Abstract

Atrial fibrillation (AF) associated with fibrosis is characterized by the appearance of interstitial myofibroblasts. These cells are responsible for the uncontrolled deposition of the extracellular matrix, which pathologically separate cardiomyocyte bundles. The enhanced fibrosis is thought to contribute to arrhythmias “indirectly” because a collagenous septum is a passive substrate for propagation, resulting in impulse conduction block and/or zigzag conduction. However, the emerging results demonstrate that myofibroblasts in vitro also promote arrhythmogenesis due to direct implications upon cardiomyocyte electrophysiology. This electrical interference may be considered beneficial as it resolves any conduction blocks; however, the passive properties of myofibroblasts might cause a delay in impulse propagation, thus promoting AF due to discontinuous slow conduction. Moreover, low-polarized myofibroblasts reduce, via cell-density dependence, the fast driving inward current for cardiac impulse conduction, therefore resulting in arrhythmogenic uniformly slow propagation. Critically, the subsequent reduction in cardiomyocytes resting membrane potential in vitro significantly increases the likelihood of ectopic activity. Myofibroblast densities and the degree of coupling at cellular border zones also impact upon this likelihood. By considering future in vivo studies, which identify myofibroblasts “per se” as a novel targets for cardiac arrhythmias, this review aims to describe the implications of noncardiomyocyte view in the context of AF.

1. Introduction

The normal function of the heart is a painstaking cooperation between cardiomyocytes and fibroblasts. It is well known that cardiomyocytes provide the “pumping” function of the organ, whereas fibroblasts are responsible for organizing the cellular scaffold and maintaining the proper 3D-network and thus the normal mechanical function. Moreover, fibroblasts contribute importantly to the uniformity of the excitable substrate and to the continuous and rapid electrical activation of the myocardium. In the healthy normal heart, fibrosis-related arrhythmia is normally absent, which indicates that although fibroblasts outnumber cardiomyocytes roughly three-to-one [1], they do not exert any arrhythmogenic effect. Though there is a general assumption that cardiomyocytes play the crucial role in atrial arrhythmogenesis, little is known regarding an “active” role of the connective tissue in this respect.

A variety of pathological conditions, including pressure overload, volume overload, infarction, and aging [2], induces structural remodelling of the heart leading to heart failure and cardiac arrhythmias. This structural remodelling involves changes in the 3D organization of the heart and is based on complex and diverse responses to injury; as a result, all types of cardiac cells are involved. Histopathologically, cardiac remodelling typically involves changes in myocytes size (hypertrophy), the activation and proliferation of fibroblasts, uncontrolled deposition of the extra cellular matrix (ECM), and cell death [3]. This is in favour of the beginning and perpetuation of supraventricular and ventricular arrhythmias due to the presence of collagenous septa, which physically separate regions of cardiomyocytes, thus inducing structural discontinuities at cellular and tissue levels. This can result in conduction block and zigzag conduction, both of which permit structurally determined reentrant propagation of cardiac impulse.

Functionally, cardiac remodelling leads to mechanical dysfunction which increases the likelihood of life-threatening cardiac arrhythmias [10]. Consequently, arrhythmias arising from structurally remodelled hearts are caused by changes in electrical properties of cardiomyocytes and/or by the remodelling of the ECM.

Electrically, remodelling of cardiomyocytes affects a large number of ion channels, ionic pumps, and proteins [11, 12]. Furthermore, redistribution and regulation of gap junction proteins (connexins) alter the physiological anisotropic ratio, which causes abnormal impulse propagation, thus enabling reentrant electrical activity [13].

2. Role of Myofibroblasts in Perpetual Atrial Fibrillation

Atrial interstitial fibrosis has been shown to increase with age in humans and has been observed in patients with atrial fibrillation (AF) [14, 15], in animal models of aging [16, 17] and in congestive heart failure [18]. Through these studies, it has been shown that atrial fibrosis creates a substrate that promotes AF. Increased collagen deposition has been documented in patients with AF secondary to mitral valve disease versus those in sinus rhythm [19]. Extracellular matrix volume and composition correlate with AF persistence [20]. These findings highlight the association between atrial fibrosis and AF, although determining the causal importance of tissue fibrosis in AF occurrence and persistence remains an important challenge.

