[Frontiers in Bioscience S4, 532-546, January 1, 2012]
Regulation of cardiac excitability by protein kinase C isozymes
Julio Cesar Batista Ferreira1,2, Daria Mochly-Rosen1, Mohamed Boutjdir3
1
TABLE OF CONTENTS
1. ABSTRACT
Cardiac excitability and electrical activity are determined by the sum of individual ion channels, gap junctions and exchanger activities. Electrophysiological remodeling during heart disease involves changes in membrane properties of cardiomyocytes and is related to higher prevalence of arrhythmia-associated morbidity and mortality. Pharmacological and genetic manipulation of cardiac cells as well as animal models of cardiovascular diseases are used to identity changes in electrophysiological properties and the molecular mechanisms associated with the disease. Protein kinase C (PKC) and several other kinases play a pivotal role in cardiac electrophysiological remodeling. Therefore, identifying specific therapies that regulate these kinases is the main focus of current research. PKC, a family of serine/threonine kinases, has been implicated as potential signaling nodes associated with biochemical and biophysical stress in cardiovascular diseases. In this review, we describe the role of PKC isozymes that are involved in cardiac excitability and discuss both genetic and pharmacological tools that were used, their attributes and limitations. Selective and effective pharmacological interventions to normalize cardiac electrical activities and correct cardiac arrhythmias will be of great clinical benefit.
2. INTRODUCTION
The final common pathway of electrical excitability in the heart is the generation of conducted action potentials, whereas voltage-gated ion channels and gap junctions play an important role in the action potential electrogenesis (1, 2). Cardiovascular diseases (i.e. coronary artery disease, stroke and heart failure) are associated with changes of cardiac electrical excitability due to transcriptional and post-translational modifications of ion channels and gap junction proteins (3, 4).
Conceptual and technical breakthroughs during the last decade have led to revolutionary advances in our knowledge of allosteric regulation of ion channels, whereas several studies have focused on identifying cellular nodes where signals converge and serve as multi-effector brakes to re-establish the normal electrophysiological properties inside the damaged heart. Nowadays, there is abundant evidence showing that channel phosphorylation can influence profoundly the electrical properties of cardiomyocytes and other cells (5, 6), whereas various kinases have been described as candidate mediators of the pathological cardiac electrophysiological remodeling (6-8). Among different kinases, activation of PKC isozymes has been a subject of great attention in the cardiovascular field since it is implicated in pathological settings such as heart failure (9, 10), ischemia (11, 12) and ischemic preconditioning (13-15).
We first demonstrated the relevance of PKC isozymes to cardiac excitability by showing that prolonged exposure of isolated neonatal cardiomyocytes to 4-beta phorbol ester 12-myristate-13-acetate (PMA, 1-100nM, a non-selective PKC activator) enhanced the rate of contraction in a dose-dependent fashion (16). Indeed, several studies have reported the contribution of specific PKC isozymes to cardiac excitability by regulating ion channel expression (17-19) and activity (20-22), and inotropic and chronotropic effects (23). In this review, we focus on insights gained from the rational design of small molecule inhibitors and activators of selective PKC isozymes to understand their critical role in modulating cardiac excitability (Figure 1).
2.1. PKC family
PKC is a group of ten closely related phospholipid-dependent serine-threonine protein kinases (24). These isozymes are classified based on their structure and activation requirements into three subgroups: conventional PKCs (alpha, betaI, betaII and gamma), which are Ca-dependent and activated by diacylglycerol (DAG) and phosphatidylserine (PS); novel PKCs (epsilon, delta, eta and theta), which are Ca-independent but activated by DAG and PS; and atypical PKCs (zeta and iota/lambda), which are Ca and DAG-independent but activated by PS.
Of these PKC isozymes, alpha, betaI, betaII, epsilon, theta, lambda, delta, zeta and gamma PKC have been found in the heart in different animal species (25, 26), and high levels of PKC isozymes alpha, betaI, betaII, delta and epsilon have been reported in tsA201 and HL-1 cell lines (27). The presence of multiple PKC isozymes in the same tissue and even in the same cell type suggests that individual isozymes mediate distinct cellular functions. The effort to dissect the roles of individual PKC isozymes in cell functions has been hampered by the lack of isozyme-specific activators and inhibitors.
