Vol. 273, Issue 4, H1933-H1940, October 1997
Positive chronotropic and inotropic effects of C-type
natriuretic peptide in dogs
Pierre
Beaulieu1,3,
René
Cardinal1,3,
Pierre
Pagé2,3,
François
Francoeur4,
Johanne
Tremblay4, and
Chantal
Lambert1
Departments of 1 Pharmacology
and 2 Surgery, Faculty of
Medicine, Université de Montréal, Montreal H3C 3J7;
3 Research Center, Hôpital
du Sacré-Coeur, Montreal H4J 1C5; and
4 Research Center,
Hôtel-Dieu de Montréal, Montreal, Quebec, Canada H2W 1T8
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ABSTRACT |
We have recently
reported that C-type natriuretic peptide (CNP) has a positive
chronotropic effect in dogs. We further investigated the effect of CNP
on canine cardiac functions: 1) in
situ, by exploring the effects of isoproterenol (10 µg), angiotensin
II (ANG II, 5 µg), and CNP (40 µg) injections
(n = 8) on computerized epicardial
mapping of atrial activation to detect a shift in pacemaker location;
2) by examining the presence of
natriuretic peptide receptor (NPR)-A and -B mRNAs in atrial and nodal
tissues using semiquantitative reverse-transcription polymerase
chain reaction; 3) in vitro, using
spontaneously beating right atrial preparations (n = 6), by recording the
transmembrane potentials of sinoatrial node (SAN) cells
before and after injection of CNP (25 µg); and 4) by observing the effects of CNP
(25 µg) on contractile force of paced isolated right atrial
preparations (n = 6). The results indicate that 1) the site of
earliest extracellular electrical activation in the SAN remains mostly
unchanged in response to CNP, whereas it shifts to the superior region
of the SAN after isoproterenol and ANG II injections;
2) NPR-A and -B mRNAs are present in
atrial and nodal tissues; 3) CNP
significantly increases the maximal rate of diastolic depolarization
and decreases the action potential duration at 75 and 90% of
repolarization; and 4) CNP
significantly increases atrial contractile force. These results suggest
that CNP modifies cardiac ionic currents to produce positive
chronotropic and inotropic effects by stimulation of NPR-B receptors,
located in the SAN region, and that CNP plays a role in the modulation
of cardiac function.
sinoatrial node; natriuretic peptide receptors; cardiac
electrophysiology; inotropy
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INTRODUCTION |
THE NATRIURETIC PEPTIDE family is composed of atrial
natriuretic peptide (ANP), brain natriuretic peptide (BNP), and C-type natriuretic peptide (CNP). ANP and BNP are circulating peptides of
primarily cardiac origin and activate natriuretic peptide receptor (NPR)-A. CNP, isolated by Sudoh et al. in 1990, is present mainly in
the brain and vascular endothelium and appears to play a role in the
local regulation of vascular tone (9). The diuretic and natriuretic
effects of CNP are weak compared with those of ANP (10). It is actually
doubtful that CNP has any endocrine function, but cardiac paracrine and
autocrine actions have been proposed (10, 26). In support of these
possibilities, it was found that the genes coding for the NPR-B, for
which CNP is the natural ligand, are expressed in the rat heart, where
NPR-B mRNA was most abundant in the atria (15). Activation of NPR-B
receptors stimulates production of guanosine 3',5'-cyclic
monophosphate (cGMP), which is thought to mediate the biological
effects of CNP.
Boineau et al. (6) have put forth the concept of a widely distributed
atrial pacemaker complex, with dominant pacemaker shifts occurring in
response to sympathetic and parasympathetic nerve stimulation as well
as to adrenergic and cholinergic agonists. Dominant pacemaker shifts
could be related to differential nerve inputs to the atria as well as
to differential receptor densities between the sinoatrial node (SAN)
and other areas of the atrial pacemaker complex (3, 25). Recent
evidence suggests that peptides, especially neuropeptides, play a role
in heart rate regulation (4, 11, 14, 19, 22, 23). Calcitonin
gene-related peptide (11), vasoactive intestinal peptide (23), and
angiotensin II (ANG II) (14) produce positive chronotropic effects in
various animal preparations, whereas bradykinin (22) and endothelin-1 (19) exert negative chronotropic actions. The influence of peptides on
the dominant pacemaker location within the atrial pacemaker complex has
not been investigated.
