Abstract
Arrhythmias arise from breakdown of orderly action potential (AP) activation, propagation and recovery driven by interactive opening and closing of successive voltage-gated ion channels, in which one or more Na+ current components play critical parts. Early peak, Na+ currents (I Na) reflecting channel activation drive the AP upstroke central to cellular activation and its propagation. Sustained late Na+ currents (I Na-L) include contributions from a component with a delayed inactivation timecourse influencing AP duration (APD) and refractoriness, potentially causing pro-arrhythmic phenotypes. The magnitude of I Na-L can be analysed through overlaps or otherwise in the overall voltage dependences of the steady-state properties and kinetics of activation and inactivation of the Na+ conductance. This was useful in analysing repetitive firing associated with paramyotonia congenita in skeletal muscle. Similarly, genetic cardiac Na+ channel abnormalities increasing I Na-L are implicated in triggering phenomena of automaticity, early and delayed afterdepolarisations and arrhythmic substrate. This review illustrates a wide range of situations that may accentuate I Na-L. These include (1) overlaps between steady-state activation and inactivation increasing window current, (2) kinetic deficiencies in Na+ channel inactivation leading to bursting phenomena associated with repetitive channel openings and (3) non-equilibrium gating processes causing channel re-opening due to more rapid recoveries from inactivation. All these biophysical possibilities were identified in a selection of abnormal human SCN5A genotypes. The latter presented as a broad range of clinical arrhythmic phenotypes, for which effective therapeutic intervention would require specific identification and targeting of the diverse electrophysiological abnormalities underlying their increased I Na-L.
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Introduction
Arrhythmias follow disruption of the normal interacting succession of ion channel activation and inactivation that produces the transmembrane currents underlying the propagated action potential (AP) [10, 23, 80]. In skeletal muscle, these manifest as a range of syndromes associated with repetitive action potential firing associated with a number of ion channel abnormalities. Where involving the heart, ventricular arrhythmia potentially results in sudden cardiac death (SCD), which accounts for ∼4 to 5 million deaths per year worldwide [17]. Cardiac ischaemia accounts for most cases of arrhythmia [9], but ∼10–20% of arrhythmic deaths may result from ion channelopathy [40]. These could affect ion channels carrying Na+, I Na, and Ca2+ depolarizing currents, I Ca, and a number of, I to, I Kr, I Ks and I K1, K+ channels contributing repolarizing current [57, 70]. The depolarisation-activated I Ca induces Ca2+ release from intracellular sarcoplasmic reticular Ca2+ stores which triggers mechanical activity. The detailed AP timecourse in different cardiac regions or animal species is determined by their corresponding patterns of ion channel expression [71]. Once generated, local circuit currents driven by the inward flux of Na+ propagate APs to hitherto quiescent myocardial regions through gap junctions between successive cells. The result is a wave of membrane depolarisation followed by refractoriness [39].
The Na+ channel is central to this excitation process in view of its strategic role in initiation of the cardiac AP. The Na+ current, I Na, may comprise a mixture of currents with different kinetics. These might arise from modulations in the principal Nav species or distinct channel subpopulations [67, 68]. Functional alterations in the biophysical properties of the Na+ channel thus lead to a range of arrhythmic conditions. An important group of these is the result of sustained inward Na+ current. The repetitive firing observed in skeletal muscle fibres in patients with paramyotonia congenita arises from an incomplete voltage-dependent Na+ channel inactivation thus leaving some channels in a conductive state [45]. This results from mutations in the skeletal muscle Nav1.4 channel [22, 44, 69] that produce positive shifts in the half maximal voltage of its steady-state inactivation function (V inact). Alternatively, negative shifts in the voltage dependence of Na+ channel activation (V act) permit channel activation with smaller depolarisations. Either situation potentially results in sustained inward current that follows excitation that can cause recurrent channel re-activation [12, 28, 29].