2.2. General PKC regulators (non-isozyme selective)
A number of small molecule drugs that regulate PKC isozymes have been generated over the last decades. Many of these compounds are competitive inhibitors of ATP binding to the catalytic site of the kinase (Table 1). However, because the catalytic site within the PKC family as well as in other protein kinases is highly conserved, generating a truly selective inhibitor of one protein kinase has proven to be a challenge (28)(Table 1). Small molecule activators of PKC isozymes are also available. Those compounds mimic the second messenger DAG and are related to the tumor promoter phorbol ester, PMA (29), to bryostatin (30) and some other natural compounds. Some activators have higher affinity for one specific PKC subgroup over others in a dose-dependent manner (16). However, considering that these compounds are not able to distinguish the activation of PKC isozymes in the same subgroup, they are usually described as non-selective PKC activators. Furthermore, because there are multiple diacylglycerol-binding proteins (31), using them as PKC isozyme selective tools works only in a narrow concentration range and can activate proteins other than PKCs.
2.3. Isozyme-selective PKC regulators
Over twenty years ago, we suggested that protein-protein interactions play a critical role in determining the selectivity of individual PKC isozymes. We identified a family of proteins, collectively termed RACKs (Receptors for Activated C Kinase) that anchor individual activated PKC isozymes near their substrates and away from others (32). We then designed peptide regulators of these protein-protein interactions as isozyme-selective inhibitors (Figure 2). The rationale used for the design of the peptides and the data used to demonstrate their selectivity was provided in over 200 publications from a variety of labs. For recent review see (33). In short, the peptides, 6-10 amino acids in length, correspond to unique sequences within the PKC isozyme-binding site on the RACK or the RACK-binding site on that PKC isozyme. Using this approach, we have identified selective inhibitors for all the PKC isozymes (see Table 1).
Selective 6-10 amino acid-long peptide activators of PKC isozymes were also rationally designed. These peptides are derived from intra-molecular interaction sites within each PKC isozyme (34). Each peptide activator interferes with an isozyme-specific (or sub-family-specific) inhibitory intra-molecular interaction within that PKC; each peptide is identical in sequence to one of the two intra-molecular interaction sites. By acting as a competitive inhibitor of the inhibitory intra-molecular interactions, the peptide acts as a selective activator of that isozyme. The intra-molecular interaction that we focused on is the pseudo-RACK site, the site that covers the RACK-binding site when PKC is inactive. Peptides derived from the pseudo-RACK binding site are selective activators of the corresponding PKC. Using this approach, we have identified a selective activator for all the conventional PKC isozymes, pseudo-beta RACK, and isozyme-selective activators for delta, epsilon, eta and theta PKCs (see Table 1).
Peptides that act intracellularly need to be conjugated to carrier peptides to deliver them across biological membranes. A number of such short peptide carriers were identified. We used mainly TAT47-57 (35). All the peptide regulators of PKC conjugated to such peptide carriers showed high selectivity for the corresponding isozyme. They were efficacious in vitro and in vivo at low nanomolar concentrations and were well-tolerated when acutely injected intravenously, intraperitoneally, and subcutaneously. They were also effective when delivered in a sustained fashion, using subcutaneous Alzet pumps to obtain weeks of constant delivery (3-10mg/kg/day).
3. PKC AND Ca CHANNELS
Ca channels consist of a central alpha1 subunit, which forms the ion-conducting pore, and the auxiliary subunits alpha2-delta, beta and gamma, which modulate surface expression and biophysical properties. In the sarcolemma of cardiac cells, two types of Ca channels have been identified: the high-voltage, L-type Ca channel, and the low-voltage, T-type Ca channel (2). They play an important role in normal and diseased myocytes (1).
3.1. L-type Ca channels
The influx of Ca through L-type Ca channels plays an essential role in both cardiac excitability and excitation-contraction coupling. The depolarizing current through L-type Ca channels contributes to the cardiac action potential plateau and to Ca-induced Ca release from the sarcoplasmic reticulum. Four genes encode L-type Ca channel alpha1 subunits in mammals: Cav1.2 (alpha1C), Cav1.3 (alpha1D), Cav1.1 (alpha1S) and Cav1.4 (alpha1F) (36). Alpha1S and alpha1F expression is restricted to the skeletal muscle and the retina. Alpha1C is assumed to be the most abundant isoform in the cardiovascular system, whereas alpha1D is expressed in neurons and neuroendocrine cells (1, 37). It is therefore believed that the contribution of L-type Ca currents to the physiology/pathophysiology of the heart and the therapeutic effects of Ca channel antagonists are mainly mediated through alpha1C Ca channels. This assumption has been challenged by recent findings that alpha1D knockout mice unexpectedly exhibited intrinsic sino-atrial dysfunction and predisposition to atrial fibrillation (38-40), suggesting an important functional role for the alpha1D Ca channel in the supraventricular tissue.
