Pacemaker Mechanisms

Normal automaticity involves a spontaneous, slow, progressive decline in the transmembrane potential (i.e., the membrane voltage becomes less negative) during diastole. This process is known as “spontaneous diastolic depolarization” or “phase 4 depolarization.” Once this spontaneous depolarization reaches threshold (approximately −40 mV), a new action potential is generated ( Fig. 3.1 ) ( see Chapter 1 ).

Normal Cardiac Automaticity.

Action potentials from typical sinus nodal and His-Purkinje cells are shown with the voltage scale on the vertical axes; dashed lines are threshold potential, and numbers on the figure refer to phases of the action potential. Note the qualitative differences between the two types of cells, as well as different rates of spontaneous depolarization. Ca ²⁺ , Calcium; HPS , His-Purkinje system; Na ⁺ , sodium.

The ionic mechanisms responsible for normal pacemaker activity in the sinus node are still controversial. The fall in membrane potential during phase 4 seems to arise from a changing balance between positive inward currents, which favor depolarization, and positive outward currents, with a net gain in intracellular positive charges during diastole (i.e., a net inward depolarizing current) ( Fig. 3.2 ).

Ionic Currents Involved in Producing the Sinus Node Pacemaker Potential.

A typical action potential of spontaneously beating rabbit sinus node is shown on the top (red trace) . The different phases are labeled, with phase 4 representing diastolic depolarization, the defining feature of pacemaking cells. The timing and magnitude of the components of the “membrane clock” is shown in the middle (green bracket) . There is voltage-dependent decay of the outward rectifier K ⁺ current I _K , and voltage-dependent activation of inward currents: I _f , I _CaL , and I _CaT . The timing and magnitude of the components of the “calcium clock” are shown at the bottom (dark blue bracket) . Ca ²⁺ entry into the cell via I _CaL and I _CaT results in spontaneous local Ca ²⁺ release (LCR) from the sarcoplasmic reticulum (SR) through RyR2 channels. During phase 4, this rise in total intracellular Ca ²⁺ activates the Na ⁺ -Ca ²⁺ exchanger (NCX1) which generates the net inward I _NCX (or I _Na-Ca ) current. Toward the end of diastole, activation of L-type Ca ²⁺ channels causes Ca ²⁺ -induced Ca ²⁺ release from the SR via RyR2, resulting in the whole cell Ca ²⁺ transient. Cytoplasmic Ca ²⁺ is then removed by the SR Ca ²⁺ pump sarcoplasmic/endoplasmic reticulum calcium adenosine triphosphatase (SERCA) and by the sarcolemmal Na ⁺ -Ca ²⁺ exchanger. AP , Action potential; DD , diastolic depolarization; I _CaL , L-type voltage-dependent Ca ²⁺ current; I _CaT , T-type voltage-dependent Ca ²⁺ current; I _f , funny current; I _K , delayed rectifier potassium current; I _NCX , sodium-calcium exchange current; LCRs , local Ca ²⁺ releases; MDP , maximum diastolic potential.

(From Murphy C, Lazzara R. Current concepts of anatomy and electrophysiology of the sinus node. J Interv Card Electrophysiol . 2016;46:9–18.)

Hierarchy of Pacemaker Function

Automaticity is not limited to the cells within the sinus node. Under physiological conditions, cells in parts of the atria and within the atrioventricular node (AVN) and the His-Purkinje system (HPS) also possess pacemaking capability. However, the occurrence of spontaneous activity in these cells is prevented by the natural hierarchy of pacemaker function that causes these sites to be latent or subsidiary pacemakers. The spontaneous discharge rate of the sinus node normally exceeds that of all other subsidiary pacemakers (see Fig. 3.1 ). Therefore the impulse initiated by the sinus node depolarizes subsidiary pacemaker sites and keeps their activity depressed before they can spontaneously reach threshold. However, slowly depolarizing and previously suppressed pacemakers in the atrium, AVN, or ventricle can become active and assume pacemaker control of the cardiac rhythm if the sinus node pacemaker becomes slow or unable to generate an impulse (e.g., secondary to depressed sinus node automaticity) or if impulses generated by the sinus node are unable to activate the subsidiary pacemaker sites (e.g., sinoatrial exit block or atrioventricular [AV] block). The emergence of subsidiary or latent pacemakers under such circumstances is an appropriate fail-safe mechanism, which ensures that ventricular activation is maintained. Because spontaneous diastolic depolarization is a normal property, the automaticity generated by these cells is classified as normal .