In cardiac muscle, sustained inward Na+ currents also known as late Na+ currents (I Na-L) occur under physiological conditions during the cardiac AP. These currents nevertheless have conductance, mean open time and selectivity properties identical to the remaining Nav1.5 current [25, 37]. It remains possible to consider both early Na+ currents and potentially arrhythmogenic I Na-L in terms of the overall activation and inactivation characteristics that they produce in cardiac myocytes. A comparison with clinical findings will demonstrate that cardiac muscle shows a wider range of possible variations in such characteristics than the straightforward shifts in steady-state activation and inactivation reported so far in skeletal muscle. These findings have implications for therapeutic intervention.
Na+ channel activation and inactivation
The cardiac Na+ channel multi-unit protein comprises principal Nav1.5, α- and associated auxiliary β-subunits. The α-subunit consists of four homologous domains (I–IV) each containing six transmembrane segments (S1–S6) [8], and it suffices to mediate ion selectivity, and the voltage-gated activation and inactivation properties of the channel [62]. Voltage-gated Nav1.5 activation depends on transitions in the S4 segment whose positively charged amino acids at every third position likely subserve a voltage-sensing function [13]. Membrane depolarisation moves the S4 segment relative to other channel segments so that the voltage-sensing domain, formed by the S1–S4 block, rotates. This permits Na+ influx through the pore-forming component made up of the S5 and S6 segments and the re-entrant P loop [21, 50]. This early I Na drives the rapid AP upstroke resulting in further channel activation. Hodgkin and Huxley (1952) had first described such activation in terms of three m particles undergoing a voltage-dependent, first-order transition from an inactive to active state, giving channel openings of higher-order kinetics [32]. The maximum attainable Na+ current would depend upon the number of available channels, and be compromised in situations of Nav1.5 insufficiency, as in Brugada syndrome (BrS) [42].
Nav1.5 inactivation terminates the inward I Na permitting membrane repolarisation also driven by other, outward, ionic currents. Nav1.5 inactivation involves two, fast and slow, kinetic components. Fast inactivation occurs within milliseconds and results from the cytoplasmic III–IV linker occluding the pore [38]. This may involve an isoleucine-phenylalanine-methionine (IFM) motif, which is a hydrophobic triplet in the III–IV linker that may act as a ‘latch’ keeping the fast inactivation gate shut [38]. Docking sites for this inactivation gate likely include the S6 segment in domain IV and the S4–5 loops in domains III and IV [8]. Hodgkin and Huxley correspondingly described a parallel first-order, voltage-dependent h-inactivation process resulting in refractoriness with prolonged depolarisation and recovery from such refractoriness with repolarisation. Slow inactivation, subsequently reported in NaF-perfused Loligo axons [14, 63], may include structurally distinct components [83], likely involving conformational changes of the pore component of the α-subunit [81].
These processes have been organised in a reaction scheme in which a channel transitions through several closed (C 0 to C 3) resting states, then an open (O) state, with voltage-dependent rate constants k mn intervening between any given pair of states m and n. The channel then transitions through inactivated (I 1 and I 2) states, followed by recovery from inactivation, similarly governed by voltage-dependent rate constants α h and β h (Fig. 1). The latter suggests resting, activated and inactivated states of the channel in which the channel is closed during resting and inactivated states, with separate processes mediating activation and inactivation. Channel opening with depolarisation is dependent not only upon the extent of activation but also upon the extent to which channels have transitioned into an inactivated state. These openings increase the membrane Na+ conductance, g Na, in turn permitting a peak I Na or I Na-L to take place down its net electrochemical driving force (V-E Na), contributing to the in vivo waveform of the cardiac AP (Fig. 2a). An early peak I Na related to the activation process of the channel drives the upstroke of the AP and rapidly inactivates within a few milliseconds. The Na+ channel component underlying I Na-L shows a diminished or slowed inactivation and a more negative (20 mV) voltage dependence in its activation properties than the remaining I Na [68]. Early modelling predicted an I Na-L of magnitude ∼1–2% of peak I Na [48, 58]. Increases in I Na-L thus influence AP duration and refractoriness. Currents arising from additional background I bNa attributed to Na+-K+-ATPase and Na+-Ca2+ exchange-mediated leak currents are distinct from the voltage-dependent Na+ channel processes analysed here [7, 15, 31, 58].
