Function of human intrinsic cardiac neurons in situ

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Function of human intrinsic cardiac neurons in situ

Rakesh Christopher Arora¹, Gregory Matthew Hirsch¹, Kristine Johnson Hirsch², Camille Hancock Friesen¹, and John Andrew Armour³

Departments of ¹ Surgery, ² Anesthesiology, and ³ Physiology and Biophysics, Dalhousie University, Halifax, Nova Scotia, B3H 4H7, Canada

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We sought to determine the behavior of intrinsic cardiac neurons in human subjects undergoing cardiac surgery and to correlatetheir activity with hemodynamics status. A lead II electrocardiogram,pulmonary artery pressure, and systemic arterial pressure wererecorded along with extracellular activity generated by rightatrial neurons in 10 patients undergoing coronary artery bypasssurgery. Identified neurons generated spontaneously activity thatwas, for the most part, unrelated to the cardiac cycle. Most neuronswere activated by gentle mechanical distortion of ventricularepicardial loci. The activity generated by neurons in each patientincreased when arterial pressure increased and decreased whenarterial pressure fell. Intrinsic cardiac neurons continued togenerate activity during cardioplegia and cardiopulmonary bypass,but at reduced levels. Normal neuronal activity was restored postbypass.It is concluded that human intrinsic cardiac neurons generatespontaneous activity and that many receive inputs from ventricularmechanosensory neurites. The latter may account for the fact thattheir behavior depends, in part, on cardiac dynamics. They arealso sensitive to intravenously administered pharmacological agents.These data also indicate that cardiopulmonary bypass and cardioplegiado not induce residual depression of theirfunction.

$alpha$ -adrenoceptor agonist; cardiac mechanosensory neurites; cardioplegia; cardiopulmonary bypass

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

MULTIPLE NEURONAL SUBTYPES have been identified within the mammalian intrinsic cardiac nervous system, both anatomically (4,6, 8, 10) and functionally (1, 2). It has been proposedthat the intrinsic cardiac nervous system is important for themaintenance of adequate cardiac output (11), particularly indisease states such as myocardial ischemia (2). Canine intrinsiccardiac neurons display complex behavioral patterns that rely,to a considerable degree, on their cardiovascular sensory inputs.These inputs, in turn, are dependent on cardiovascular status(1, 2). It is known that the human cardiac efferent nervoussystem displays functional characteristics similar to those foundin animals (5, 9). It remains to be established whetherneurons in the human heart behave in a manner similar to thatidentified in animal models. Furthermore, we do not know whateffects cardiopulmonary bypass (CPB) and cardioplegia have onthe human intrinsic cardiac nervoussystem.

The present experiments were designed to determine whether human intrinsic cardiac neurons generate spontaneous activity and,if so, how they respond to altered cardiovascular status. Additionally,we sought to determine whether cardiac afferent inputs to thehuman intrinsic cardiac nervous system alter its behavior. Finally,we sought to determine whether CPB and cardioplegia exert deleteriouseffects on human intrinsic cardiac neuronalfunction.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

General methods. Ethical approval for human experimentation at our institution is reached through a clinical and layperson peer-reviewed processat the Queen Elizabeth II Hospital, Halifax, Nova Scotia, Canada.Once full ethical approval of the study was achieved, patientswere approached for entry into the study in accordance with guidelinesset forth by the Queen Elizabeth II Hospital Ethics Committee.To qualify for entry into this study, a patient needed to haveangiographic evidence of a lesion in at least one major coronaryartery that required the coronary artery bypass grafting (CABG)procedure (Table 1). Patients were excluded from this study ifthey had depressed left ventricular function, required anotherprocedure combined with the CABG procedure, or refused to consentto the recording procedure. Ten patients scheduled for CABG proceduresentered this study. Basic demographic data and comorbid variableswere collected from each patient upon entry into the study. Leftventricular ejection fractions were determined in each patientby means of transthoracic or transesophageal echocardiography,radionucleotide imaging, or left ventriculography performed attime of selective coronary catheterization. Operative variablesrelating to pump and aortic cross- clamp times, times to extubationpostprocedure, as well as intensive care unit and total lengthof stay were assessed for each patient.