Multiple G protein-coupled receptors in the heart act through phospholipase C-dependent hydrolysis of membrane phosphoinositides to regulate many cellular proteins, including the L-type Ca channels. Early studies suggested that neurohormones (i.e. endothelin-1and angiotensin II) modulate L-type Ca channels in a PKC isozyme-dependent manner. For example, acute endothelin 1 treatment (which activates PKC) resulted in increased, decreased or no change in basal Ca influx in isolated cardiomyocytes under different conditions (41-43).
Disparate results have also been found in studies using non-selective PKC activators. The published work from our group showed that PMA (a non-selective PKC activator) consistently inhibited Ca channels in rat ventricular cells (22, 44). However, PMA has also been reported to inhibit, have no effect, stimulate, or initially stimulate but later inhibit L-type Ca currents in cardiac myocytes (45). Non-selective PKC activators produce inconsistent responses in non-cardiac Ca channels as well. Stimulation of Ca channels by phorbol esters has been reported in Aplysia bag cell neurons (46), neuroblastomas (47), secretory RINm5f cells (48) and frog sympathetic neurons (49). Conversely, inhibition of Ca channels by phorbol esters has been reported in chick DRG cells (50), and PC-12 cells (51). Because specific PKC isozymes contribute to a wide variety of cellular responses and sometimes exert even opposite effects inside the cell, the usage of non-selective PKC activators might provide misleading information on the relative contribution of PKC isozymes to Ca channels. It seems therefore that the outcome of PKC activation is species and tissue-dependent, probably because of the isozyme type present in each cell type.
Over the last decade, the rational design of selective PKC modulators as well as the use of genetic models has contributed to better understanding the role of selective PKC isozymes on both alpha1C and alpha1D L-type Ca channels. The PKC phosphorylation sites of the cardiac alpha1C subunit of the L-type Ca channel have been mapped to threonines 27 and 31 of the N-terminus, in which conversion of the threonines 27 and 31 to alanine abolishes the PKC-mediated inhibition of alpha1C Ca channel current (ICa-L) in tsA-201 cells (52). In parallel, mutating the threonines 27 and 31 to aspartate restored the PKC sensitivity of alpha1C ICa-L, suggesting that change in net charge by phosphorylation of threonines 27 and 31 of the N-terminus is responsible for the alpha1C ICa-L inhibition (52). In order to dissect the role of specific PKC isozymes in the regulation of cardiac Ca channels, we took advantage of PKC-regulating peptides developed by our lab (24, 33). Intracellular delivery of selective epsilon PKC activator peptide (pseudo-epsilon RACK V1-7) resulted in significant inhibition of ICa-L in ventricular myocytes isolated from adult rats (22). The inhibitory effect of pseudo-epsilon RACK V1-7 was completely prevented by the epsilon PKC peptide inhibitor (epsilon V1-2). Because sustained epsilon PKC activation has been associated with cardiac dysfunction and heart failure in different animal models (53-55), we tested whether chronic in vivo modulation of epsilon PKC leads to altered ICa-L. Using transgenic mice with specific cardiac constitutive activation of epsilon PKC (expressing the pseudo-RACK sequence of epsilon PKC, pseudo-epsilon RACK), we found that sustained epsilon PKC resulted in reduced basal ICa-L density as well as blunted the beta-adrenergic activation of ICa-L (56).
Besides the negative effects of epsilon PKC on alpha1C ICa-L by phosphorylating aminoacid residues at N-terminal domain, Yang et al. (2005) have demonstrated in HEK293 cells that alpha, epsilon and zeta PKC isozymes phosphorylated serine 1928 at the C-terminal domain of the alpha1C L-type Ca channel, resulting in increased alpha1C L-type Ca channel activity (57). The serine 1928 phosphorylation has been previously related to up-regulation of alpha1C L-type Ca channel activity in a protein kinase A-dependent manner (58). Furthermore, Yang et al. (2009) have showed in Langendorff-perfused heart that both serines 1674 and 1928 were phosphorylated in response to PMA (non-selective PKC activator) (59). Using GST fusion proteins, the authors provided evidence that alpha, betaI, betaII, gamma and theta PKC isozymes were able to phosphorylate the serine 1674 site in HEK293 cells. Therefore, isolated hearts from transgenic mice over-expressing alpha PKC displayed increased phosphorylation of serine 1674 and 1928 (59). Conversely, alpha PKC knockout mice presented decreased cardiac levels of serines 1674 and 1928 phosphorylation (59). Besides its effect on cardiomyocyte excitability, alpha PKC may affect cardiac excitation-contraction coupling through a negative regulation of sarcoplasmic reticulum Ca load, thereby affecting cardiac performance during cardiac dysfunction and heart failure (60).