Graphical representation of Na+ channel activation and inactivation
Figure 3 illustrates graphical representations of the consequences of these activation and inactivation processes and their possible interaction, which predicts the resulting I Na. First, the steady-state activation curve illustrates the potential increase in Na+ conductance and therefore of I Na as a function of the membrane potential V. Each individual I Na component would reflect a conductance contribution g Na described by a Boltzmann distribution between two, open and closed, states whose energies that vary linearly with V. This would predict a sigmoid relationship between g Na and V. In the equation,
term g Na * is the maximum value of g Na and V act is the voltage at its half-maximum value. The term k act is the slope factor for activation, which characterises the voltage sensitivity of the component channel in terms of the valency, z, of the charge transfer involved in its transitions between the open and closed states, through the equation k act = RT/(zF), where R = gas constant, T = temperature and F = Faraday’s constant. Either increasing the value of z or reducing the value of k act will increase the steepness of the activation-voltage relationship.
Second, steady-state inactivation curves normalised to the interval [0,1] give an indication of the fraction of activatable channels mediating each Na+ conductance component, h, as limited by the degree of inactivation, each with its own inactivation slope factor k inact,
Third, in addition to their steady-state properties, the activation and inactivation processes show distinct kinetics. Inactivation kinetics is typically slower than activation kinetics and extends over timescales comparable to the recovery phase of the AP. A family of inactivation curves rather than a single inactivation curve could be used to represent the time evolution of the inactivation process as might occur following imposition of a given voltage step. For any given component, the simplest two-state model might assume activatable and inactivated states of energies E 1(V) and E 2(V), respectively, linearly dependent on the voltage V through a coefficient dependent on their effective position in the membrane field. It could then incorporate forward, α, and backward, β, rate constants determined by the energy of the barrier E *(V) given by α(V) = A exp{[E 1(V) − E *(V)]/kT} and β(V) = A exp{[E 2(V) − E *(V)]/kT}, where k in this instance represents the Boltzmann constant and A the Arrhenius constant [1].
The relationship between Na+ channel activation and inactivation curves and the late Na+ current, I Na-L
The relative contributions of activation and inactivation properties can be assessed from plots of their respective overall dependencies upon voltage. These are shown in functions illustrated using established experimental values in Fig. 3a [51]. An imposed voltage step would produce a rapid activation of g Na, whose value would fall close to the corresponding ordinate of the activation curve. Thus, there will initially be little evidence of the slower inactivation process, but this will subsequently cause g Na to decline. This time evolution of inactivation is represented by the successive dotted transient inactivation curves that progressively approach the steady-state inactivation curve, which would predict full inactivation at depolarised voltages. Alternatively, a persistent conductance would result from an incomplete inactivation either at times when the relevant decay is incomplete or in the event of an incomplete steady-state inactivation at the voltage in question. Thus, the effective g Na at any given time following a particular voltage step is effectively the ordinate in the activation multiplied by corresponding ordinate in the inactivation function.
Figure 3b reconstructs both the g Na activation (full arrows) and inactivation variables (open arrows) through the timecourse of the cardiac AP. The charging of an initially quiescent membrane at the resting potential (i) by local circuit currents through the passive cable formed by intervening cardiac myocytes from previously excited membrane regions produces an activation locus ((i)–(ii)) to the foot of the activation-voltage relationship. The resulting Na+ channel opening initiates a regenerative cycle of depolarisation and further channel opening producing the steep rise of g Na along the activation curve from ((ii)–(iii)) to maximum channel activation along ((iv)–(v)), thereby completing phase 0 of the cardiac AP. The inactivation locus is then followed through phase 1 fast early repolarisation ((v)–(vi)), during which there is a rapid Na+ channel inactivation. This is succeeded by the phase 2 plateau ((vi)–(vii)), during which an incomplete development of inactivation leaves a finite I Na-L. Locus ((vii)–(viii)) traces phase 3 terminal repolarisation and a return to electrophysiological diastole at the resting potential ((viii)–(ix)). Recovery from inactivation is favoured at membrane potentials near to the resting potential and this then permits re-excitation.