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Table 1. Tabulated data on patients' age, sex, diseased vessel territories, and risk factors

Operative procedures. After instigation of general anesthesia, a midline sternotomy was performed to expose the heart, and the appropriate bypassconduit was harvested in the usual fashion for CABG. Once thepericardotomy was completed, baseline systemic and pulmonary arterypressures were recorded along with a two-lead (leads II and V₅)electrocardiogram (ECG). Patients were heparinized and underwentaorto-right atriocaval cannulation in case CPB compromised hemodynamics,so that CPB could be instigatedimmediately.

Recording neuronal activity. Fatty tissue on the lateral surface of the right atrium that contains the right atrial ganglionated plexus (RAGP) (4, 6,10) was exposed. A tungsten recording microelectrode was employedto record the extracellular activity generated by right atrialneurons (7). The microelectrode had a shank diameter of 100µm, an exposed tip of 5 µm, and an impedance of 9-11 M $Omega$ at 1,000Hz. The electrode was held in place by a micromanipulator attachedto a variable extension arm (Octopus 1; Medtronic, Minneapolis,MN) to stabilize itsmotion.

The fat on the lateral surface of the right atrium was explored with this microelectrode from its epicardial surface and moredeeply to adjacent atrial tissue. An indifferent electrode wasattached to the adjacent mediastinum. The RAGP was chosen forinvestigation because it contains one of the largest collectionsof intrinsic cardiac neurons without an associated large coronaryartery (4). Thus we could explore it with an electrode withoutpotentially injuring a major coronary artery. The midline sternotomypermitted easy access to this plexus and thereby minimized stimulationof mechanosensory nerve endings located in the epicardium thatcould confound neuronal activityresults.

The activity generated by right atrial neurons so recorded was amplified differentially by means of two Princeton AppliedResearch (model 113) amplifiers that had band-pass filters setat 300 Hz to 10 kHz and amplification ranges of 100-500×, placedin series. The output of these battery-driven amplifiers was ledto an audio monitor as well as an Astromed MT9500 eight-channelrectilinear chart recorder. Action potentials generated by individualneurons with signal-to-noise ratios greater than 3:1 were studied,with individual neural units being identified by the amplitudeand configuration of their action potentials. Gradually movingthe electrode away from an active site reduced the amplitude ofrecorded action potentials without altering their configurations.Action potentials generated by adjacent axons of passage are ofsimilar magnitude as the background noise. Therefore, with thesetechniques and criteria, the recording microelectrode identifiesaction potentials generated by neuronal somata (cell bodies) and/ordendrites.

Intraoperative procedures. Once an active site was identified, various loci on the exposed epicardial surfaces of the right and left ventricles weretouched gently. The epicardial mechanical stimuli so applied wereinsufficient to distort the heart and thus alter the positionof the recording electrode tip. This procedure was performed todetermine whether identified RAGP neurons received mechanosensoryinputs from such epicardial regions. Then systemic arterial pressurewas reduced or increased by ~30% after administration of nitroglycerin(50-100 µg iv boluses) or phenylephrine (50-100 µg iv boluses),respectively.

Neuronal activity and cardiovascular variables were also monitored during the following interventions: 1) just before instigatingtotal CPB, 2) when the patient was on full CPB before the aorticcross clamp was applied, 3) during cardioplegia as ECG quiescenceoccurred, and 4) at the end of the initial cardioplegia infusionbefore starting the first distal coronary artery anastomosis.A combination of cold blood and crystalloid (4:1 ratio) is employedfor cardioplegia at our institution during CPB. Once the coronaryrevascularization procedures had been completed, neuronal activityand cardiovascular variables were monitored as CPB was discontinued.Lastly, variables were monitored during the subsequent administrationof protamine hydrochloride in 0.9 sodium chloride (150-250 mgiv). This agent is routinely employed after completion of theCABG procedure to reverse the effects of the previously administeredheparin. Protamine was administered over 10- to 15-min periods.Monitored hemodynamic variables were unaffected by thisintervention.