AF is also capable of enhancing atrial fibrosis. In human lone AF, it has been shown that long-term assessment of patients diagnosed with AF, which had normal sized atria upon diagnosis, does lead to structural remodeling of the atria causing atrial enlargement and dilatation over a subsequent period of 20 months [21]. The studies suggest that atrial fibrosis acts as both a trigger and a by-product of AF, potentially through a mechanism affecting signaling pathways associated with atrial dilatation [22, 23].

The mechanism of AF that is associated with an increased level of fibrosis is still under debate as both focal and reentrant mechanisms have been observed in patients and animal models of AF. In the dog model of ventricular tachypacing induced congestive heart failure, atrial fibrosis causes localized regions of conduction slowing, increasing conduction heterogeneity and providing an AF substrate [18]. Conduction abnormalities provide a basis for unidirectional conduction block and macroreentry [24].

In contrast, in the study by Stambler et al. on dogs with rapid ventricular pacing-induced congestive heart failure, AF was shown to be focal in origin caused by triggered activity [25]. This triggered activity was shown to be produced by delayed afterdepolarizations initiated by intracellular Ca2+ overload. Drugs that reduced intracellular Ca2+ levels (verapamil, flunarizine, and ryanodine) all terminated AF. Fenelon et al. expanded on this study by performing biatrial mapping in dogs with heart failure and showed that the majority of AF episodes had a focal mechanism [26].

There is evidence that atrial fibrosis is associated with a profound remodelling of the atrial pacemaker complex. It has been shown that the function of the SAN declines in AF [27], heart failure [2830], and with age [31], conditions associated with an increased level of fibrosis. A strong correlation between these conditions and the incidence of sick sinus syndrome has been observed [31, 32]. It should be noted that, histologically, the healthy SAN is distinguished from the surrounding atrial muscle by a remarkably large amount of interstitium (e.g., up to 75%–90% of SAN volume in cat) [33]. It allows SAN electrical insulation from the surrounding atrial myocardium, except for several critical conduction pathways. Indeed, the SAN as a leading pacemaker requires both anatomical (fibrosis, fat, and blood vessels) and/or functional (paucity of connexins) barriers to protect it from the hyperpolarizing influence of the surrounding myocardium [3436]. The presence of conduction barriers and pathways explain how a small cluster of pacemaker cells in the SAN pacemaker complex manages to depolarize widely distributed areas of the right atria. An increased level of interstitial fibrosis can further insulate the SAN thereby altering the delicate balance between depolarized cells (source) and the resting tissue ahead (sink) [37].

On the other hand, an increased fibrosis can unmask the latent pacemakers by forming specialized, isolated clusters of pacemakers located throughout the atrial pacemaker complex [4, 38]. It has been known for over a century that pacemaker cells are widely distributed throughout the entire region located between the superior and inferior vena cava and between the crista terminalis and intra-atrial septum [33, 39]. Canine and human studies [4044] have revealed an extensive distributed system of atrial pacemakers, the atrial pacemaker complex, which extends well beyond the anatomically defined SAN and includes primary and subsidiary pacemakers located within the right atrium. Functional anatomy of the atrial pacemaker complex has been extensively studied in mouse models of sick sinus syndrome. Recently, in calsequestrin 2 null mice which were characterized by an increased susceptibility to AF, we have shown, using a high-resolution optical mapping and 3D atrial immunohistology a selective interstitial fibrosis in the atrial pacemaker complex [4], Figure 1. Deletion of calsequestrin 2 depressed primary SAN activity and conduction, but enhanced atrial ectopic activity and AF associated with macro- and micro-reentry during autonomic stimulation (Figure 2). It depressed primary SAN activity and conduction but enhanced atrial ectopic activity and AF associated with macro- and microreentry during autonomic stimulation (Figure 2). Thus, the latent pacemakers will be more stable compared to the primary pacemaker, SAN, probably due to protective electrical insulation role of fibrosis. Such aberrantly isolated clusters of latent pacemakers could become activated and take over the role of the leading pacemaker which can be exaggerated during the abnormal response to autonomic stimulation.