Importance of late Na+ current, I Na-L
Figure 2a illustrates a presence of I Na-L during the AP plateau phase, whereas Fig. 2b illustrates circumstances of increased I Na-L. In addition to extending the plateau duration before AP recovery, an increased I Na-L can lead to the development of various triggers and substrates for arrhythmogenesis. First, it can cause diastolic depolarisation phenomena, which trigger inappropriate APs in the sino-atrial node (SAN) and the potentially pacemaking atrioventricular node (AVN) and His-Purkinje cells. This can result in an abnormal automaticity reduced by inhibiting such I Na-L [23, 76]. Second, enhanced I Na-L can predispose to afterdepolarisations during or immediately following an AP [87]. Of these, early afterdepolarisations (EADs) occur during phase 2 or 3 of a prolonged AP [5, 23]. This then causes a regenerative L-type Ca2+ channel re-activation, whilst the membrane remains depolarised during a prolonged AP plateau phase. EADs have been observed both in genetic conditions such as long QT syndrome (LQTS) and acquired conditions such as cardiac failure [36]. Delayed afterdepolarisations (DADs) follow full repolarisation in cells with Ca2+ overload. These in turn predispose to depolarizing, transient inward currents. Although smaller than the peak I Na, I Na-L has a 50–100-fold longer duration and thereby can increase cellular Na+ loading, in turn reducing the gradient for Ca2+ efflux through sodium-calcium exchange current [58]. DADs may underlie arrhythmias seen in some heart failure patients, patients with digitalis toxicity and patients with catecholaminergic polymorphic ventricular tachycardia [5].
Third, the presence of I Na-L also bears upon re-entrant processes re-exciting recovered regions, thus furnishing arrhythmic substrate perpetuating the initial arrhythmic event [3]. I Na-L upregulation by Anemonia sulcata toxin (ATX-II) increased dispersion of repolarisation and refractoriness. This could lead to the torsades de pointes associated with LQTS [4]. Finally, I Na-L also increases the slope of the AP duration (APD) restitution curve relating AP duration to the diastolic interval intervening between AP recovery and generation of the subsequent AP during regular stimulation at successively higher frequencies [59, 78]. A pathological I Na-L upregulation therefore promotes arrhythmic triggers and substrates through a variety of pathways, summarised in Fig. 4.
I Na-L and altered gNa activation
Increased I Na-L thus potentially constitutes a final common pathway explaining a wide range of pro-arrhythmic phenomena. However, a wide range of alterations in either or both of the biophysical properties of g Na activation and inactivation (Fig. 5a) provide potential causative mechanisms for increased I Na-L. These range from alterations in maximum g Na despite an otherwise unaltered activation-voltage plot, as could occur following an increased surface membrane Na+ channel expression (Fig. 5b). This situation would contrast with the consequences of some Brugada syndrome cases, which contain a Nav1.5 haploinsufficiency [51].
In the remaining cases, changes in either the steady-state or kinetic properties of activation and/or inactivation alters the interrelationship between these curves. This determines the size of I Na-L whether in the form of a prolonged opening of Na+ channels or a re-opening of previously inactivated channels [58]. In situations in which there are overlap regions in the steady-state activation and inactivation functions, an experimental situation involving the imposition of voltage clamp steps would demonstrate a persistent steady-state equilibrium, window current [48, 54]. Similar overlaps could occur prior to achievement of a steady state. These would particularly arise from the kinetics of either activation or inactivation that would remain amenable to the graphical analysis adopted here.