Data analysis. Cardiac variables were analyzed over 30-s periods of time before and during peak responses elicited by each of the interventionsdescribed above. Action potentials with signal-to-noise ratiosgreater than 3:1 generated within a locus of the RAGP were countedfor 30-s periods of time to establish average activity immediatelybefore and during maximal responses elicited by each intervention.Fluctuations in the amplitude of action potentials generated byindividual neurons varied by <25 µV over several minutes, retainingtheir same configurations over time. Action potentials recordedin a given locus with the same configuration and amplitude wereconsidered to be generated by the somata and/or dendrites of asingle neuron. The means (± SE) of data recorded during controlstates as well as during each intervention were calculated. ANOVAand paired t-test with Bonferroni correction for multiple testswere employed for statistical analysis where appropriate. A significancevalue of P < 0.01 was used for thesedeterminations.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Patient and operative variables. Patient demographics, comorbid variables, and medications are listed in Table 1. The average age of patients was 62 yr, with80% of the patients being male. All patients had preserved leftventricular function. All but one patient received at least twografts that consisted of a left internal mammary artery to theleft anterior descending artery and either a radial artery and/ora reversed saphenous vein graft to the remaining diseased territories.Two patients were classified as "in-house" urgent cases, havingbeen in the coronary care unit awaiting the CABG procedure. Therewere no complications arising from the intraoperative recordingprocedure. No in-hospital deaths occurred in this cohort of patients.The majority of patients was extubated within 4-7 h postoperatively.Both in-house urgent patients had prolonged hospital stays (17and 18 days). One of these urgent patients developed left lowerlobe pneumonia postoperatively. The other patient had low cardiacoutput postoperatively requiring low doses of dopamine and epinephrinefor 24 h. The rest of the patients had uncomplicatedrecoveries.

Neuronal activity. Using the criteria mentioned above, we identified spontaneous activity generated by two to three intrinsic cardiac neuronsin each patient before any intervention. Multiple neuronal activitywas evidenced by the different amplitudes of their recorded actionpotentials (Fig. 1; Table 2). The configuration and amplitudeof each identified neuronal unit did not vary over time, allowingfor comparison of changes in neuronal activity before and afteran intervention. The activity so identified was sporadic in natureand, for the most part, not related to a specific phase of thecardiac cycle (Fig. 1). Immediately before the CPB, the activitygenerated by right atrial neurons in anesthetized patients averaged59 ± 11 impulses per minute. At that time, these patients' systemicarterial pressure was, on average, 90/56 mmHg (Table 2).

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Fig. 1. Continuous recording of the activity generated by right atrial neurons and cardiovascular indexes obtained before and after administering a bolus dose of phenylephrine into the circulation (arrow, bottom). Neuronal activity increased soon after this occurred and before any change in recorded cardiovascular variables was detected (note that a paper fold prevented recording partway through the record). ECG, electrocardiogram; AP, aortic pressure; PAP, pulmonary pressure (the same abbreviations are used in the other figures).

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Table 2. Alterations in heart rate, pulmonary artery pressure, and aortic pressure, as well as activity generated by right atrial neurons recorded during various interventions

The activity generated by identified, spontaneously active neurons increased in seven of the 10 patients when limited locion the exposed anterior epicardium of the right or left ventricleswere touched gently (Table 2). No responses were elicited inthe other three patients when the exposed surfaces of the twoventricles were touched. In six of these seven patients, additionalneurons were recruited when mechanical stimuli were applied tothe epicardium, as determined by the varied configurations ofthe action potentials identified (Fig. 2).

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Fig. 2. Neuronal responses elicited by a gentle touch of a locus on the left ventricular ventral epicardium (horizontal line below). A burst of activity was generated by right atrial neurons (neural, bottom) during application of this stimulus. Monitored cardiovascular variables remained unchanged.

When systemic arterial pressure increased after systemic administration of the $alpha$ -adrenoceptor agonist phenylephrine, intrinsiccardiac neuronal activity increased (Fig. 1; Table 2). This includedthe recruitment of new neuronal units with different amplitudesthan identified during baseline conditions (before phenylephrineadministration). In some instances, the activity generated byright atrial neurons increased before any detectable changes inmonitored cardiovascular variables became evident (Fig. 1). Incontrast, when systemic arterial pressure was reduced by the systemicadministration of nitroglycerin, intrinsic cardiac neuronal activitydecreased (Table 2).