Unlike the well-characterized alpha1C L-type Ca channels, alpha1D L-type Ca channels have not been highlighted in earlier studies. We have demonstrated in the tsA201 cell line, using single channel analysis, that PMA (non-selective PKC activator) treatment resulted in a decrease in open probability and increase in closed-time without any significant effect on the conductance of the alpha1D L-type Ca channel (61). More recently, we showed that phosphorylation of serine 81 in the N-terminal region plays a negative role in alpha1D Ca channel activity in tsA201 cell line (62). This response was mediated by non-selective PKC activation. The introduction of a negatively charged residue at position 81, by converting serine to aspartate, mimicked the PKC phosphorylation effect on the alpha1D Ca channel. The modulation of the alpha1D Ca channel by PKC was prevented by dialyzing cells with a 35 amino acid peptide mimicking the alpha1D N-terminal region comprising serine 81. In addition, we evaluated, in the tsA201 cell line, the role of specific PKC isozymes on alpha1D ICa-L by using different PKC isozyme-selective inhibitor peptides. We first demonstrated that betaII V5-3 (selective beta IIPKC inhibitor) and epsilon V1-2 (selective epsilon PKC inhibitor) peptides antagonized the negative effects of PMA on alpha1D ICa-L (62). These results indicate that phosphorylation of serine 81 by betaII PKC and epsilon PKC is required for inhibition of alpha1D Ca channel activity. Parallel to their effects on cardiomyocyte excitability, betaII PKC and epsilon PKC may affect cardiac excitation-contraction coupling through a negative myofilament Ca-sensitivity and cardiac hypertrophy, respectively, thereby affecting cardiac function during ventricular remodeling and heart failure (10, 54, 63).
3.2. T-type Ca channels
Transient low-voltage activated currents (ICaT) characterize T-type channels. They have been identified in the sinoatrial node, AV node, Purkinje system, vascular smooth cells, and in neurons (2, 37). The T-type Ca channel has been involved in pacemaking and in Ca signaling in secretory cells and vascular smooth muscle (37). ICaT has been implicated in triggering Ca release from the sarcoplasmic reticulum (64) and in contraction of Purkinje cells (65). There is evidence indicating that T-type Ca channels also promote cell proliferation and growth (66). In this regard, increased levels of re-expression of T-type Ca channels in certain pathologic states, such as ventricular hypertrophy, have been reported by others (67) and us (68). Only a few studies reported on the interaction of PKC with T-type Ca channels in the heart. Tseng and Boyden (69) demonstrated that PKC activation inhibited ICaT in canine cardiac cells. Similarly, Zhang et al. (2000) showed that indirect activation of PKC by arachidonic acid attenuated the recently cloned human T-type alpha1H current expressed in HEK 293 cells (70). At the molecular level, Cribbs et al. (1998) showed the existence of several PKC consensus motifs on the T-type Ca channel alpha1H subunit (71). Two sites are located on the domain I-II cytoplasmic loop and one site on the domain III-IV connector. Zheng et al. (2010) recently showed that lysophosphatidylcholine up-regulated T-type Ca channels in a PKC-dependent manner (72). However, the identity of the PKC isozyme which regulates T-type Ca channels is not yet known.
Based on the findings described above, we summarize that integration of different regulatory mechanisms controlled by specific PKC isozymes may provide sensitive modulation of Ca channel activity in response to cardiac pathophysiology. In fact, it is possible that different PKC isozymes may have opposing effects on Ca channels, as previously suggested by the effect of PMA on the L-type Ca channel activity. Therefore, considering that Ca channels are the main mediators of Ca influx and are pivotal in cardiac function, further studies clarifying the physiological contribution of PKC isozyme-mediated Ca channel function need to be performed in normal and diseased hearts.