There is also a natural hierarchy of the intrinsic rates of subsidiary pacemakers that have normal automaticity, with atrial pacemakers having faster intrinsic rates than AV junctional pacemakers, and AV junctional pacemakers having faster rates than ventricular pacemakers.

Subsidiary Pacemakers

Regulation of Pacemaker Function

The intrinsic rate at which the sinus node pacemaker cells generate impulses is determined by the interplay of three factors: the maximum diastolic potential, the threshold potential at which the action potential is initiated, and the rate (slope) of phase 4 depolarization ( eFig. 3.1 ). A change in any one of these factors will alter the time required for phase 4 depolarization to carry the membrane potential from its maximum diastolic level to threshold and thus alter the rate of impulse initiation.

Abnormalities of Automaticity.

(A) Normal His-Purkinje action potential. (B) Modulation of rate of depolarization from baseline (1) by slowing rate of phase 4 depolarization (2) , increasing threshold potential (3) , starting from a more negative resting membrane potential (4) , all of which slow discharge rate, or by increasing rate of phase 4 depolarization (5) , thus yielding a faster discharge rate. (C) Abnormal automaticity with change in action potential contour (resembling sinus nodal cell) when resting membrane potential is less negative, inactivating most sodium channels.

The sinus node is innervated by the parasympathetic and sympathetic nervous systems, and the balance between these systems importantly controls the pacemaker rate. The classic concept has been that of a reciprocal relationship between sympathetic and parasympathetic inputs. However, more recent investigations stress dynamic, demand-oriented interactions, and the anatomical distribution of fibers that allows both autonomic systems to act quite selectively. Muscarinic cholinergic and beta ₁ -adrenergic receptors are nonuniformly distributed in the sinus node, and they modulate both the rate of depolarization and impulse propagation.

Inappropriate Sinus Node Discharge

Examples of these arrhythmias include inappropriate sinus bradycardia, sinus arrest, inappropriate sinus tachycardia, and inappropriate respiratory sinus arrhythmia. Such arrhythmias result simply from an alteration in the rate of impulse initiation by the normal sinus node pacemaker, without a shift of impulse origin to a subsidiary pacemaker at an ectopic site, although there can be shifts of the pacemaker site within the sinus node itself during alterations in sinus rate. These arrhythmias are often a result of the actions of the autonomic nervous system on the sinus node.

Escape Ectopic Automatic Rhythms

Impairment of the sinus node can allow a latent pacemaker to initiate impulse formation. This would be expected to happen when the rate at which the sinus node overdrives subsidiary pacemakers falls considerably below the intrinsic rate of the latent pacemakers or when the inhibitory electrotonic influences between nonpacemaker cells and pacemaker cells are interrupted.

The rate at which the sinus node activates subsidiary pacemakers can be decreased in certain situations, including sinus node dysfunction, with depressed sinus automaticity (secondary to increased vagal tone, drugs, or intrinsic sinus node disease), sinoatrial exit block, AV block, and parasystolic focus. The sinus node and AVN are most sensitive to vagal influence, followed by atrial tissue, with the ventricular conducting system being least sensitive. Moderate vagal stimulation allows the pacemaker to shift to another atrial site, but severe vagal stimulation suppresses the sinus node and blocks conduction at the AVN and therefore can allow a ventricular escape pacemaker to become manifest.

Interruption of the inhibitory electrotonic influences between nonpacemaker cells and pacemaker cells allows those latent pacemakers to fire at their intrinsic rate. Uncoupling can be caused by fibrosis or damage (e.g., infarction) of the tissues surrounding the subsidiary pacemaker cells or by reduction in gap junction conductance secondary to increased intracellular Ca ²⁺ , which can be caused by digitalis. Some inhibition of the sinus node is still necessary for the site of impulse initiation to shift to an ectopic site that is no longer inhibited by uncoupling from surrounding cells because the intrinsic firing rate of subsidiary pacemakers is still slower than that of the sinus node.