The activity generated by intrinsic cardiac neurons remained at control levels (57.4 ± 18.4 impulses per minute) upon instigationof CPB before the application of the aortic cross clamp and infusionof cardioplegia. Intrinsic cardiac neurons continued to generateactivity (41.1 ± 28.6 impulses per minute) during infusion ofthe cardioplegia solution (Fig. 3B). Neuronal activity persistedwhen the ECG became quiescent, but at a reduced level. For instance,during a period of prolonged cardiac standstill after the initialcardioplegia period, right atrial neurons generated 21.0 ± 12.1impulses per minute (P < 0.01, compared with control values; Fig.3C). After completing the CABGs and weaning the patient from CPB,neurons generated activity levels that were similar to those recordedbefore these interventions were instigated (Table 2). At theend of the procedure, protamine hydrochloride was administeredinto the systemic circulation to reverse the effects of previouslyadministered heparin. When neuronal activity was monitored infour patients during this intervention, we observed that thispeptide enhanced the activity generated by some neurons whileactivating previously quiescent neurons in other instances (Fig.4). This occurred without any alterations in monitored cardiovascularvariables being detected. No untoward reactions were elicitedafter protamine administration.

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Fig. 3. A and B represent a continuous record of the ECG, AP, and right atrial neuronal activity obtained from the beginning of infusing cardioplegia solution until the point of ECG quiescence. Note that neuronal activity persisted in the presence of suppressed cardiac electrical activity (B). C: data obtained after cardioplegia infusion had been instituted for some time, just before the first distal anastomosis was performed.

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Fig. 4. A burst of activity was generated by right atrial neurons soon after the administration of protamine into the circulation commenced (arrow, bottom). Recorded cardiovascular indexes remained unchanged.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The results obtained in these experiments demonstrate that populations of human intrinsic cardiac neurons generate spontaneousactivity in patients undergoing cardiac surgery after anesthesiais induced and a midline sternotomy is performed. These data supportthose derived from the canine model (7) in as much as, first,the activity generated by right atrial neurons was for the mostpart sporadic in nature and thus unrelated to the cardiac cycle(Fig. 1). Second, as has been found in experimental animals, populationsof human intrinsic cardiac neurons receive inputs from ventricularmechanosensory neurites. Third, cardioplegia or CPB proceduresdo not appear to reduce the capacity of human intrinsic cardiacneurons to generate spontaneous activity after their discontinuance(Table 2). Fourth, the activity generated by human intrinsiccardiac neurons is dependent, in part, on cardiodynamicstatus.

Right atrial neurons were activated in most patients when limited loci on the ventral epicardial surfaces of either ventriclewere touched briefly (Fig. 2). Presumably, not all investigatedneurons responded to this intervention (Table 2) because notall of them received mechanosensory inputs from the epicardialareas investigated with local mechanical stimuli, as occurs inanimal models (2, 7). The fact that human intrinsic cardiacneurons receive cardiac mechanosensory inputs may explain, inpart, the fact that the activity generated by many identifiedright atrial neurons changed in concordance with alterations incardiovascular status (Fig. 1). For instance, when systemic arterialpressure increased as a consequence of the administration of phenylephrine(representing an increase in afterload), neuronal activity increased.Likewise, when systemic arterial pressure decreased after systemicadministration of nitroglycerin (representing a reduction in afterloadand preload), neuronal activity decreased. These data supportthose derived from the canine model, in as much as animal intrinsiccardiac neurons are known to receive direct inputs from ventricularmechanosensory neurites and thus are sensitive to changing cardiodynamics(2, 7). In accord with that, most identified neurons becameinactive when systemic arterial pressure fell below 60 mmHg. Presumably,that was primarily due to a relative reduction of cardiac mechanosensoryinputs to the intrinsic cardiac nervous system. This agrees withthe fact that neuronal activity was lowest during cardiac standstillwhen the ECG wasquiescent.

Administering the $alpha$ -adrenergic agonist phenylephrine increased right atrial neuronal activity concomitant with increases insystemic arterial pressure (Table 2). These neuronal responsesaccompanied changes in monitored cardiovascular indexes, presumablyreflecting increased sensory inputs as well as increasing inputsarising from central reflexes as a result of global changes incardiovascular status. In some patients, activation of right atrialneurons occurred even before any detectable changes in monitoredcardiovascular indexes became evident (Fig. 1). Populations ofcanine intrinsic cardiac neurons are known to be sensitive toexogenous applied $alpha$ -adrenoceptor agonists (3). Thus $alpha$ -adrenoceptoragonists may directly affect some human intrinsic cardiac neurons.Human intrinsic cardiac neurons also proved to be sensitive toprotamine (Fig. 4). The fact that some atrial neurons were modifiedby this peptide is in accord with the fact that canine intrinsiccardiac neurons are sensitive to multiple chemicals, includingpeptides and amino acids (2).