Nevertheless, the relatively rapid kinetics of Na+ channel activation over timescales substantially preceding recovery processes related to I Na-L permit its approximation by its steady-state activation curve properties. A number of activation curve variants could then potentially influence the existence or magnitude of I Na-L. Of these, negative shifts in the voltage dependence of activation quantified by negative changes in V act have been reported with genetic modification in either the Nav1.5 α- or β-subunits [27]. Alternatively, this negative change could occur in situations shifting the electric field seen by the voltage sensor for activation with reductions in external or increases in internal Ca2+ or Mg2+ concentration (Fig. 5c) [52, 73, 75]. These would shift the foot of the activation voltage curve closer to the threshold voltage and increase the likelihood of re-activation phenomena. In addition, an increased steepness in the activation curve (Fig. 5d) quantified by a decrease in k act and therefore an increase in the effective valency z could arise in mutations affecting the charge on the voltage sensor controlling Na+ channel gating.
I Na-L and altered gNa inactivation
Figure 6a illustrates both steady state and a family of curves (dotted lines) representing the kinetics of inactivation following a depolarizing voltage step, which explores the development of inactivation independently of its recovery. Both positive shifts, with increased V inact (Fig. 6b) or a decreased steepness with increased k inact, of steady-state inactivation (Fig. 6c), could increase overlap between steady-state activation and inactivation, accentuating I Na-L through an increased window current. In addition, alterations in inactivation kinetics could take place incidental to such shifts in steady-state inactivation or in a presence of otherwise normal steady-state properties. A slowing of the kinetics even in the absence of any steady-state abnormality (Fig. 6d) could result in a further mechanism of increasing I Na-L manifested in bursting phenomena. Bursting reflects a transient kinetic failure of Na + channel inactivation. The resulting gating mode is associated with a small proportion of the channels alternating between the last closed available state and open state (Fig. 1), and these frequent openings could give rise to I Na-L [18, 79].
Finally, voltage steps restoring the resting membrane potential drive Na+ channel recovery from inactivation over a refractory period (Fig. 7a). As in the case of inactivation, recovery kinetics can similarly follow altered (Fig. 7b) or take place in the presence of normal steady-state voltage dependencies of inactivation (Fig. 7c). This can increase I Na-L by a non-equilibrium gating process. The latter could cause channel re-opening due to a decreased recovery time from inactivation during the terminal repolarisation phase of the AP. This re-opening could take place beyond the overlap region between steady-state activation and inactivation curves. Thus, rapid recovery of a small subpopulation of the channels from inactivation permits their immediate re-activation [19]. Even following full restoration of the resting membrane at the end of the step, the examples in Fig. 7b, c may show similarly altered recovery kinetics. Such altered kinetics might reflect shifted steady-state inactivation curves, which would corespondingly shift rate constants involving inactivation or recovery from inactivation along the voltage axis. They could also result from alterations in the rate constants themselves. Either would alter rates of recovery from inactivation at a given voltage.
I Na-L and clinical genetic arrhythmic conditions
The previous sections thus suggest a hypothesis invoking a convergence of a range of Na+ channel activation and inactivation abnormalities, all of which produce I Na-L. Table 1 summarises a selection of experimental studies using expression systems of a range of inherited clinical mutations in human SCN5A, all of which have been associated with increased I Na-L. It confirms that each mutation results in characteristics illustrating one or more of all the biophysical examples discussed above as illustrated by Figs. 5, 6 and 7. Conversely, the mutations in the table cover all these biophysical cases when taken together. Thus, an enhanced I Na-L can result from a large variety of abnormalities in Na+ channel gating.