4. PKC AND Nd CHANNELS
Voltage-gated Na channels are the primary channels responsible for the rising phase of the action potential in excitable cells. The regulation of Na channels by PKC has been studied using general PKC activators such as PMA (73) and OAG (1-oleoyl-2-acetyl-sn-glycerol) (74). In general, activation of PKC by these non-isozyme specific activators leads to a reduction in Na current in both brain and heart (75-77). Heterologously expressed rat brain (rBIIA) (73, 77) and human cardiac Na channel currents (hH1) (76) were reduced upon PKC activation. While both rBIIA and hH1 contain consensus sites for phosphorylation by PKC, most of the sites are not conserved between these two isozymes. In one study (76), elimination of conserved consensus PKC sites in the hH1 interdomain III-IV linker, which contains the putative PKC site (Ser1503) does not completely eliminate the PMA-induced Na current inhibition, implying that other phosphorylation site(s) may exist. Considering that Na channels are associated with other proteins forming a multi-protein complex (78), the remaining Na current may be due to PKC regulation of other kinases or phosphatases, and not necessarily to phosphorylation of another Na channel residue.
While these previous studies implicated PKC in the regulation of Na channels, the role and the identity of the isozyme(s) responsible for this regulation remained largely unexplored. Our laboratory has utilized rationally designed PKC modulators to gain insight into the Na channel regulation by PKC. Studies from our lab using Xenopus oocytes showed that the Na current is inhibited by PMA, a general PKC activator. In addition, the use of the peptide specific activator of epsilon PKC, pseudo-epsilon RACK (Table 1, mimicked PMA effects on INa and the use of the peptide specific inhibitor of epsilon PKC, epsilon V1-2 (Table 1), prevented these effects, thus establishing the involvement of at least epsilon PKC in the regulation of Na channels. Similarly, the decrease in the neuronal Nav1.8 peak current induced by PMA was prevented by a specific epsilon PKC isozyme peptide antagonist, whereas the PMA effect on Nav1.7 was prevented by epsilon PKC and betaII PKC peptide inhibitors (79).
Considering that betaII PKC and epsilon PKC are key molecules involved in cardiac hypertrophy, heart failure (for recent review see (24)), and disrupted cardiac excitability (i.e. inhibition of Ca and Na channel currents), it may be possible to consider using betaII PKC and epsilon PKC isozyme-selective inhibitors as therapeutic tools for the treatment of chronic cardiac diseases.
5. PKC AND K CHANNELS
K channels are of importance in determining the shape and mostly the repolarization of the cardiac action potential (80). In cardiac myocytes, at least eleven K currents have been characterized pharmacologically or by molecular cloning. These currents include the inward rectifier K current, IKl; the transient outward K current, Ito; the ultra-rapidly activating delayed rectifier K current, IKur; and the rapidly IKr and slowly IKs activating delayed rectifier K currents (4). In general, the initial and rapid phase (phase 2) of the repolarization is caused by outward K movement (transient outward current, Ito) through rapidly activating and inactivating K channels, and the late phase (phase 3) is under the control of the delayed rectifier current (IK). As such, K currents can modulate the duration of the action potential and refractoriness of the myocardium. It is noteworthy to emphasize that there is considerable heterogeneity in the morphology of action potentials and underlying K currents from various areas of the heart and between species.
The human ether-a-go-go-related gene hERG encodes the voltage-gated K channel underlying IKr, which initiates repolarization and terminates the plateau phase of the action potential (81). Several papers have reported that either alpha-adrenergic or non-selective PKC stimulation by PMA reduces hERG currents in cardiomyocyte (82-85). However, this phenomenon seems to be independent of direct PKC phosphorylation of the channel, since deletion by mutagenesis of PKC-dependent phosphorylation sites in hERG does not abolish PMA-induced effects on the channel (85). The cellular mechanisms of this PKC-mediated are still not completely understood. Of interest, the non-selective PKC inhibitor, BIM-I blocks hERG currents in a PKC-independent manner (86). Thus, PKC-independent effects have to be carefully considered when using non-selective PKC inhibitors in models involving IKr currents. Other K currents such as Ito1, IKl and Kv4.2/Kv4.3 currents are also negatively regulated by non-selective PKC activation in the heart (87), whereas increased epsilon PKC translocation (and not d PKC) indirectly attenuates K currents by suppressing the synthesis of K channel proteins in the heart (88).