We have recently reported that CNP causes direct sustained positive
chronotropic effects when injected into the SAN artery of canine
preparations, whereas ANP does not influence heart rate (4). These
effects of CNP were independent of changes in systemic arterial blood
pressure and of 
-adrenergic and muscarinic receptors. The present
study was conducted to further evaluate the effects of CNP on cardiac
functions as well as to investigate the possible mechanisms mediating
these effects in the dog. Our first goal was to map the dominant
pacemaker location during maximal positive chronotropic responses to
CNP injected into the SAN artery of in situ preparations compared with
dominant pacemaker shifts occurring in response to the -adrenergic
agonist isoproterenol and ANG II. Second, the presence of NPR-A and -B
mRNAs was evaluated in tissue samples collected from the SAN area and
from a trabecula located in a portion of the right atrium (lateral
wall) not involved in pacemaker activity. Third, we studied the effects
of CNP, injected into the SAN artery, on transmembrane action
potentials recorded from the SAN area in multicellular right atrial
preparations. Finally, the effects of CNP on atrial contractility were
also evaluated in in vitro preparations using constant drive to assess inotropic responses independent of the chronotropic effects.
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METHODS |
Atrial mapping.
A median sternotomy was performed on eight adult mongrel dogs
(20-30 kg), anesthetized with thiopental sodium (25 mg/kg iv) followed by 
-chloralose (15 mg · kg
1 · h1
iv) and heparinized (250 IU/kg iv followed by 1,000 IU/h) for the
purpose of direct atrial mapping. The SAN artery and both femoral
arteries and veins were cannulated. A fluid-filled cannula (PE-50) was
used to cannulate the SAN artery. These cannulations were followed by
bilateral cervical vagotomy and later blockade of -receptors
(propranolol, 1 mg/kg iv; Sigma, St. Louis, MO) to abolish
the baroreflex. Activation sequences of both atria were obtained from
192 unipolar recording electrodes made of stainless steel (75 µm) and
insulated with Teflon. These electrodes were fixed to five flexible
templates (silicone plaque) designed to fit the epicardium of the right
atrial free wall, the posteroinferior wall of the left atrium and
coronary sinus, the posterior aspect of the left atrium, the left
atrial free wall, and the interatrial band (20). The anatomic mapping
grid is shown in Fig. 1. The 192 unipolar
signals were simultaneously recorded along with an electrocardiogram.
Isochronal activation maps were constructed from the activation times
detected during a selected time window; the earliest excitation
detected was used as the time reference (t = 0). The mapping system used a
micro-VAX host computer (Digital Equipment) and custom-made software
(Cardiomap, Institut de Génie Biomédical, École
Polytechnique, Université de Montréal). Signals were
amplified by programmable-gain analog amplifiers, sampled at 1,000 Hz,
and converted to a 12-bit digital format.
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Fig. 1.
Anatomic grid for atrial epicardial mapping in which position of 5 flexible templates used is shown along with important vascular
structures.  , Position of 192 unipolar electrodes. RA, right atrium;
LA, left atrium; LA post, posterior aspect of left atrium (surrounded
by 4 pulmonary veins); LA cs, posteroinferior wall of left atrium and
coronary sinus; IAB, interatrial band; SVC, superior vena cava; IVC,
inferior vena cava; SAN art, sinoatrial node artery.
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After a 30-min period of stabilization after the surgical preparation,
the effects of isoproterenol (10 µg in 1 min; Sigma), injected into
the SAN artery, on computerized epicardial mapping of atrial activation
were explored. These were compared, after administration of
propranolol, with the effects of ANG II (5 µg in 1 min; Sigma) and
CNP (40 µg in 1 min; Peninsula Laboratories, Belmont, CA) injections.
The doses of isoproterenol, ANG II, and CNP used in this protocol were
chosen to produce an increase in heart rate of similar magnitude. Each
administration, by manual injection, of peptides or drug (each
dissolved in 1 ml of Tyrode solution) was preceded (5 min) by the
injection of Tyrode solution (1 ml) as control. An interval of at least
30 min was allowed between the injection of each pharmacological agent.