Accelerated Ectopic Automatic Rhythms

Accelerated ectopic automatic rhythms are caused by enhanced normal automaticity of subsidiary pacemakers. The rate of discharge of these latent pacemakers is then faster than the expected intrinsic automatic rate. Once the enhanced rate exceeds that of the sinus node, the enhanced ectopic pacemaker prevails and overdrives the sinus node and other subsidiary pacemakers. A premature impulse caused by enhanced automaticity of latent pacemakers comes early in the normal rhythm. In contrast, an escape beat secondary to relief of overdrive suppression occurs late in normal rhythm.

Enhanced automaticity is usually caused by increased sympathetic tone, which steepens the slope of diastolic depolarization of latent pacemaker cells and diminishes the inhibitory effects of overdrive. Such sympathetic effects can be localized to subsidiary pacemakers in the absence of sinus node stimulation. Other causes of enhanced normal automaticity include periods of hypoxemia, ischemia, electrolyte disturbances, and certain drug toxicities. There is evidence that in the subacute phase of myocardial ischemia, increased activity of the sympathetic nervous system can enhance automaticity of Purkinje fibers, thus enabling them to escape from sinus node domination.

Parasystole

Parasystole is a result of interaction between two fixed rate pacemakers having different discharge rates. Parasystolic pacemakers can exist in either the atrium or the ventricle. The latent pacemaker is protected from being overdriven by the dominant rhythm (usually NSR) by intermittent or constant entrance block (i.e., impulses of sinus origin fail to depolarize the latent pacemaker secondary to block in the tissue surrounding the latent pacemaker focus).

Various mechanisms have been postulated to explain the protected zone surrounding the ectopic focus. It is possible that the depolarized level of membrane potential at which abnormal automaticity occurs can cause entrance block, leading to parasystole. This would be an example of an arrhythmia caused by a combination of an abnormality of impulse conduction and impulse initiation. However, such block must be unidirectional, so that activity from the ectopic pacemaker can exit and produce depolarization whenever the surrounding myocardium is excitable. The protected pacemaker is said to be a parasystolic focus. In general, under these conditions, a protected focus of automaticity of this type fires at its own intrinsic frequency, and the intervals between the discharges of each pacemaker are multiples of its intrinsic discharge rate (sometimes described as fixed parasystole ). Therefore on the surface electrocardiogram (ECG) the coupling intervals of the manifest ectopic beats wander through the basic cycle of the sinus rhythm. Accordingly, the traditional ECG criteria used to recognize the fixed form of parasystole include: (1) the presence of variable coupling intervals of the manifest ectopic beats; (2) interectopic intervals that are simple multiples of a common denominator; and (3) the presence of fusion beats. Occasionally, the parasystolic focus can exhibit exit block, during which it may fail to depolarize excitable myocardium.

Although the parasystolic focus is protected, it may not be totally immune to the surrounding electrical activity. The effective electrical communication that permits the emergence of the ectopic discharges can also allow the rhythmic activity of the surrounding tissues to electrotonically influence the periodicity of the pacemaker discharge rate (described as modulated parasystole ). Electrotonic influences arriving during the early stage of diastolic depolarization result in a delay in the firing of the parasystolic focus, whereas those arriving late accelerate the discharge of the parasystolic focus. As a consequence, the dominant pacemaker can entrain the partially protected parasystolic focus and force it to discharge at periods that may be faster or slower than its own intrinsic cycle and give rise to premature discharges whose patterns depend on the degree of modulation and the basic heart rate, occasionally mimic reentry, and occur at fixed coupling intervals. Therefore appropriate diagnosis of modulated parasystole relies on the construction of a phase response curve as theoretical evidence of modulation of the ectopic pacemaker cycle length (CL) by the electrotonic activity generated by the sinus discharges across the area of protection.

All these features of abnormal automaticity can be found in the Purkinje fibers that survive in regions of transmural MI and cause ventricular arrhythmias during the subacute phase.

Arrhythmias Caused by Abnormal Automaticity

There appears to be an association between abnormal Purkinje fiber automaticity and the arrhythmias that occur during the acute phase of MI (e.g., an accelerated idioventricular rhythm). However, the role of abnormal automaticity in the development of ventricular arrhythmias associated with chronic ischemic heart disease is less certain. In addition, isolated myocytes obtained from hypertrophied and failing hearts have been shown to manifest spontaneous diastolic depolarization and enhanced I _f , findings, suggesting that abnormal automaticity can contribute to the occurrence of some arrhythmias in heart failure and ventricular hypertrophy.