IKs channel is encoded by KvLQT1 and minK genes. KvLQT1/MinK channel contributes to the phase 3 slow repolarization of cardiac action potential. PKC has been suggested as a key mediator of KvLQT1/MinK channel regulation. The inhibition of the KvLQT1/MinK channel in ventricular myocytes by angiotensin II occurs in a PKC-dependent manner (89). In contrast, PKC is implicated in KvLQT1/MinK channel activation upon beta-3 adrenergic stimulation in Xenopus oocytes (90). Considering that different PKC isozymes have opposite effects in the cell (91), future studies are required in order to better understand the contribution of specific PKC isozymes in these processes. Mouse and rat IKs currents were decreased by PKC activation (92), whereas guinea pig IKs was activated by PKC (93). These findings suggest that regulation of IKs by PKC is also species dependent. In mouse and rat minK channel, there is a putative PKC phosphorylation site at Ser102. Position Ser102 in the minK protein has been shown to be critical in determining the effect of PKC. Work in our lab has focused on the use of rationally designed small molecules to gain insight into the modulatory actions of PKC on the delayed rectifier, IKs. The data from our lab showed that in Xenopus oocytes, activation of PKC by PMA activates the human cardiac IKs channel and that selective inhibition of betaII PKC, but not betaI PKC (using betaII V5-3 and betaI V5-3, respectively; Table 1) abolishes PMA-induced IKs activation. These findings support the hypothesis of specialized function of only betaII PKC (21). However, additional work is required to better understand the behavior of K channels upon betaII PKC activation during cardiac stress such as ventricular dysfunction and heart failure. In addition, the identification of the particular PKC isozymes that mediate the regulation of K currents is of importance for the understanding of the mechanism of ion channel regulation and the development of new therapeutic agents. Future studies utilizing rationally designed PKC modulators may help to answer this question.
6. PKC AND GAP JUNCTION
In the heart, the gap junction plays an essential role in the electrical cell-to-cell coupling and impulse propagation between cells. Gap junction proteins are encoded by the connexin multigene family, whereas connexin 43 (Cx43) is the most abundant and widespread of the connexins in the heart. Cx43 phosphorylation influences its expression, degradation and functional properties such as conductance and open-probability of channels. Thus, dysfunction of the cardiac gap junction due to Cx43 post-translational changes mainly contributes to ventricular arrhythmia. Over the last decade, PKC-mediated phosphorylation of Cx43 has been reported and associated with both increased (94, 95) and decreased conductance (7, 96). However, the contribution of specific PKC isozymes to this phenomenon remains poorly understood due to the utilization of non-selective PKC isozyme inhibitors.
Among different PKC isozymes, only epsilon PKC and alpha PKC have been described to co-localize with Cx43 in the heart (3, 97, 98). Bowling et al. (2001) showed that both epsilon PKC and alpha PKC co-localize with Cx43 in non-failing and failing hearts, however, only epsilon PKC directly phosphorylates Cx43 (99). Doble et al. (2000) demonstrated that non-specific PKC activation by either fibroblast growth-factor 2 (FGF-2) or PMA increased epsilon PKC but not alpha PKC co-localization with Cx43 in myocytes, resulting in decreased gap junction permeability, whereas chelerythrine treatment (a non-selective PKC inhibitor) blocked the effects of FGF-2 on Cx43 phosphorylation and permeability (7, 13). Furthermore, evidence that the epsilon PKC isozyme is directly involved in Cx43 phosphorylation was provided by showing that over-expression of the mutated dominant-negative form of epsilon PKC decreased myocyte Cx43 phosphorylation and permeability (7, 13). Therefore, Cx43 phosphorylation by epsilon PKC has been associated with decreased gap junctional intercellular communication. Bao et al. (2004) proposed that phosphorylation of Ser-368 by PKC produces a conformational change in the C-terminal domain that leads to a decrease in Cx43 permeability (100).
7. PKC AND Na/Ca EXCHANGER
The cardiac Na/Ca exchanger (NCX) plays a pivotal role in regulating intracellular Ca homeostasis to maintain normal electrical and mechanical activities of the heart. NCX1 is particularly important to excitability because during each action potential, NCX1 rapidly extrudes the Ca which entered the myocytes and brings Ca into the myocytes during cardiac depolarization.