Cardiac NPR-A and -B mRNAs.
Total RNA (0.5 µg) was extracted from dog tissue samples located in
the lung (reference), right atrium (lateral wall), and SAN
(n = 2) by the acid-guanidinium
thiocyanate-phenol-chloroform method (8), and the quality of the
preparations was verified by gel electrophoresis. Preliminary
histochemical studies (cholinesterase staining using acetylthiocholine
as substrate) were performed to help identify the canine SAN region
near the junction between the superior vena cava and the right atrium.
Furthermore, the SAN tissue samples were taken from an area situated
between the two branches of the SAN artery as it bifurcates while
coursing along the atriocaval junction. The fibrous connective tissue
from the epicardial surface and the superficial layer from the
endocardial surface (including endocardial endothelium) were excised
while atrial and nodal tissue samples were obtained. However, despite these precautions, a contribution from nonmyocytic cell types, such as
endothelial cells and fibroblasts, cannot be excluded. RNA
concentrations were measured by ultraviolet spectrophotometry. NPR-A
and -B mRNA levels were measured by semiquantitative
reverse-transcription (RT) polymerase chain reaction (PCR) assay using
mutated NPR-A and -B fragments as internal standards. This method was
first designed for the quantification of NPR-A and -B mRNA levels in rat organs (12). In the present experiments, the same primers and
internal standards were used, since the NPR-A and -B receptors have not
been cloned and sequenced in the dog. From the high degree of homology
found between the sequences of human and rat NPRs, it was assumed that
the sequences of rat and dog were sufficiently homologous to proceed by
this way. For the quantification of NPR-B, the PCR conditions were
slightly modified to obtain optimal amplification of NPR-B mRNA from
dogs. The sequences of the internal standards differ from native NPR-A
or -B cDNAs by only two bases, introducing a new
EcoR I restriction site in the middle
of each sequence. Tissue RNA and a known amount of mutated cRNA were
mixed, reverse transcribed, and coamplified by PCR. PCR products were
digested by EcoR I and
electrophoresed on 1.5% agarose gel. The densities of the nondigested
and digested amplicons were quantified by PhosphorImager (Molecular
Dynamics). The levels of NPR-A and -B mRNAs in each organ were
expressed as a ratio to the corresponding standard. Multiple
determinations were made for each animal.
Electrophysiological study.
Six adult mongrel dogs of either sex (20-30 kg) were anesthetized
with thiopental sodium (25 mg/kg iv) and artificially ventilated with
room air. The heart was exposed through a left thoracotomy, and the
pericardium was opened. One minute after the injection of heparin
(1,000 IU in 1 ml) into the left ventricle, the heart was excised and
quickly immersed in cooled Tyrode solution. Right atrial preparations
consisting of the anterior free wall of the atrium, the right atrial
appendage, and the SAN and its artery were isolated and bathed in
Tyrode solution. Preparations were perfused through the SAN artery (6 ml/min) and superfused (20 ml/min) with Tyrode solution kept at 37.5 ± 0.5°C and gassed with a 95%
O2-5%
CO2 mixture (pH 7.4 ± 0.1).
The composition of the Tyrode solution used in all experiments was (in
mM) 128 NaCl, 4.7 KCl, 1.2 MgSO4,
20.1 NaHCO3, 0.5 NaH2PO4,
2.3 CaCl2, and 11.1 dextrose (all
from Sigma). Atrial preparations were fixed with the endocardium facing
upward.
After 1 h of stabilization, action potentials (sampled at 1,000 Hz)
were recorded using a conventional floating glass microelectrode filled
with 3 M KCl and suspended at the end of a spiraled chlorided silver
wire (0.25 mm) connected to a high-impedance preamplifier and
direct-current differential amplifier, an Ag/AgCl half-cell immersed in
the perfusion chamber being used as a reference electrode. The
intracellular electrograms were continuously displayed on an
oscilloscope to verify the stability of impalement. The recordings were
transferred to a data-acquisition system consisting of a microcomputer
equipped with an analog-to-digital converter card and a custom-made
software (21).