Abnormal automaticity can underlie atrial tachycardia, accelerated idioventricular rhythms, and ventricular tachycardia (VT), particularly that associated with ischemia and reperfusion. It has also been suggested that injury currents at the borders of ischemic zones can depolarize adjacent nonischemic tissue, thus predisposing to automatic VT.

Although automaticity is not responsible for most clinical tachyarrhythmias, which are usually caused by reentry or triggered activity, normal or abnormal automaticity can lead to arrhythmias caused by nonautomatic mechanisms. Premature beats, caused by automaticity, can initiate reentry. Rapid automatic activity in sites such as the cardiac veins can cause fibrillatory conduction, reentry, and atrial fibrillation (AF).

Ionic Basis of Delayed Afterdepolarizations

DADs usually occur under a variety of conditions in which Ca ²⁺ overload develops in the cytoplasm and sarcoplasmic reticulum. During the plateau phase of the normal action potential, Ca ²⁺ flows through voltage-dependent L-type Ca ²⁺ channels (I _CaL ). Although the rise in intracellular Ca ²⁺ is small and not sufficient to induce contraction, the small amount of Ca ²⁺ entering the cell via I _CaL triggers a massive release of Ca ²⁺ from the sarcoplasmic reticulum (the major store for Ca ²⁺ ) into the cytosol by opening the RyR2 channels (present in the membrane of the sarcoplasmic reticulum) in a process known as calcium-induced calcium release (CICR). During electrical diastole, most of the surplus Ca ²⁺ in the cytosol is resequestered into the sarcoplasmic reticulum by the sarcoplasmic/endoplasmic reticulum calcium adenosine triphosphatase (SERCA), the activity of which is controlled by the phosphoprotein phospholamban. In addition, some of the Ca ²⁺ is extruded from the cell by the Na ⁺ -Ca ²⁺ exchanger to balance the Ca ²⁺ that enters via I _CaL . Recurring Ca ²⁺ release-uptake cycles provide the basis for periodic elevations of the cytosolic Ca ²⁺ concentration and contractions of myocytes, hence for the orderly beating of the heart ( Fig. 3.6 ).

Signal Transduction Schema for Initiation and Termination of Cyclic Adenosine Monophosphate (cAMP) -Mediated Triggered Activity.

See text for discussion. A1R , α1-adenosine receptor; AC , adenylyl cyclase; ACh , acetylcholine; ADO , adenosine; ATP , adenosine triphosphate; Ca , calcium; CCB , calcium channel blocker; DAD , delayed afterdepolarization; GDP , guanosine diphosphate; GTP , guanosine triphosphate; Gαi , inhibitory G protein; Gαs , stimulatory G protein; I _ti , transient inward current; M2R , muscarinic receptor; Na , sodium; NCX , sodium (Na ⁺ )-calcium (Ca ²⁺ ) exchanger; PKA , protein kinase A; PLB , phospholamban; RyR , ryanodine receptor; SR , sarcoplasmic reticulum; β -AR , β-adrenergic receptor.

(From Lerman BB. Mechanism of outflow tract tachycardia. Heart Rhythm . 2007;4:973.)

Under various pathological conditions, Ca ²⁺ concentration in the sarcoplasmic reticulum can rise to a critical level during repolarization (i.e., Ca ²⁺ overload), at which time a secondary spontaneous release of Ca ²⁺ from the sarcoplasmic reticulum occurs after the action potential, rather than as a part of excitation-contraction coupling. This secondary release of Ca ²⁺ results in inappropriately timed Ca ²⁺ transients and contractions. Spontaneous Ca ²⁺ waves can be arrhythmogenic; they induce Ca ²⁺ -dependent depolarizing membrane currents (transient inward current [I _ti ]), mainly by activation of the Na ⁺ -Ca ²⁺ exchanger. Increases in intracellular Ca ²⁺ levels can stimulate the Na ⁺ -Ca ²⁺ exchanger (I _Na-Ca ), which exchanges three Na ⁺ ions for one Ca ²⁺ ion; the direction depends on the Na ⁺ and Ca ²⁺ concentrations on the two sides of the membrane and the E _m difference. At resting E _m and during a spontaneous sarcoplasmic reticulum Ca ²⁺ release event, this exchanger operates in the forward mode (three Na ⁺ ions in for one Ca ²⁺ ion out) and generates a net Na ⁺ influx, causing transient oscillations of the membrane potential (DADs). After one or several DADs, myoplasmic Ca ²⁺ can decrease because the Na ⁺ -Ca ²⁺ exchanger extrudes Ca ²⁺ from the cell, and the membrane potential stops oscillating.