Ruknudin et al. (2007) have shown that NCX is a member of a macromolecular complex that includes different kinases and phosphatases (101). However, the role of protein phosphorylation in the NCX has not been well defined. Iwamoto et al. (1996, 1998) first provided evidence that the cardiac isoform of NCX can be phosphorylated by PKC in CCL39 fibroblasts, resulting in increased NCX activity (102, 103). They found that NCX1 was phosphorylated upon incubation with PMA (non-selective PKC activator). Of interest, when all the consensus sites of the PKC phosphorylation were mutated in the NCX1, the protein still showed response after PMA stimulation (102), suggesting that either PMA stimulation could result in non-specific kinase activation or that there could be nonconsensus sites for PKC on NCX1.
Zhang et al. (2001, 2009) have reported that chelerythrine (a non-selective PKC inhibitor) abolished the deleterious effect of endothelin-1 treatment on NCX1 activity in guinea-pig ventricular myocytes (8, 104). Using an animal model, Katanosaka et al. (2007) showed increased NCX phosphorylation and association of NCX1 with alpha PKC in the hypertrophic hearts of thoracic aortic-banded (TAB) mice (105). Indeed, transgenic mice over-expressing an NCX1 mutation in specific-PKC phosphorylation sites (NCX1-S249A/S250A/S357A) were more resistant to TAB-induced cardiac hypertrophy (105). To date, it is well-established in the literature that NCX level and activity are increased in heart failure as consequence of sarcoplasmic reticulum dysfunction and cytosolic Ca accumulation during diastole (106). Direct PKC-mediated NCX phosphorylation contributes to NCX activation. In fact, cardiac NCX1 was shown to be stimulated by acute treatment with protein kinase C (PKC) activators, such as PMA and Gq-coupled receptor agonists (103, 107). In that sense, the use of rationally designed inhibitor peptides of selective PKC isozymes might contribute to correct NCX hyper activation and improves heart failure prognosis.
Besides its direct effect on NCX activity, PKC indirectly regulates NCX function by phosphorylating phospholemman, a small transmembrane protein which belongs to a family of proteins (FXYD gene family) that bind to and regulate NCX. Many papers have reported that regulation of cardiac contractility and NCX1 activity by phospholemman is critically dependent of its phosphorylation at serines 63 and 68 by PKC in cardiac myocytes (108-110). In fact, overexpression of S68E or S63A mutations in phospholemman inhibited NCX activity. Indeed, NCX1 activity is known to be modulated by alpha-adrenergic stimulation in a PKC-dependent manner (103, 111). NCX1 activity is also regulated by PKA phosphorylation at serine 68.
Phospholemman phosphorylation also regulates the membrane Na/K ATPase (Na/K pump) activity, a vital component for the maintenance of normal electrical activity. Han et al. have demonstrated that non-selective PKC activation (using PMA) increases Na/K pump Vmax (112). Of interest, PKC-associated Na/K pump activation is abrogated in phospholemman deficient mice, providing evidences that PKC regulates Na/K pump by phosphorylating phospholemman (113). Phospholemman phosphorylation at both Ser63 and Ser68 is necessary for completely relieving the phospholemman-induced Na/K pump alteration (114). Considering that NCX and the Na/K pump are found together in a functional complex in cardiac myocytes (115), the contribution of PKC-mediated phospholemman phosphorylation to this complex needs to be better exploited. Therefore, futures studies using rationally designed peptides regulators may help to clarify the contribution of PKC isozymes to direct and indirect NCX and Na/K pump regulation.
8. PKC AND ARRHYTHMIAS
Ischemic heart disease is the leading cause of congestive heart failure and death in the Western world (116). Early reperfusion after coronary occlusion improves cardiac function and reduces infarct size, but it is invariably accompanied by an overload of intracellular Ca that mediates cellular damage, contractile dysfunction (117, 118) and fatal ventricular arrhythmias, such as ventricular fibrillation. Efforts have thus been made to minimize the adverse arrhythmic events related to myocardial ischemia-related reperfusion. While the protective role of epsilon PKC activation in myocardial ischemia-reperfusion injury was extensively characterized regarding the alteration in hemodymamics, cellular damage, and infarction size (119), the potential protective effect of epsilon PKC activation on the fatal ventricular arrhythmia associated with ischemia-reperfusion is just emerging.