In particular, Table 1 illustrates the above points in detail for long QT syndrome type 3 (LQTS3) using the relatively large number of examples from which selections can be made for analysis [33, 49, 55, 61, 65, 72, 85]. LQTS3 is one of a range of genetic (LQTS1–LQTS13) long QT syndromes characterised by prolonged QT intervals, reflecting increased ventricular APD and additional aberrant T-wave ECG signatures. They are all associated with a predisposition to normally self-terminating episodic polymorphic ventricular tachycardia (VT), torsades de pointes (TdP), with the potential to degenerate into ventricular fibrillation and/or SCD [2]. LQTS3 patients commonly exhibit bradycardia, and they show a greater risk of arrhythmia at lower heart rates, such as during rest and sleep [64]. The most common mechanism of LQTS3 pathophysiology is the disruption of the fast inactivation kinetics of the channel, enhancing I Na-L [30]. However, the list of mutations in Table 1 suggests that each hypothetical alteration in activation and inactivation properties proposed above is associated with a particular case of LQTS3. The one exception concerns situations resulting in an increased steepness of the activation-voltage relationship and a consequent decrease in k act. Nevertheless, the latter phenotype was represented in the particular, R225P and R814W, mutations. These are associated with complex arrhythmias combined with dilated cardiomyopathy. They showed an increased voltage sensitivity of the Na+ channel. This took the form of a decrease in k act without any change in the inactivation curve [53].
Conversely, a given I Na-L phenotype could be associated with a wide range of clinical manifestations in different patients. In addition to LQTS3, these include sudden infant death syndrome (SIDS), multifocal ectopic Purkinje-related premature contractions (MEPPC) and atrial fibrillation (AF). SIDS is a significant cause of infant mortality, and arrhythmias are an important cause of SIDS, with inherited LQTS making up 9.5% of SIDS cases [6]. The S1333Y mutation in Table 1 associated with SIDS involves the domain III S4–S5 linker near the proposed docking site of regions implicated in channel inactivation. The mutant channel showed enhanced window and persistent inward currents, producing a LQTS3-like phenotype [34]. This mutation led to changes in both activation and inactivation processes that taken together would tend to increase I Na-L. Thus, the S1333Y mutation resulted in an increased maximum g Na, a negatively shifted V act but a positively shifted V inact. There was also a more rapid recovery from inactivation. However, there does exist a A1330P mutation that has similar ionic channel effects and also causes SIDS, yet does not produce enhanced I Na-L [34].
The autosomal dominant MEPPC syndrome is associated with an arrhythmia characterised by premature ventricular contractions that originate from ectopic foci along the fascicular-Purkinje system. This results in non-sustained VT and, depending on its severity, SCD [47]. A consistently observed window current may increase the excitability of the fascicular-Purkinje system [47]. Table 1 exemplifies one particular R222Q mutation, which clearly co-segregated with the MEPPC phenotype. This was uniformly present in three unrelated families, and dilated cardiomyopathy appeared as a secondary consequence. The triggered APs and premature ventricular contractions were attributed to altered voltage dependencies of Nav1.5 activation. They were absent at higher pacing frequencies, consistent with their disappearance during exercise [43]. Accordingly, as shown in Table 1, this MEPPC mutation resulted in a negatively shifted V act.
AF is an abnormal heart rhythm manifesting as rapid, irregular beating and palpitations; dyspnoea; dizziness; and chest pain [41, 55]. The gain-of-function K1493R mutation associated with AF showed a positively shifted V inact that would increase the window current and reduce the excitation threshold and a slowed kinetics for inactivation [46]. However, mutations in genes other than SCN5A have also been associated with AF, including SCN10A and SCN1B. SCN10A encodes the voltage-gated Nav1.8 known to be highly expressed in intracardiac neurons [84]. Its role is not fully understood but mutations in it are associated with disease phenotypes. Thus, the A1073 variant increases risks of AF consistent with functional studies, demonstrating increased peak I Na, increased I Na-L and prolonged fast inactivation [35]. Although peak Nav1.8 current is much smaller than peak Nav1.5 current, I Na-L arising from Nav1.8 is 20–50 times higher than I Na-L arising from Nav1.5. Therefore, Nav1.8-mediated I Na-L could strongly influence APD [35]. Finally, a given I Na-L phenotype could be associated with more than one clinical manifestation. Thus, a negatively shifted V act arising from three different mutations, P1332L, p.R222Q and p.I141V, gave LQTS3, MEPPC and exercise-induced polymorphic arrhythmia, respectively [43, 65, 77].