When the DADs are of low amplitude ( subthreshold DAD), they usually are not apparent or clinically significant. However, during pathological conditions (e.g., myocardial ischemia, acidosis, hypomagnesemia, digitalis toxicity, and increased catecholamines), the amplitude of the Ca ²⁺ -mediated membrane depolarization is increased and can reach the stimulation threshold ( suprathreshold DAD) and an action potential is triggered (called triggered activity ). If this process continues, sustained tachycardia will develop. Triggered action potentials can also initiate reentry when they encounter a vulnerable tissue substrate.

Probably the most important influence that causes subthreshold DADs to reach threshold is a decrease in the initiating CL because that increases both the amplitude and rate of the DADs. Therefore initiation of arrhythmias triggered by DADs can be facilitated by a spontaneous or pacing-induced increase in the heart rate.

Subthreshold DADs can also play a role in arrhythmogenesis by partially depolarizing the cell membrane and hence inactivating a portion of Na ⁺ channels and reducing their availability during the subsequent (triggered or nontriggered) action potential. The resultant regional dispersion of excitability or refractoriness can generate a tissue substrate vulnerable to unidirectional conduction block and reentry.

Role of Delayed Afterdepolarizations in Arrhythmogenesis

A suprathreshold DAD can trigger an action potential and generate triggered activity, which can cause focal, nonreentrant arrhythmias (triggered activity atrial or ventricular ectopic beats or tachycardia) or, when it encounters a vulnerable tissue substrate, the triggered action potential can act as a trigger for initiation of reentrant arrhythmias.

Both suprathreshold and subthreshold DADs can potentially generate a vulnerable substrate and promote reentry by regionally decreasing excitability sufficiently to cause regional conduction block of a subsequent nontriggered action potential. In addition, when both subthreshold and suprathreshold DADs coexist in the same tissue, the combination of triggers and a vulnerable substrate can lead directly to reentry initiation. DADs can potentially generate both a vulnerable substrate that promotes reentry, as well as a trigger for initiation of reentrant arrhythmias. In some regions, suprathreshold DADs can trigger an action potential, whereas in other regions, subthreshold DADs promoting regional conduction block. Once the triggered action potential propagates to the region of conduction block, it may initiate reentry.

DAD-related triggered activity is thought to be a mechanism for tachyarrhythmia associated with MI, reperfusion injury, digitalis toxicity, and some idiopathic VTs, as well as some arrhythmias associated with inherited channelopathies. DADs are more likely to occur with fast spontaneous or paced rates or with increased premature beats.

Properties of Delayed Afterdepolarizations

The amplitude of DADs and the possibility of triggered activity are influenced by the level of membrane potential at which the action potential occurs. The reduction of the membrane potential during DADs may also result in Na ⁺ channel inactivation and hence slowing of conduction.

The duration of the action potential is a critical determinant of the presence of DADs. Longer action potentials, which are associated with more transsarcolemmal Ca ²⁺ influx, are more likely to be associated with DADs. Drugs that prolong action potential duration (e.g., class IA antiarrhythmic agents) can increase DAD amplitude, whereas drugs that shorten action potential duration (e.g., class IB antiarrhythmic agents) can decrease DAD amplitude.

The number of the action potentials preceding the DAD affects the amplitude of the DAD (i.e., after a period of quiescence, the initiation of a single action potential can be followed by either no DAD or only a small one). With continued stimulation, the DADs increase in amplitude, and triggered activity can eventually occur.