Similar results have been observed in other genetically engineered mouse models. Deletion of some structural proteins (such as Cx40 [45, 46], ankyrin-B [38], liver kinase B1 (LKB1) [47], natriuretic peptide receptor C [48], or overexpression of tumor necrosis factor- (TNF-) α [49]) has been linked to enhanced fibrosis, depression of the SAN function, and increased atrial arrhythmogenesis. Shift of the leading pacemaker outside of the SAN structure and a beat-to-beat competition between different pacemakers have been revealed in these mouse models and resulted in heart rate irregularities, tachy-brady arrhythmias, and AF. Interestingly, autonomic stimulation [4] or consecutive thermal ablation of such ectopic sites [45] resulted in leading pacemaker shift back to the SAN but at a prolonged intrinsic cycle length.

In addition to the concept that enhanced interstitial fibrosis contributes to cardiac arrhythmias “indirectly” by affecting passive properties of impulse conduction, recent studies demonstrate that at least a paracrine interaction, or likely a direct electrical coupling, exists between the cardiomyocytes and (myo)fibroblasts (MFBs, see paragraphs below). It has been suggested that structural remodelling including fibrosis of the SAN complex could be attributable to abnormal Ca2+ handling in the pacemaker cells [28]. Enhanced diastolic Ca2+ could directly lead to increased fibrosis within the SAN complex as well as in the latent pacemaker areas by favouring downstream activation of apoptosis due to cytosolic Ca2+ overload. In fact, it has been suggested that chronic Ca2+ leak from the sarcoplasmic reticulum can directly stimulate cell damage and fibrogenesis [50]. Increased intracellular [Ca2+] could also stimulate activation of the multifunctional Ca2+/calmodulin-dependent protein kinase II (CaMKII) which in turn promotes myocardial dysfunction [51] and heart failure [52], SAN cell apoptosis, increased fibrosis and alternating atrial arrhythmogenesis [28].

Finally, the emerging results demonstrate that MFBs in vitro also promote cardiac arrhythmogenesis due to direct implications upon cardiomyocyte electrophysiology [9, 53]. When coupled to cardiomyocytes, MFBs have a depolarizing effect on cardiomyocyte resting membrane potential, which can lead to partial or total sodium channel inactivation. Recent studies have indicated that depolarization in the resting membrane potential of fibroblasts is the most critical factor promoting cardiomyocyte early after depolarizations ectopic activity [8, 54].

3. Role of Myofibroblasts in the Heart

Under the pathological conditions like hypertension, fibrosis, and infarction, MFBs appear in the myocardium. These cells have an important role in reparative fibrosis; they share a phenotype with fibroblasts and smooth-muscle cells and were first identified years ago in skin wound tissue [55] and granulation tissue [56]. However, it is not yet known if these cells are resident changed-phenotype-fibroblasts, endothelial-mesenchymal derived cells or from fibrocytes [57, 58]. Their role is merely reparative and they disappear following programmed cell death. Currently, the most reliable marker for MFBs is alpha-smooth-muscle actin (αSMA), which is expressed in smooth-muscle cells but not in fibroblasts. It has also been shown that MFBs participate in the process of reparative fibrosis in the lung [59], liver [60], and pancreas [61], where they produce excessive ECM, a process similar to that of fibrotic heart remodelling. The trigger for recruitments of MFBs to the diseased heart is not fully understood. The local upregulation of cytokines including foremost TGF-B1 seems to play a prominent role. However it has been demonstrated that tissue stiffening following excessive ECM deposition drives transdifferentiation of precursor cells into forming fibrogenic MFBs [62]. Myofibroblasts themselves produce uncontrolled ECM; hence, a vicious circle ensues. It has also been shown that variation in oxygen (O2) concentration plays a key role in the proliferation of cardiac MFBs. Adult mouse cardiac fibroblasts cultured at 21% O2 express de novoαSMA [63]; in contrast the same was observed when human fetal cardiac fibroblasts were exposed to low percentage O2 [64].