The location of the dominant pacemaker was determined by identifying
the earliest depolarizing cells within the SAN using two roving
extracellular bipolar electrodes. The first reference electrode was
positioned on the endocardial surface of the preparation where the SAN
region was located, and electrical activity was recorded and displayed
on a storage oscilloscope. A second mobile electrode was then used to
estimate the site that depolarized before the region beneath the
reference electrode. When this was accomplished, the second electrode
then became the reference electrode, and the first was used as an
exploring electrode trying to display an even earlier signal, and so
forth. We assumed that the electrode recording the earliest
depolarization was closest to the origin of pacemaker activity. From
there, a microelectrode was slowly advanced from the endocardial
surface recording action potentials from several cell layers until an
action potential displaying the characteristic morphology of a dominant
pacemaker was recorded. A typical pacemaker potential consisted of a
slow diastolic depolarization phase followed by a smooth transition to
the upstroke. Microelectrode recordings were from the same impalement
maintained (for at least 2.5 min) from basal conditions to the
development of maximal effects after bolus (2 min) injection of 25 µg
of CNP in 1 ml of Tyrode solution into the SAN artery.
The following parameters were computerized from the numeric data:
atrial cycle length (in ms), rate of diastolic depolarization (in
mV/s), takeoff potential (in mV), maximal rate of depolarization during
phase 0 (dV/dtmax
in mV/ms), action potential amplitude (in mV), action potential
duration at 50, 75, and 90% of repolarization (APD50,
APD75, and
APD90, respectively, in ms), and
maximal diastolic potential (in mV). The
dV/dtmax
was determined using a three-point derivative.
Atrial contractility.
Isolated right atrial preparations, obtained as described for the
electrophysiological study, were used
(n = 6). The superior part of the
atrial preparation (near crista terminalis) was connected to an
isometric force transducer (model FT03, Grass Instrument, Quincy, MA)
by a silk thread. Two pairs of bipolar silver electrodes were brought
into contact with the surface of the preparation. One pair was used to
record the atrial electrogram, from which atrial rate was derived. The
other pair was used to drive the preparation with suprathreshold
electrical stimuli (1.5 times diastolic threshold intensity) of 2-ms
duration generated by use of a stimulus isolation unit (model A385,
World Precision Instrument, Sarasota, FL) synchronized with a pulse
stimulator (model SD9, Grass Instrument). After determination of the
spontaneous atrial rate, the preparation was paced at a rate 20%
greater than basal rate to eliminate the influence of heart rate
changes on contractility measurements. Isometric tension was recorded
on a polygraph (model WI-641G, Nihon Kohden), and the atrial muscle was
stretched to a resting tension of 2 g. In each preparation, after a
30-min period of stabilization, Tyrode solution was first injected into the SAN artery as control (0.5 ml in 1 min) followed by the injection of CNP (25 µg in 0.5 ml of Tyrode in 1 min) to observe its inotropic effect.
All the experimental procedures were done in accordance with the
guidelines of the Canadian Council for Animal Care and monitored by an
Institutional Animal Care Committee.
Statistics.
Data are expressed as means ± SE. Comparison between groups in the
cardiac mapping, electrophysiological, and contractility studies was
made using Student's paired t-tests
or one-way analysis of variance with the Bonferroni correction for
multiple comparisons. The critical level of significance was set at
P 
0.05.
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RESULTS |
Atrial mapping.
The atrial activation sequences determined during sinus rhythm showed
that, typically, the impulse originated in the area supplied by the SAN
artery, as illustrated in Fig. 2, showing activation times at the recording sites carried by the right atrial electrode template. In all preparations, the impulse originating in the
vicinity of the SAN activated the right atrium along the pathway of the
crista terminalis as well as the left atrium along the pathway of the
interatrial band; the site of latest activation was localized near the
farthest edge of the left atrial free wall (70-ms isochrone, not shown,
to provide greater resolution in region of pacemaker complex).
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Fig. 2.
In situ right atrial mapping showing site of earliest extracellular
electrical activation before and after injection (1 min) into SAN
artery of drug and peptides dissolved in 1 ml of Tyrode.
