Kir2.1-Nav1.5 Channel Complexes Are Differently Regulated than Kir2.1 and Nav1.5 Channels Alone

Utrilla, Raquel G.; Nieto-Marín, Paloma; Alfayate, Silvia; Tinaquero, David; Matamoros, Marcos; Pérez-Hernández, Marta; Sacristán, Silvia; Ondo, Lorena; Andrés, Raquel; Díez‐Guerra, F. Javier; Tamargo, Juan; Delpón, Eva; Caballero, Ricardo

doi:10.3389/fphys.2017.00903

Cited by 40 publications

(46 citation statements)

References 40 publications

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“…Interestingly, when a Nav1.5 mutant produces a DNE on Nav1.5, this does not necessarily imply that it concomitantly produces a DNE on Kir2.1/2.2 channels (p.D1690N) and vice versa (p.D1816VfsX7). This reinforces the contention that the biology of Nav1.5-Kir2.1 complexes differs somehow from that of each channel alone, even though the anterograde and retrograde trafficking routes of the complexes are similar to those of Nav1.5 channels alone (7).…”

Section: Discussionsupporting

confidence: 81%

“…Therefore, the results would indicate that, at least at some stages (biosynthesis and/or forward and retrograde trafficking), Nav1.5 and Kir2.1 proteins do interact, forming complexes. Indeed, previous results from our group demonstrated that at least a pool of Nav1.5 and Kir2.1 channels form complexes early after their synthesis at the ER (8) and that these complexes, whose cellular biology is regulated differently than that of Nav1.5 and Kir2.1 channels alone (7), exhibit preferential forward trafficking toward the membrane (7,8). Interestingly, when a Nav1.5 mutant produces a DNE on Nav1.5, this does not necessarily imply that it concomitantly produces a DNE on Kir2.1/2.2 channels (p.D1690N) and vice versa (p.D1816VfsX7).…”

Section: Discussionmentioning

confidence: 89%

“…In the 1950s Weidmann (4) established that the encompassed voltage-dependent activity of I Na and I K1 is a major determinant of cardiac excitability and conduction velocity. Furthermore, we demonstrated that the functional expression of Nav1.5 and Kir2.1/Kir2.2 channels is reciprocally regulated (5)(6)(7)(8), a mechanism that probably strengthens control of ventricular excitability.…”

Section: Introductionmentioning

confidence: 74%

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Brugada syndrome trafficking–defective Nav1.5 channels can trap cardiac Kir2.1/2.2 channels

Pérez-Hernández¹,

Matamoros²,

Alfayate³

et al. 2018

JCI Insight

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Cardiac Nav1.5 and Kir2.1-2.3 channels generate Na (INa) and inward rectifier K (IK1) currents, respectively. The functional INa and IK1 interplay is reinforced by the positive and reciprocal modulation between Nav15 and Kir2.1/2.2 channels to strengthen the control of ventricular excitability. Loss-of-function mutations in the SCN5A gene, which encodes Nav1.5 channels, underlie several inherited arrhythmogenic syndromes, including Brugada syndrome (BrS). We investigated whether the presence of BrS-associated mutations alters IK1 density concomitantly with INa density. Results obtained using mouse models of SCN5A haploinsufficiency, and the overexpression of native and mutated Nav1.5 channels in expression systems - rat ventricular cardiomyocytes and human induced pluripotent stem cell-derived cardiomyocytes (hiPSC-CMs) - demonstrated that endoplasmic reticulum (ER) trafficking-defective Nav1.5 channels significantly decreased IK1, since they did not positively modulate Kir2.1/2.2 channels. Moreover, Golgi trafficking-defective Nav1.5 mutants produced a dominant negative effect on Kir2.1/2.2 and thus an additional IK1 reduction. Moreover, ER trafficking-defective Nav1.5 channels can be partially rescued by Kir2.1/2.2 channels through an unconventional secretory route that involves Golgi reassembly stacking proteins (GRASPs). Therefore, cardiac excitability would be greatly affected in subjects harboring Nav1.5 mutations with Golgi trafficking defects, since these mutants can concomitantly trap Kir2.1/2.2 channels, thus unexpectedly decreasing IK1 in addition to INa.