The amplitude of DADs and the coupling interval between the first triggered impulse and the last stimulated impulse that induced them are directly related to the drive CL at which triggered impulses are initiated. A decrease in the basic drive CL (even a single drive cycle; i.e., premature impulse), in addition to increasing the DAD amplitude, results in a decrease in the coupling interval between the last drive cycle and the first DAD-triggered impulse, with respect to the last driven action potential, and an increase of the rate of DADs. Triggered activity tends to be induced by a critical decrease in the drive CL, either spontaneous, such as in sinus tachycardia, or pacing induced. The increased time during which the membrane is in the depolarized state at shorter stimulation CLs or after premature impulses increases Ca ²⁺ in the myoplasm and the sarcoplasmic reticulum (because of repeated activation of I _CaL ), thus increasing the I _ti responsible for the increased DAD amplitude, causing the current to reach its maximum amplitude more rapidly, and decreasing the coupling interval of triggered impulses. This characteristic property can help to distinguish triggered activity from reentrant activity because the relationship for reentry impulses initiated by rapid stimulation is often the opposite (i.e., as the drive CL is reduced, the first reentrant impulse occurs later with respect to the last driven action potential because of rate-dependent conduction slowing in the reentrant pathway).

In general, triggered activity is markedly influenced by overdrive pacing. These effects are dependent on both the rate and the duration of overdrive pacing. When overdrive pacing is performed for a critical duration of time and at a critical rate during a catecholamine-dependent triggered rhythm, the rate of triggered activity slows until the triggered rhythm stops, because of enhanced activity of the electrogenic Na ⁺ -K ⁺ exchange pump induced by the increase in intracellular Na ⁺ caused by the increased number of action potentials. When overdrive pacing is not rapid enough to terminate the triggered rhythm, it can cause overdrive acceleration (in contrast to overdrive suppression observed with automatic rhythms). Single premature stimuli also can terminate triggered rhythms, although termination is much less common than it is by overdrive pacing.

Ionic Basis of Early Afterdepolarizations

Normal cardiac repolarization relies on a critical balance between depolarizing inward currents and repolarizing outward currents during the action potential plateau. Repolarization has built-in redundancy (“repolarization reserve”) to protect against excessive prolongation of the action potential duration. The plateau of the action potential is a time of high membrane resistance (i.e., membrane conductance to all ions falls to rather low values), when there is little current flow. Consequently, small changes in repolarizing or depolarizing currents can have profound effects on the action potential duration and profile. Normally, during phases 2 and 3, the net membrane current is outward. Any factor that transiently shifts the net current in the inward direction can potentially overcome and reverse repolarization (a condition termed “reduced repolarization reserve”) and lead to EADs and EAD-related arrhythmias. Such a shift can arise from decreased outward (repolarizing) currents (mostly carried by K ⁺ at that time), increased inward (depolarizing) currents (carried by Na ⁺ or Ca ²⁺ at that time), or both. However, although reduced repolarization reserve is sufficient to prolong action potential duration, it is not sufficient to produce EADs. Other conditions are required to generate the voltage oscillations pathognomonic of EADs, which arise from different causes. The most critical to the dynamics of EAD oscillations include window I _CaL , late I _Na , and I _Ks . In addition, EADs can also be promoted by intracellular Ca ²⁺ oscillations or by prolonged Ca ²⁺ transients via Na ⁺ -Ca ²⁺ exchanger current (I _Na-Ca ).

EADs have been classified as phase 2 (occurring at the plateau level of membrane potential) and phase 3 (occurring during phase 3 of repolarization) (see Fig. 3.4 ). The ionic mechanisms of phase 2 and phase 3 EADs and the upstrokes of the action potentials they elicit can differ. At the depolarized membrane voltages of phase 2, Na ⁺ channels are inactivated; hence the I _CaL and I _Na-Ca are the major currents potentially responsible for EADs. Voltage steady-state activation and inactivation of the L-type Ca ²⁺ channels are sigmoidal, with an activation range over −40 to +10 mV (with a half-activation potential near −15 mV) and a half-inactivation potential near −35 mV. However, a relief of inactivation for voltages positive to 0 mV leads to a U -shaped voltage curve for steady-state inactivation. Overlap of the steady-state voltage-dependent inactivation and activation relations defines a “window” current near the action potential plateau, within which transitions from closed and open states can occur. As the action potential repolarizes into the window region, I _CaL increases and can potentially be sufficient to reverse repolarization, thus generating the EAD upstroke ( Fig. 3.7 ).

Only gold members can continue reading. Log In or Register to continue

Share this:

• Click to share on Twitter (Opens in new window)
• Click to share on Facebook (Opens in new window)

Related

Related posts:

1. Focal Atrial Tachycardia
2. Atrioventricular Nodal Reentrant Tachycardia
3. Sinus Node Dysfunction
4. Paroxysmal Supraventricular Tachycardias

Stay updated, free articles. Join our Telegram channel

Join