A: control (Tyrode);
B: isoproterenol (10 µg);
C: ANG II (5 µg);
D: C-type natriuretic peptide (CNP, 40 µg). Time scale of activation is indicated in ms. Injection of
isoproterenol and ANG II (producing an increase in heart rate of 31 and
10 beats/min, respectively) shifted site of earliest activation to
superior region of SAN complex, whereas CNP (increase in heart rate of
10 beats/min) did not modify atrial activation patterns. PV, pulmonary
veins.
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Injection of Tyrode solution did not modify the atrial activation
pattern nor the location of the earliest activation (Fig. 2A). In contrast, isoproterenol
administration produced a shift of the site of earliest activation in a
superior direction (Fig. 2B): here,
the dominant pacemaker shifted four recording sites away, i.e., a
distance of 20 mm, from its location under basal conditions. Similar
shifts occurred in response to isoproterenol in all preparations and
were associated with a mean increase in heart rate of 33 ± 5 beats/min (from 114 ± 7 to 147 ± 9 beats/min) and with a change
in mean arterial pressure from 98 ± 5 to 89 ± 4 mmHg. After
recovery from the chronotropic response to isoproterenol and
-blockade, the site of earliest activation was the same as under
basal conditions before isoproterenol injection (as indicated in Fig.
2A). ANG II injection also produced
a shift of the site of earliest activation in a superior direction (to
same site as in response to isoproterenol) in five preparations (Fig.
2C), in which the positive
chronotropic responses ranged from 7 to 29 beats/min. In two other
preparations, the activation pattern was not modified by ANG II despite
chronotropic responses of 12 and 16 beats/min, respectively. In one
preparation, the site of earliest activation was shifted a single
electrode away in the inferior direction in association with a
chronotropic response of 13 beats/min. ANG II injections produced a
mean increase in heart rate of 16 ± 3 beats/min (from 94 ± 2 to
110 ± 3 beats/min) and an increase in mean arterial pressure from
89 ± 4 to 115 ± 6 mmHg. The effects of ANG II on heart rate
were reversible in 2-3 min, as previously reported (14), and the
site of earliest activation also shifted back to the same location as
under basal conditions. In response to CNP injection producing a mean
increase in heart rate of 11 ± 2 beats/min (from 94 ± 2 to 105 ± 3 beats/min) and a decrease in mean arterial pressure from 90 ± 4 to 85 ± 4 mmHg, the site of earliest activation remained
the same as under basal conditions in five dogs (Fig.
2D), in which the chronotropic responses ranged between 3 and 13 beats/min. The site of earliest activation shifted four and five electrode sites away in the inferior direction in two preparations showing chronotropic responses of 13 and
19 beats/min, respectively, and in the superior direction (7 beats/min)
in the other preparation (to same location as in response to
isoproterenol).
Cardiac NPR-A and -B mRNAs.
NPR-A and -B mRNA levels were determined in atrial and nodal tissue
samples of two animals and compared with lung tissues known to express
both types of receptors (Fig. 3). The
levels of both receptors were expressed as a ratio to a known
concentration of corresponding internal standard (5 × 106 mutated NPR-A cRNA and 5 × 107 mutated NPR-B cRNA)
for an equal amount of total RNA (0.5 µg) extracted from each tissue
sample. Because of potential differences in PCR amplification between
dog tissue and rat standards, comparisons were made between the three
tissues for the same receptor subtype but not between the two receptor
subtypes. Both atrial and nodal tissues showed high expression of NPR-B
receptors compared with lung (reference) tissue. For the NPR-A
receptor, mRNA levels appeared higher in nodal than in atrial tissue,
but these levels appeared lower than in the lung.
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Fig. 3.
Natriuretic peptide receptor (NPR)-A (A) and -B
(B) mRNA levels measured by semiquantitative
reverse-transcription polymerase chain reaction (PCR). An aliquot of
0.5 µg of total RNA and 5 × 106 molecules of mutated NPR-A
cRNA or 5 × 107 molecules of
mutated NPR-B cRNA were mixed, reverse transcribed, and coamplified by
PCR. PCR products were digested by
EcoR I to cut standard and
electrophoresed on 1.5% agarose gel. After quantification of 2 bands
(endogenous RNA and mutated cRNA), levels of NPR-A and -B mRNAs in each
organ were expressed as a ratio to corresponding standard.
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Electrophysiological study.