I Na-L as a pharmacological target
Increased I Na-L thus potentially triggers and provides substrate for arrhythmia under diverse circumstances. The analysis above would indicate that potential therapeutic candidates should target I Na-L through their action on the steady-state voltage dependence of Na+ channel activation and/or inactivation and their kinetic properties. This would require such action to take directions and extents appropriate to minimizing I Na-L in the particular condition concerned. Such an action could be further enhanced if the applied agent selectively acted upon I Na-L as opposed to peak I Na.
This strategy is exemplified by recent explorations directed at paramyotonia congenita in skeletal muscle. For example, the anticonvulsant lamotrigine negatively shifted the inactivation V 1/2, modifying inactivation kinetics and decreasing I Na, in a HEK293 expression system expressing Nav1.4 [56]. Rufinamide positively shifted the voltage dependence of I Na activation in human Nav1.1 transiently expressed in Xenopus oocytes [24]. Both lamotrigine and rufinamide at concentrations appropriate for achieving clinical anticonvulsant activity reduced myotonia in isolated human and rat skeletal muscle [74]. This could provide a model for selective therapeutic modifications of activation and inactivation in the cardiac Nav1.5 channel. These could be targeted at patients with particular specific genetic mutations if their underlying electrophysiological abnormalities could be characterised in order to predict their response to these drugs. The latter in turn could prompt clinical trials to assess the efficacy of the resulting I Na-L inhibitors on the arrhythmic variants concerned.
Studies investigating the precise effects of I Na-L inhibitors on the biophysical properties of the Na+ channel could lead to therapy targeted at cardiac arrhythmias associated with increased I Na-L. LQTS patients who responded well to mexiletine carried mutations resulting in a negative shift in V act, whereas patients whose QT intervals were not modified in response to mexiletine did not have a negative shift in V act [65]. This has implications in that it may be necessary to target the specific biophysical alteration in Na+ channel function to effectively inhibit the pro-arrhythmic effects of I Na-L. This would require further investigations of its biophysical actions on mutant Nav1.5. However, mexiletine did not affect voltage-dependent activation but negatively shifted steady-state fast and slow inactivation and markedly prolonged recovery from inactivation of Nav1.5. These actions culminated in a use-dependent I Na block in expressed WT Na+ channels [86]. Nevertheless, mexiletine rescued negatively shifted steady-state activation voltage dependencies in SCN7A-L858F-mutated channels [20].
Recent reports have shown that ranolazine was 9 to 45 times more selective in inhibiting I Na-L than peak I Na in isolated canine ventricular myocytes [82]. It decreased QTc interval in a group of eight LQTS3 patients carrying SCN5A-D1790G. The blocking effect of ranolazine on I Na-L was recapitulated in a TSA201 expression system [16]. Meta-analysis showed that ranolazine significantly reduced incidences of AF relative to control groups in various clinical settings [26, 66]. The trial compound GS-458967 similarly appeared to inhibit I Na-L in preference to peak I Na particularly in the atria as opposed to the ventricles [11]. The further agent vernakalant (RSD1235) did not show selectivity for I Na-L over peak I Na [60].