4. Electrical Communications between MFBs and Adjacent Parenchymal Cells

MFBs form gap junctions with the resident parenchymal cells and can exist in different organs like skin [65], intestines [66], and bladder walls [67]. In the healthy heart, MFBs are present only in the valve leaflets; postinfarct MFBs appear in large numbers a few days after injury at the site of infarction. These MFBs differ from those in skin wounds as they can persist in the infarct area for 20 years [68, 69] whilst maintaining intimate contact with the surviving cardiomyocytes.

It is assumed that MFBs primarily differentiate from resident fibroblasts. This process is initiated by transforming growth factor β (TGFβ), followed by an activation of several “canonical” cellular pathways (Smad, ERK, P38 kinase, AP-1 but not JNK) [59]. In culture, neonatal rat cardiac fibroblasts undergo transdifferentiation into MFBs. De novo expression of αSMA increases in parallel with the expression of connexin43 (Cx43) [70]; thus, cutback in expression of Cx43 by small interfering RNAs technique significantly inhibits αSMA expression. There is evidence that fibroblasts in the infarct scar tissue express Cx43 and Cx45 [71]. Other investigations have demonstrated that these fibroblasts are in fact (myo) fibroblasts (Figure 4) [72]. However, questions about electrical coupling between MFBs and cardiomyocytes remain unanswered. It is essential to note that it is not yet reported whether MFBs in vivo establish a heterocellular electronic coupling with cardiomyocytes. We have successfully engineered the heterocellular contact in vitro by coculturing neonatal rat cardiomyocytes and MFBs from cardiac origin (Figure 3). As expected [73], these fibroblasts became MFBs when cultured on rigid substrates (glass coverslips). This was confirmed by observed de novo expression of αSMA (Figure 3(a)). We have also demonstrated that in vitro MFBs express gap junction proteins Cx43 and 45 (not Cx40) at MFB-MFB cell-cell contacts and importantly also at MFB-CM cell-cell contacts (Figure 3(c)) [7]. The successful establishment of this heterocellular contact in vitro together with our previous investigations into a variety of histoarchitectures in vivo now allows for the study of two different situations normally encountered in the infarcted heart.

Immunohistochemical images of chronic infarct in rat cardiac tissue (37 weeks) shown in Figure 4 demonstrate that there is an intimate contact between the areas heavy populated with MFBs (αSMA, brown) and the areas of surviving cardiomyocytes (white). We hypothesised that an area of MFBs might (i) interrupt or affect impulse propagation and (ii) induce ectopic activity, due to electrical coupling.

5. Areas of Myofibroblasts Linking Up Separate Bundles of Cardiomyocytes

The general assumption is that cardiac impulse conduction is blocked at site where cardiomyocyte areas are in contact with collagenous septa or with fibrotic tissue (like infarct regions or sutures site follow heart transplantation). This latter case sporadically reports an unexpected synchronization between donor and recipient heart [74]. Because MFBs are present in the fibrotic tissue, we tested this hypothesis, by engineering the situation represented in Figure 4(a) top, in vitro, by seeding cardiomyocytes in a geometrical defined pattern, and interrupted them with an insert of MFBs (Figure 4(a), bottom).

Details of the experiments are represented in Figure 5(a) [6]. Strands were stimulated from the left hand side and the characteristics of impulse propagation were assessed optically after being exposed to a voltage sensitive dye [75]. For the final analysis, we took into consideration only the insert of MFBs without “cardiomyocytes contamination” (Figure 5(a), lower panel). Each photodiode recorded an optical action potential upstroke, which was correlated with the activation time. Whereas activation time was rapid in the cardiomyocyte area, a passive local electrotonic transmission induced a delay of 30 ms across the MFB insert (Figure 5(c)). As shown in Figure 5(d), the delay is strictly related to the length of the insert. Under these experimental conditions MFBs can support impulse propagation up to ~320 μm; at lengths greater than this, propagation invariably failed. These experiments demonstrate that the heterocellular electrical coupling between the two cell populations can reinstate conduction across an interrupted network of cardiomyocytes resulting in a discontinuity of propagation. In consequence, one has to take into consideration that patchy fibrosis as encountered in the remodelled atria (i.e., ageing) [76] may alter the normal pattern of propagation by inducing discontinuous slow conduction, playing a key role in the context of reentrant circuits.