Transmembrane action potentials displaying the typical features of
dominant cardiac pacemaker cells, with a smooth transition between
phase 4 and the action potential upstroke, were recorded in all six
isolated right atrial preparations. Figure
4A shows the configuration of such action potentials recorded before CNP injection into the SAN artery, and Fig. 4,
B and
C, depicts spontaneous action
potentials recorded from the same nodal cell during and after the
injection of CNP. The injection of CNP produced an increase in atrial
rate (i.e., decrease in cycle length) and significantly modified some
variables of the SAN action potentials as presented in Table
1. Specifically, CNP significantly
increased the rate of diastolic depolarization and
dV/dtmax
and significantly decreased the cycle length,
APD75, and
APD90. The takeoff potential,
action potential amplitude, and maximal diastolic potential remained unchanged. Whether the significant reduction in action potential duration might have been caused by the increase in rate alone and/or by a direct effect of CNP was not determined, since the action potentials were not recorded during constant drive.
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Fig. 4.
Typical sinoatrial action potentials recorded, using a floating glass
microelectrode, in same nodal cell before and after injection into
SAN artery of CNP (25 µg in 2 min) dissolved in 1 ml of
Tyrode. A: basal heart rate (86 beats/min); B: end of CNP injection
(99 beats/min); C: maximal
effect 30 s after end of CNP injection (103 beats/min).
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Table 1.
Effects of CNP injected into sinoatrial node artery of canine isolated,
spontaneously beating right atrial preparations on action potentials of
sinoatrial node cells recorded by floating glass microelectrodes
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Atrial contractility.
The injection of CNP directly into the SAN artery of six isolated right
atrial preparations, during pacing at a rate 20% greater than the
spontaneous beating rate, induced a positive inotropic effect with a
significant increase in contractile force from 0.9 ± 0.3 to 1.7 ± 0.6 g (Fig. 5). This inotropic
effect was maximal 76 ± 13 s after the beginning of CNP injections
and lasted for 326 ± 12 s before complete return to baseline
values. The spontaneous rate during CNP injections never exceeded the
pacing rate in any of the preparations.
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Fig. 5.
Contractile force recorded, using an isometric transducer, from an
isolated RA preparation paced at 120 beats/min before and after
injection into SAN artery of CNP (25 µg in 1 min) dissolved in 0.5 ml
of Tyrode.
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DISCUSSION |
Traditionally, autonomic cardiac control has been attributed solely to
adrenergic and cholinergic neurotransmitters. However, there is
accumulating evidence that neuropeptides within the cardiovascular system function as hormones, transmitters acting via their own receptors, neuromodulators influencing the release and/or the action of classic or other transmitters, and trophic agents (23, 29).
These peptides can be localized as follows:
1) within autonomic efferents or
sensory neurons innervating the heart (coexistence of peptides with
classic neurotransmitters is now well established and indeed chemical
coding of neurons for a particular peptide may reflect its
participation in a well-defined physiological event);
2) in vascular cells [intimate
contact between endothelial cells and cardiac myocytes, with no
cardiomyocytes being >2-3 µm from a coronary vascular
endothelial cell (26), certainly makes paracrine interactions between
these two types of cells highly plausible]; and
3) in endocardial endothelial cells.
It is now recognized that the endocardial endothelium regulates the performance of underlying cardiac muscle by the release of various factors (17). Among the factors released by endothelial cells, numerous
endogenous substances, such as nitric oxide, calcitonin gene-related
peptide, substance P, vasoactive intestinal peptide, ANG II,
bradykinin, endothelin-1, prostaglandins, adenyl purines, neuropeptide
Y, somatostatin, enkephalin, neurotensin, and neurokinins have been
shown to modulate cardiac functions and, in particular, sinoatrial
activity (4, 11, 14, 17, 19, 22, 23, 26, 29). Results reported herein
as well as in a previous study (4) provide evidence that CNP, which is
not currently considered as a cardiac peptide, might be involved in the
modulation of cardiac functions through positive chronotropic and
inotropic responses, contrasting with ANP.
The site of earliest extracellular electrical activation is known to
shift in response to autonomic stimuli: with infusion of acetylcholine,
it shifts mainly inferiorly, whereas with infusion of norepinephrine,
it consistently shifts to the superior region of the SAN (25). The
mechanisms underlying this phenomenon as well as the determinants of
the location of dominant pacemaker activity have not been elucidated.