We used optical mapping techniques to focus on the potential protective role of epsilon PKC modulation on ischemia-reperfusion arrhythmias in two lines of transgenic mice which moderately over-express the epsilon PKC (termed epsilon PKC agonist mice) activator peptide (pseudo-epsilon RACK, Table 1)(120) resulting in a 20% increase in epsilon PKC activity, and epsilon PKC inhibitor peptide (epsilon V1-2; Table 1) resulting in a 15% inhibition of epsilon PKC activity (termed epsilon PKC antagonist mice) in the heart only (expression of the peptides was restricted to cardiac myocytes) (121). Mice were subjected to 10 min global ischemia and 30 min reperfusion and voltage action potentials and intracellular Ca transients were recorded simultaneously at 37 0C. In the epsilon PKC antagonist group, in which epsilon PKC activity was down-regulated, 10 out of 13 (76.9%) TG mice developed ventricular tachycardia, of which six (46.2%) degenerated into sustained ventricular fibrillation upon reperfusion (121). Interestingly, in epsilon PKC agonist mice, in which the activity of epsilon PKC was up-regulated, no ventricular fibrillation was observed and only 1 out of 12 mice showed only transient ventricular tachycardia during reperfusion. During ischemia and reperfusion, intracellular Ca transient decay was exceedingly slower in the antagonist mice compared to the agonist TG mice. The data showed that moderate in vivo activation of epsilon PKC exerts beneficial anti-arrhythmic effects vis a vis the lethal reperfusion arrhythmias (121). Similarly, in vivo treatment of pigs with the epsilon PKC activator, pseudo-epsilon RACK, early during ischemia completely blocked post-ischemic arrhythmia (122). It is interesting to note that although both delta PKC inhibition (by treatment with deltaV1-1) and epsilon PKC activation (by treatment with pseudo-epsilon RACK) resulted in similar reduction in infarct size in this transient ischemic model in pigs, only epsilon PKC activation prevented post-ischemic arrhythmia (123). These findings have important implications for the development of PKC isozyme targeted therapeutics and subsequently for the treatment of ischemic heart disease. Further studies are required in order to identify the specific targets involved in this anti-arrhythmic PKC-mediated phenomenon.
9. SUMMARY AND PERSPECTIVES
In this review, we describe a continuum of responses emanating from different PKC isozymes that contribute to cardiac excitability. It is clear that PKC isozymes play critical roles in the individual ion channels, gap junction and exchangers, which ultimately interfere in the initiation and propagation of the action potential and thus cardiac excitability (Figure 1). The conflicting data on the role of individual PKC isozymes in the regulation of cardiac excitability may be due not only to the differences between species and tissue distribution, but also to the pharmacological and genetic tools used in the studies. Because PKC isozymes have unique, and sometimes, opposing functions, the use of isozyme-selective tools is critical. Using either genetic manipulation or pharmacological tools able to deliver selective agonist and antagonist peptides for the same PKC isozyme in the heart is particularly useful; it helps to determine the contribution of selective PKC isozyme(s) to cardiac excitability-related processes. Clearly, PKC isozymes are central in regulating the electrical activity of the heart. Using these isozyme-selective inhibitors and activators, we demonstrated a role for specific PKC isozymes in the regulation of Ca, Na and K channels (1-3). It may be possible now to investigate the positive and negative contributions of specific PKC isozymes to action potential electrogenesis and excitation-contraction coupling in different pathological conditions such as ischemia, cardiac dysfunction and heart failure. Therefore, in vivo studies using different animal models will help to point out the relevance of specific PKC isozymes as therapeutic targets for the treatment of electrochemical changes induced by cardiovascular diseases.
10. ACKNOWLEDGEMENTS
The work in the authors' laboratories was supported by NIH (R01-HL-077494) and the Veterans Affairs MERIT grants to MB and by an NIH (HL52141) to DM-R. JCBF holds a post-doctoral fellowship from Fundação de Amparo a Pesquisa do Estado de São Paulo (FAPESP 2009/03143-1). DM-R is the founder and a share holder of KAI Pharmaceuticals, Inc, a company that plans to bring PKC regulators to the clinic. However, none of the work described in this study is based on or supported by the company. JCBF and MB has no disclosure.
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Key Words: Protein Kinase C, Ion Channels, Excitation-Coupling, Arrhythmia, Review
Send correspondence to: Mohamed Boutjdir, Research and Development Office (151), VA New York Harbor Healthcare System, 800 Poly Place, Brooklyn, NY 11209, Tel: 718-630-3645, Fax: 718-630-3796, E-mail:Mohamed.Boutjdir@va.gov