6. Myofibroblasts Overlaid as to Completely Cover an Area of Cardiomyocytes

To further investigate any direct electrical coupling consequences, MFBs were also cultured in order to overlay the cardiomyocytes. In Figure 4(b), the situation is such that the fibrotic area is heavily populated with MFBs, which infiltrate and diffuse throughout the area of cardiomyocytes, thus increasing the heterotissue interaction (as compared with Figure 4(a)). Due to the depolarized resting membrane potential of MFBs [7], we hypothesized that these circumstances, together with the increased electrical cell-to-cell interaction area, might produce a large depolarized region which can affect local impulse propagation. This, in turn, might reduce the conduction velocity for the cardiac tissue, which is in contact with MFBs. Utilising the same pattern growth technique we engineered 80 μm wide strands of neonatal rat ventricular cardiomyocytes, to which a layer of MFBs is seeded on top of [7] (Figure 4(b), bottom). The conduction velocity () in control preparations, which are virtually devoid of MFBs, is high (~43 cm/s, Figure 6(a), left). However, the presence of MFBs drastically reduces by up to 25 cm/s (Figure 6(a), right). An overall analysis of dependence on MFB coverage area is represented in Figure 6(b) left; denotes biphasic behaviour towards the number of MFBs per measured area. This behaviour is highly reminiscent of the phenomena of supernormal conduction in cardiac tissue investigated both in vivo [77] and in vitro [78]. Both demonstrated that is biphasically dependent on the gradual increment of extracellular potassium concentration. Similar, but in a MFBs density-dependent manner, our results show a similar behaviour, suggesting that MFBs may directly depolarize cardiomyocytes resembling the well-known depolarizing effect of . This hypothesis was proved by conventional intracellular microelectrode techniques for measuring diastolic resting membrane potential (). We found that MFBs gradually depolarized cardiomyocytes in a density-dependent manner (Figure 6(b), right) where recorded dropped from ~−80 mV at a MFB density less than 5% to ~−55 mV when more than 40% of the cardiomyocytes area is covered by MFBs. This data propose that, assuming the same effect in vivo at the epicardial border zone where the minimal wall thickness is comparable to a two-dimensional layer, infiltrated laminae of MFBs might induce epicardium slow conduction velocity. In contrast, in a 3D architecture (ventricular wall) the coupling of cardiomyocytes bordering infarct area might counterbalance this depolarizing effect. The consequences in the context of AF are clear: MFBs can directly depolarize the surrounding cardiomyocytes tissue and thus lead to local conduction slowing and enhance the likelihood of arrhythmia (cf. paragraph below).

7. Myofibroblasts Induce Ectopic Activity in Cardiac Tissue

The last part of the study sought to investigate the intimate contact between cardiomyocytes and MFBs (Figure 4(b), right) and how ectopic electrical activity was elicited following heterocellular coupling [8]. An in vitro fibrotic situation was created by coating strands of neonatal rat ventricular myocytes with increasing densities of MFBs (Figure 7). Spontaneous electrical activities were recorded for 4 seconds. The overview of preparation in Figure 7(a) corresponds to a single frame taken from such recording. In this point in time the quasicompletely coverage of MFB elicits spontaneous activity in two strands; the recording shows action potentials occurred regularly with a frequency of 75 bpm. Crucially, the presence of spontaneous activity is strictly proportional to MFBs densities (Figure 7, top). When MFB coverage was below 16% all the preparations were invariably quiescent; however, when coverage was above ~80%, all preparations exhibited spontaneous activity. In contrast, we found beat frequency reduced from ~80 bpm (20% MFBs density) to ~40 bpm (60% MFBs density) due to progressive reduction in the diastolic membrane potential (Figure 6(b)). A comparison of cardiac membrane potential between isolated cardiomyocytes and heterocellular strands is demonstrated in Figure 7(b), right. Gradual reduction of resting in single cardiomyocytes was examined using a patch clamp technique. Stepwise depolarization during injection of 30 sec long current pulses exhibits electrical spontaneous activity elicited at membrane potential less negative than −67 mV. These results were similar to those found in the heterocellular strands where spontaneous impulse initiation was induced with a minimal density of MFBs corresponding to ~−66 mV. These findings indicate that the heterocellular coupling between MFBs and cardiomyocytes might structurally form an ectopic focus. The firing area is preferentially generated from MFBs and not from the injured cardiomyocytes. In our experiments, the cardiac network appears healthy but ectopic activity could be as well induced.