Because intrinsic cardiac neuronal activity was restored to baseline values by the end of bypass (Table 2), cardioplegiaand CPB do not appear to adversely affect the capacity of humanintrinsic cardiac neurons to generate spontaneous activity. Wehave proposed that proper functioning of the final common regulatorof cardiac behavior, the intrinsic cardiac nervous system, maybe important in the maintenance of adequate cardiac output (11).This aspect of the human intrinsic cardiac nervous system maybe relevant with respect to modifying cardiac function in theperioperativeperiod.

Perspectives

Human intrinsic cardiac neurons generate spontaneous activity, as is found in animal models. Furthermore, as in the caninemodel, human intrinsic cardiac neuronal activity is dependenton cardiovascular status. Exogenously administered therapeuticagents can also modify the neurons' behavior. These data providea basis for the development of novel therapy targeting the humanintrinsic cardiac nervous system in the perioperative period.The fact that intrinsic cardiac neurons retain their functionafter CPB implies that the human intrinsic cardiac nervous systemcan be manipulated to advantage in the postoperativeperiod.

	ACKNOWLEDGEMENTS

The authors gratefully acknowledge the technical assistance of R.Livingston.

	FOOTNOTES

This work was supported by the Medical Research Council of Canada (MA-10122), the Nova Scotia Heart and Stroke Foundation,and the Queen Elizabeth IIFoundation.

Address for reprint requests and other correspondence: J. A. Armour, Dept. of Physiology and Biophysics, Dalhousie Univ.,Halifax, Nova Scotia, B3H 4H7, Canada (E-mail: jarmour{at}is.dal.ca).

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate thisfact.

Received 29 November 2000; accepted in final form 9 February 2001.

	REFERENCES

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

1. Ardell, JL. Anatomy and function of mammalian intrinsic cardiac neurons. In: Neurocardiology, edited by Armour JA, and Ardell JL.. New York: Oxford University Press, 1994, p. 95-114.

2. Armour, JA. Anatomy and function of the intrathoracic neurons regulating the mammalian heart. In: Reflex Control of the Circulation, edited by Zucker IH, and Gilmore JP.. Boca Raton, FL: CRC, 1991, p. 1-37.

3. Armour, JA. Intrinsic canine cardiac neurons involved in cardiac regulation possess $alpha$ ₁-, $alpha$ ₂-, $beta$ ₁- and $beta$ ₂-adrenoceptors. Can J Cardiol 13: 277-284, 1997[Web of Science][Medline].

4. Armour, JA, Murphy DA, Yuan BX, MacDonald S, and Hopkins DA. Anatomy of the human intrinsic cardiac nervous system. Anat Rec 297: 289-298, 1997.

5. Carlson, MD, Geha AS, Hsu J, Martin J, Levy MN, Jacobs G, and Waldo AL. Selective stimulation of parasympathetic nerve fibers to the human sinoatrial node. Circulation 85: 1311-1317, 1992[Abstract/Free Full Text].

6. Davies, F, Francis ETB, and King TS. Neurological studies on the cardiac ventricles of mammals. J Anat 86: 302-309, 1952.

7. Gagliardi, M, Randall WC, Bieger D, Wurster RD, Hopkins DA, and Armour JA. Activity of in vivo canine cardiac plexus neurons. Am J Physiol Heart Circ Physiol 255: H789-H800, 1988[Abstract/Free Full Text].

8. King, TS, and Coakley JB. The intrinsic nerve cells of the cardiac atria of mammals and man. J Anat 92: 353-376, 1958.

9. Murphy, DA, Johnstone DE, and Armour JA. Preliminary observations on the effects of stimulation of cardiac nerves in man. Can J Physiol Pharmacol 63: 649-655, 1985[Web of Science][Medline].

10. Singh, S, Johnson PI, Lee RE, Orfei E, Lonchyna VA, Sullivan HJ, Montoya A, Tran H, Wehrmacher WH, and Wurster RD. Topography of cardiac ganglia in the adult human heart. J Thorac Cardiovasc Surg 112: 943-953, 1996[Abstract/Free Full Text].

11. Stevenson, RS, Thompson GW, Wilkinson M, Murphy DA, and Armour JA. Neuronal-induced augmentation of cardiac output. Can J Cardiol 15: 1361-1366, 2000.

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