However, Boineau et al. (5) reported that, in the case of
-adrenergic stimulation, the distance of the shift is proportional
to the intensity of the chronotropic response. Moreover, Beau et al.
(3) have recently suggested that regional variations in receptor
density are related to differential responsiveness to autonomic stimuli
and may help to determine the spatial localization of pacemaker
activity. In agreement with the results of others, we showed that
isoproterenol infusion into the SAN artery shifted the dominant
pacemaker from a midlevel position between the venae cavae toward the
superior vena cava in all experiments. Such shifts were obtained in
association with substantial chronotropic responses (33 ± 5 beats/min), which were the smallest that we could achieve in response
to isoproterenol under our experimental conditions. In the same
experiments, the pacemaker location remained constant, at the level of
resolution afforded by our electrode array during maximal responses to
CNP (11 ± 2 beats/min). The question then arises whether the
absence of a shift might reflect an intrinsic property of CNP or might have been related to the relatively weak chronotropic responses to CNP.
ANG II was studied at doses meant to produce responses of a similar
magnitude to those to CNP. In most of the preparations, ANG II infusion
produced a pacemaker displacement in the superior direction, an action
associated with a positive chronotropic effect. Therefore, the fact
that chronotropic responses to ANG II of a similar magnitude are
associated with upward shifts of the dominant pacemaker, whereas those
to CNP are not, is in agreement with the hypothesis that the actions of
CNP are more localized to the dominant SAN. This hypothesis is further
supported by the fact that transmembrane potentials showing the typical
characteristics of pacemaker cells under basal conditions still
presented such characteristics at the same location during the
chronotropic response to CNP in the isolated atrial preparations.
However, the earliest activation site did shift in response to CNP or
ANG II injections in three of eight dogs. Two of the three dogs for
which a shift occurred in response to CNP or did not occur in response
to ANG II were actually the same dogs. Why these two dogs gave
different results from the others is unclear but possibly they were
"atypical." Therefore, the shift of the dominant pacemaker in
response to substances producing positive chronotropic effect seems
highly variable and may underline differences among the various
substrates in their respective receptor density. Unlike what is found
with isoproterenol and ANG II, when latent pacemakers appear more
sensitive than the primary one, our results suggest that, in most dogs
investigated in the present study, the SAN is functionally homogeneous
with respect to its response to CNP or that a greater density of
receptors for CNP is present in the lower SAN area, which is the
dominant pacemaker in the baseline condition.
Specific cardiac binding sites for natriuretic peptides have been
detected by ligand binding studies and autoradiography (7). The
presence of NPR-B mRNA transcripts has been clearly shown in the monkey
heart using in situ hybridization (30) as well as in rodent and human
cardiac tissues using cDNA amplification with RT-PCR (18). Furthermore,
Lin et al. (15), using Northern blot analysis for specific detection
and quantification of all three NPR subtypes in the rat heart, have
reported that NPR-B mRNA was most abundant in the atria. These authors,
using a combination of cell isolation and RT-PCR, also demonstrated
that NPR-B mRNA was retrieved in cardiomyocytes as well as in
fibroblasts. Using RT-PCR, we have shown that NPR-A and -B mRNAs are
both present in atrial and nodal tissues. If these mRNA transcripts are
translated into functional receptors in the dog heart, our results
suggest that natriuretic peptides exert direct effects on cardiac
functions via their own receptors.
The mechanisms underlying the actions of CNP on the atrium and the SAN
are still not known. In the SAN, at least three currents have been
implicated in pacemaker activity. First, a decrease in the delayed
rectifier potassium current seems to be predominantly responsible for
the first half of the spontaneous depolarization phase of sinoatrial
pacemaker cells (13). The second half is mainly caused by calcium
currents, which become activated at about 
60 to 50 mV.
The transient T-type calcium channel is responsible for the early phase
of the second half of slow diastolic depolarization, whereas
long-lasting L-type calcium channel is involved in the latter phase.