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Section: Discussionsupporting

confidence: 81%

Section: Discussionmentioning

confidence: 89%

Section: Introductionmentioning

confidence: 74%

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Brugada syndrome trafficking–defective Nav1.5 channels can trap cardiac Kir2.1/2.2 channels

Pérez-Hernández¹,

Matamoros²,

Alfayate³

et al. 2018

JCI Insight

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“…However, β1 is not the only interacting subunit and other auxiliary subunits of Nav1.5 (other β subunits and scaffolding proteins) are probably expressed in hSC-CM (Abriel, 2010). Furthermore, even other channels, such as the Kir2.1 K + channel, can form complexes with Nav1.5 (Willis et al, 2015;Utrilla et al, 2017;Ponce-Balbuena et al, 2018). As these subunits and interactions can modulate the response of Nav1.5, the expression of them in hSC-CMs most likely explains the observed difference in I Na kinetics between hSC-CMs and heterologous expressed Nav1.5+β1 (Figure 1).…”

Section: Drugmentioning

confidence: 99%

Pharmacological Profile of the Sodium Current in Human Stem Cell-Derived Cardiomyocytes Compares to Heterologous Nav1.5+β1 Model

et al. 2019

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The cardiac Nav1.5 mediated sodium current (I Na) generates the upstroke of the action potential in atrial and ventricular myocytes. Drugs that modulate this current can therefore be antiarrhythmic or proarrhythmic, which requires preclinical evaluation of their potential drug-induced inhibition or modulation of Nav1.5. Since Nav1.5 assembles with, and is modulated by, the auxiliary β1-subunit, this subunit can also affect the channel's pharmacological response. To investigate this, the effect of known Nav1.5 inhibitors was compared between COS-7 cells expressing Nav1.5 or Nav1.5+β1 using whole-cell voltage clamp experiments. For the open state class Ia blockers ajmaline and quinidine, and class Ic drug flecainide, the affinity did not differ between both models. For class Ib drugs phenytoin and lidocaine, which are inactivated state blockers, the affinity decreased more than a twofold when β1 was present. Thus, β1 did not influence the affinity for the class Ia and Ic compounds but it did so for the class Ib drugs. Human stem cell-derived cardiomyocytes (hSC-CMs) are a promising translational cell source for in vitro models that express a representative repertoire of channels and auxiliary proteins, including β1. Therefore, we subsequently evaluated the same drugs for their response on the I Na in hSC-CMs. Consequently, it was expected and confirmed that the drug response of I Na in hSC-CMs compares best to I Na expressed by Nav1.5+β1.

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“…Since previous studies have shown that Na v 1.5 and K ir 2.1 have a parallelism in expression (Milstein et al, 2012;Utrilla et al, 2017; Ponce-Balbuena et al, 2018), we next explored whether the cell shape and size affect membrane localization and activity of Na v 1.5 channels by immunostaining and electrophysiological analysis, respectively. We found that, unlike K ir 2.1, Na v 1.5 exhibited no preferential localization in the corners versus edges of star-shaped Ex293 cells (Fig.…”

Section: Integrin Engagement Increases I K1 Density In Hek Cellsmentioning

confidence: 99%

Altering integrin engagement regulates membrane localization of Kir2.1 channels

Sengupta

Rothenberg

et al. 2019

Journal of Cell Science

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How ion channels localize and distribute on the cell membrane remains incompletely understood. We show that interventions that vary cell adhesion proteins and cell size also affect the membrane current density of inward-rectifier K + channels (K ir 2.1; encoded by KCNJ2) and profoundly alter the action potential shape of excitable cells. By using micropatterning to manipulate the localization and size of focal adhesions (FAs) in single HEK293 cells engineered to stably express K ir 2.1 channels or in neonatal rat cardiomyocytes, we establish a robust linear correlation between FA coverage and the amplitude of K ir 2.1 current at both the local and whole-cell levels. Confocal microscopy showed that K ir 2.1 channels accumulate in membrane proximal to FAs. Selective pharmacological inhibition of key mediators of protein trafficking and the spatially dependent alterations in the dynamics of K ir 2.1 fluorescent recovery after photobleaching revealed that the K ir 2.1 channels are transported to the cell membrane uniformly, but are preferentially internalized by endocytosis at sites that are distal from FAs. Based on these results, we propose adhesion-regulated membrane localization of ion channels as a fundamental mechanism of controlling cellular electrophysiology via mechanochemical signals, independent of the direct ion channel mechanogating.

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Kir2.1-Nav1.5 Channel Complexes Are Differently Regulated than Kir2.1 and Nav1.5 Channels Alone

Cited by 40 publications

References 40 publications

Brugada syndrome trafficking–defective Nav1.5 channels can trap cardiac Kir2.1/2.2 channels

Brugada syndrome trafficking–defective Nav1.5 channels can trap cardiac Kir2.1/2.2 channels

Pharmacological Profile of the Sodium Current in Human Stem Cell-Derived Cardiomyocytes Compares to Heterologous Nav1.5+β1 Model

Altering integrin engagement regulates membrane localization of Kir2.1 channels

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