8. Is the Myofibroblast a Possible Target for Atrial Fibrillation?

Recently we have investigated the possibility to target MFB in order to suppress electrical disorders in the heart. Thanks to the collaboration with Professor Gorelik and Professor Williamson at Imperial College London, we have discovered that MFBs transiently appear during heart development and they can be responsible for fetal arrhythmias [79]. Clinically, it has been associated with a pregnant disease called intrahepatic cholestasis and the prognosis ameliorates after administration of ursodeoxycholic acid (UDCA). Because MFBs tend to depolarize the coupled cardiomyocytes, we sought to investigate whether UDCA may directly target MFBs. We found that UDCA hyperpolarizes MFB membrane potential by targeting the sulphonylurea receptor of   channel [9], reestablishing the normal conduction velocity and terminating reentrant arrhythmia (Figure 8). A double-blind randomized placebo-controlled crossover trial is under investigation by administering UDCA in patient with chronic heart failure [80].

9. Outlook

Electrical communication between the stromal and parenchyma tissue has been the focus of much research over the last 50 years. Certain “myths,” like that we are using a total of 10% of our brain, have been dispelled, including the discovery that indeed only 10% of the human brain is made of neurons, with the rest comprised of “Glia,” identified as stromal “glue” or nerve “putty,” which merely fills the spaces within the parenchyma tissue. In the last two decades researchers have shown that Glia cells express gap junctions and interact directly with neurons [81, 82]. In vitro, stromal cardiac MFBs are electrically and mechanically coupled with cardiomyocytes and this pairing disturbs the electrical homeostasis of the parenchymal cardiac tissue [83, 84]. If the same situation in pathological cardiac tissue will be observed in vivo, MFBs could be considered as a new cellular target for cardiac arrhythmia (Figure 9). Strategies might focus on (i) inducing the MFBs “inactive” (overturn the phenotype back to fibroblast and thus circumvent the electrical coupling) or (ii) targeting these cells, pharmacologically or genetically, for radically hyperpolarization [9, 85]. Evidence obtained so far requires further characterization in order to fully understand the impact(s) of heterocellular interactions upon the complex 3D remodelling of the cytoarchitecture, which occurs during heart failure.

Interestingly, there is speculation that MFBs might appear transiently during heart development and follow the partial state of fetal hypoxia [64] and in the aged heart [76, 86]. Additional studies are necessary to understand if MFBs are not only proarrhythmogenic in heart failure but also during heart development and aging; these are frequently subjected to other pathological “MFB-triggering” situations (diabetes, autoimmune disorder, and metabolic diseases).

Problems regarding engraftment for tissue regeneration have also been investigated and reveal that if other cells, less polarised than cardiomyocytes, were to form gap junctions with cardiomyocytes, spontaneous activity could be induced [87]. This was highlighted by our study where coating cardiomyocytes with Cx43-transfected-HeLa cells ([8], data not shown) give rise to spontaneous activity. Further studies are necessary in order to understand and predict an accurate arrhythmogenic mechanism following cell engraftment in heart failure models using possibly or conductive patches [88], embryonic cardiomyocytes [89], and progenitor stem cells [90]. Regarding the cell therapy, it is also unclear whether engraftment will perturb the electrical homeostasis of cardiac tissue due to an intrinsic resting membrane potential, and there exists the possibility that the engrafted cells might electrically couple with MFBs. Both of these may cause the regenerated cardiac tissue engraftment to become an unexpected source of arrhythmia.

Conflict of Interests

The authors declare that there is no conflict of interests regarding the publication of this paper.

Acknowledgments

This work is funded by Young Research Grant GR-2009.1530528, Italian Ministry of Health, to Michele Miragoli and Flagship Project Nanomax, (miRNano), Italian National Research Council, to Michele Miragoli.