Third, an inward current appears to play a role especially at higher
diastolic membrane potentials. The positive chronotropic responses to
CNP reported herein were associated with an increase in the slope of
the spontaneous diastolic depolarization, and the
dV/dtmax
of action potentials recorded from the SAN region using conventional
floating microelectrodes was increased. Augmentation of contractile
activity was also elicited in response to CNP in the right atrial
preparations. Taken together, these findings suggest that CNP enhances
calcium currents activity in the heart atrium, but the use of specific
calcium channel blockers is needed to confirm this hypothesis.
Classically, activation of NPR-B receptors stimulates the production of
cGMP. Paradoxically, an increase in cGMP is usually associated with
negative inotropic or chronotropic effects (27) as well as with the
inhibition of calcium channels via the activation of protein kinase G
(24). On the other hand, cGMP analogs have been reported by some
investigators to produce a positive inotropic effect (16). To explain
the controversial effects that were noted, Fabiato (personal
communication quoted in Ref. 16) suggested that cGMP has a biphasic
effect: inhibition at supraphysiological levels and enhancement of
contractility at more physiological levels (<1 µM). This hypothesis
was recently confirmed by a study from Mohan et al. (17), demonstrating
that, in papillary muscle of cat, intracellular cGMP causes a
concentration-dependent biphasic contractile response. If this is the
case and if CNP positive chronotropic and inotropic effects are via
stimulation of NPR-B receptors and cGMP production, we can then assume
that the doses of CNP used in this study were within physiological
range.
Finally, CNP has been shown to act through mechanisms other than the
production of cGMP. It is therefore possible that some of its
biological actions are not mediated by a direct coupling to guanylate
cyclase receptors. Among other alternatives, it has been reported that
CNP 1) causes relaxation of isolated
porcine coronary arterial rings through activation of potassium
channels and membrane hyperpolarization (28),
2) causes relaxation of canine
femoral veins by activation of large-conductance calcium-activated potassium channels (2), and 3)
dilates the afferent renal arterioles via the prostaglandin-nitric
oxide pathway (1). Thus, although stimulation of NPR-B receptors
located in the SAN and right atrium might explain the effects of CNP
reported in this study, since it also acts via other mechanisms,
further studies, including voltage-clamp techniques, are obviously
necessary to definitely elucidate this matter.
In conclusion, we have shown that CNP positively modulates pacemaker
activity when injected into the canine SAN artery and increases the
contractile force of the right atrium. Furthermore, if variations of
the dominant pacemaker location in response to substances producing
positive chronotropic effects are related to differences in receptor
density, the results presented herein indicate that the primary SAN
pacemaker is more sensitive to CNP, whereas subsidiary pacemakers are
more sensitive to isoproterenol and ANG II. We suggest that these
positive chronotropic and inotropic effects of CNP are the results of
an increase in cardiac calcium channel activity and that NPR-B
receptors present in right atrial and nodal tissues mediate these
actions. Other studies are needed to clarify the signaling pathway and
the currents involved in the responses to CNP as well as their
physiological significance. In addition to the classical
neurotransmitters, peptidergic transmitters are clearly present in the
cardiovascular system and have been shown to exert direct and indirect
actions on cardiac functions that may have both diagnostic and
therapeutic implications in humans. These new concepts of
cotransmission, neuromodulation, and "cross-talk" show that there
is remarkable degree of interaction between the autonomic nervous
system and neuropeptides at a specific target organ.
| |
ACKNOWLEDGEMENTS |
The authors thank Michel Vermeulen for advice in the realization of
electrophysiological experiments, Martin Laflamme for excellent
technical assistance, and Elisabeth Pérès for the artwork.
| |
FOOTNOTES |
This work was supported by grants to René Cardinal and Johanne
Tremblay from the Medical Research Council of Canada (MA-11688 and
MT-11463, respectively). P. Beaulieu holds a fellowship from the Fonds
de la Recherche en Santé du Québec and received a grant
from the Faculté des Études Supérieures,
Faculté de Médecine, Université de Montréal.
Address for reprint requests: C. Lambert, Dept. of Pharmacology,
Faculty of Medicine, Université de Montréal, CP 6128, Succursale, Centre-Ville, Montreal, Quebec, Canada H3C 3J7.
Received 6 February 1997; accepted in final form 28 May 1997.
| |
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Abstract
Introduction
