arrhythmogenic agent (Schömig, 1990; Schömig et al., 1991; Imamura et al., 1996a), the activation of this sensory/adrenergic interneuronal cross-talk system may contribute to ischemic dysrhythmias and sudden cardiac death.
Acknowledgments
We gratefully acknowledge the technical help of Neil C. E. Smith. Drs. Harry M. Lander and Thomas Maack provided helpful criticism.
Footnotes
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Send reprint requests to: Roberto Levi, M.D., Dept. of Pharmacology, Cornell University Weill Medical College, 1300 York Ave., New York, NY. E-mail: rlevi{at}med.cornell.edu
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↵1 This work was supported by National Institutes of Health Grants HL-34215, HL-46403, and CA-62948 and in part by a Fellowship of the American Heart Association, New York City Affiliate, to R. M.. A preliminary version of these findings was presented at Experimental Biology ’98, April, 1998 (San Francisco, CA) and was published in abstract form in FASEB J 1998;12:A398.
- Abbreviations:
- BK
- bradykinin
- CGRP
- calcitonin gene-related peptide
- NE
- norepinephrine
- Received February 11, 1999.
- Accepted April 15, 1999.
- The American Society for Pharmacology and Experimental Therapeutics