Conclusions
Sodium currents (I Na) are strategic to cardiac excitation and are mediated by one or more Na+ channel components, reflecting different states in the cardiac Nav1.5 or Na+ channel species that together culminate in peak I Na and late I Na-L components. Accordingly, inherited Nav1.5 abnormalities can disrupt AP generation, propagation and recovery to cause arrhythmia. In particular, an increased I Na-L leads to a variety of arrhythmic conditions and can develop from various biophysical alterations in the overall activation and inactivation gating properties of Nav1.5. Firstly, an increased overlap between the steady-state activation and inactivation functions can increase window current. Secondly, a transient kinetic failure of Na+ channel inactivation can lead to bursting phenomena, characterised by frequent channel openings. Finally, a non-equilibrium gating process can cause channel re-opening due to a decreased recovery time from inactivation. Available clinical evidence from different pro-arrhythmic Nav1.5 mutations can be used to illustrate each of the wide range of possible mechanisms. These various mechanisms for increasing I Na-L could provide a useful basis for the selection of therapeutic agents for patients with the disease phenotype. Selectively targeting the specific biophysical change underlying the increased I Na-L could improve efficacy and allow mutation-specific therapy. This would require preclinical characterisation of how the drug compounds affect the biophysical properties of the I Na-L. In turn, specifically tailored drug intervention in patients with any given genetic mutation would require characterisation of their underlying electrophysiological abnormalities in order to predict their response to these drugs.
Abbreviations
- A :
-
Arrhenius constant
- AF:
-
Atrial fibrillation
- AP:
-
Action potential
- APD:
-
Action potential duration
- ATX-II:
-
Anemonia sulcata toxin
- AVN:
-
Atrioventricular node
- BrS:
-
Brugada syndrome
- DAD:
-
Delayed afterdepolarisation
- EAD:
-
Early afterdepolarisation
- ECG:
-
Electrocardiographic
- F :
-
Faraday’s constant
- g Na :
-
Sodium conductance
- g Na * :
-
Maximum value of sodium conductance
- I Ca :
-
Calcium current
- IFM:
-
Isoleucine-phenylalanine-methionine
- I K1 :
-
Inward rectifying K+ current
- I Kr :
-
Rapid delayed rectifier K+ current
- I Ks :
-
Slowly activating delayed rectifier K+ current
- I Na :
-
Sodium current
- I Na-L :
-
Late sodium current
- I to :
-
Transient outward K+ current
- k :
-
Boltzmann constant
- k act :
-
Slope factor for activation
- k inact :
-
Slope factor for inactivation
- k mn :
-
Voltage-dependent rate constants
- LQTS3:
-
Long QT syndrome type 3
- MEPPC:
-
Multifocal ectopic Purkinje-related premature contractions
- R :
-
Gas constant
- SAN:
-
Sino-atrial node
- SCD:
-
Sudden cardiac death
- SIDS:
-
Sudden infant death syndrome
- T :
-
Temperature
- TdP:
-
Torsades de pointes
- V :
-
Membrane potential
- V act :
-
Voltage at half-maximum activation
- V inact :
-
Voltage at half-maximum inactivation
- VT:
-
Ventricular tachycardia
- z :
-
Valency
- α h :
-
Time constant for transition into inactivation
- β h :
-
Time constant for recovery from inactivation
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Acknowledgements
KC was funded by the Physiological Society, United Kingdom at the University of Surrey. KJ is funded by the Fundamental Research Grant Scheme (FRGS/2/2014/SKK01/PERDANA/02/1), Ministry of Education, Malaysia, and the Research Support Fund, Faculty of Health and Medical Science, University of Surrey. ML is funded by the British Heart Foundation (PG/14/80/31106, PG/16/67/32340) and Medical Research Council (G10002647). CLHH is funded by the Medical Research Council (MR/M001288/1), Wellcome Trust (105727/Z/14/Z), British Heart Foundation (PG/14/79/31102), the McVeigh Benefaction and SADS UK.
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Chadda, K.R., Jeevaratnam, K., Lei, M. et al. Sodium channel biophysics, late sodium current and genetic arrhythmic syndromes. Pflugers Arch - Eur J Physiol 469, 629–641 (2017). https://doi.org/10.1007/s00424-017-1959-1
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DOI: https://doi.org/10.1007/s00424-017-1959-1