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An LQT2-related mutation in the voltage-sensing domain is involved in switching the gating polarity of hERG

BMC Biology volume 22, Article number: 29 (2024) Cite this article

Abstract

Background

Cyclic Nucleotide-Binding Domain (CNBD)-family channels display distinct voltage-sensing properties despite sharing sequence and structural similarity. For example, the human Ether-a-go-go Related Gene (hERG) channel and the Hyperpolarization-activated Cyclic Nucleotide-gated (HCN) channel share high amino acid sequence similarity and identical domain structures. hERG conducts outward current and is activated by positive membrane potentials (depolarization), whereas HCN conducts inward current and is activated by negative membrane potentials (hyperpolarization). The structural basis for the “opposite” voltage-sensing properties of hERG and HCN remains unknown.

Results

We found the voltage-sensing domain (VSD) involves in modulating the gating polarity of hERG. We identified that a long-QT syndrome type 2-related mutation within the VSD, K525N, mediated an inwardly rectifying non-deactivating current, perturbing the channel closure, but sparing the open state and inactivated state. K525N rescued the current of a non-functional mutation in the pore helix region (F627Y) of hERG. K525N&F627Y switched hERG into a hyperpolarization-activated channel. The reactivated inward current induced by hyperpolarization mediated by K525N&F627Y can be inhibited by E-4031 and dofetilide quite well. Moreover, we report an extracellular interaction between the S1 helix and the S5-P region is crucial for modulating the gating polarity. The alanine substitution of several residues in this region (F431A, C566A, I607A, and Y611A) impaired the inward current of K525N&F627Y.

Conclusions

Our data provide evidence that a potential cooperation mechanism in the extracellular vestibule of the VSD and the PD would determine the gating polarity in hERG.

Background

The human Ether-a-go-go Related Gene channel (hERG) is expressed as the rapidly activating delayed rectifier potassium current (IKr) in cardiac myocytes, and it plays a critical role in the repolarization of the action potential (AP) of ventricular cardiomyocytes [1]. The deficiency of hERG is usually associated with long-QT syndrome type-2 (LQT2), featured by a prolongation of the QT interval of the surface electrocardiogram (ECG) and T-wave abnormalities [2, 3]. hERG is a depolarization-activated potassium channel, characterized by an extremely fast and atypical C-type inactivation [1, 4,5,6]. Channels will conduct potassium when hERG is in an activated state, but will not conduct ions when it is in an inactivated state and a closed state [1, 6]. Because hERG activation is slow relatively than rapid inactivation, its current-voltage (I-V) curve is demonstrated as a bell-shaped relationship [1, 6].

hERG belongs to the cyclic nucleotide-binding domain (CNBD) clade of the voltage-gated potassium channel (Kv) superfamily, which contains hyperpolarization-activated and cyclic nucleotide-gated (HCN) channels as well [7]. Both hERG and HCN channels share a similar architecture with a centrally-located pore flanked by four identical subunits [6, 8, 9]. Each channel is a homotetramer, composed of four subunits. Each subunit consists of 6 transmembrane helices (S1-S6), in which S1-S4 is the voltage-sensing domain (VSD), S5-S6 is the pore domain (PD), and the carboxy-terminal is the cyclic nucleotide-binding domain (CNBD) [6, 8, 9]. The S4-S5 linker determines the coupling between VSD and PD [1, 10, 11]. Upon depolarization, the S4 helix will translate along its axis outwardly and move across the membrane [12,13,14,15]. This gating motion of the four VSDs can drive the conformational changes in the coupling machinery of the S4-S5 linker that opens the channel’s gate eventually [11, 12, 15, 16]. Despite these structural similarities between hERG and HCN channels, hERG is activated by membrane depolarization whereas HCN channels are activated by hyperpolarization [6, 8, 9]. It is a mystery that how channel proteins with such high homology are elicited by completely different membrane voltages (depolarization vs. hyperpolarization) and mediate opposite currents. Since hERG and HCN channels have evolved from the same ancestor [7], it might be reasonable to speculate the structural basis for opposite gating polarity could be subtle and may lie in variations of several amino acid residues. However, the structural basis for the different voltage dependence between hERG and HCN channels is still largely unknown.

The PD of hERG contains all the molecular elements necessary for potassium conduction and for activation and inactivation gating. Activation is classically associated with conformational rearrangements at the inner helix bundle (the activation gate) whereas C-type inactivation involves structural changes at the selectivity filter (the inactivation gate) [1, 11, 17]. The motion of the S4 helix drives the activation gate through the S4-S5 linker at the intracellular surface and modulates the inactivation gate through the S1-S4 near the extracellular surface [15, 18,19,20,21,22,23,24,25]. Converting the depolarization-activated channel of hERG into a hyperpolarization-activated channel can be achieved by mutating a single residue in either the S4-S5 linker [23, 26] or the S6 helix [27]. D540K of hERG is a well-known channel that carries the reactivated inward current induced by hyperpolarization [23, 26]. Proline substitution of V659 (V659P) within the S6 helix of hERG also passes inward non-deactivating current upon hyperpolarization [27]. The conductance-voltage (G-V) relationship of both the D540K and V659P channel exhibits an increased conductance upon hyperpolarization, which is well described by a Boltzmann function with a V1/2 around -100 mV (-117 mV for D540K [26], and -99.7 mV for V659P [27]). For hERG and several other depolarization-activated ion channels [28, 29], the polarity of ion channel gating can be determined by the pore domain as well.

In this study, we found the voltage-sensing domain also plays a critical role in modulating the gating polarity of hERG. An LQT2-related mutant on the S4 helix, K525N [30], mediated an inwardly rectifying non-deactivating current upon hyperpolarization. K525N perturbed pore gate closure and preserved the open and inactivated state. Interestingly, K525N together with either F627Y (K525N&F627Y) or hERG blockers, created a hyperpolarization-activated channel with V1/2 is about -103.2 mV. K525N&F627Y was still inhibited by pore blockers, dofetilide, and E4031. Moreover, we found that a potential extracellular interaction between the S1 helix and the S5-P region is critical for the hyperpolarization-activation channel of K525N&F627Y.

Results

K525N&F627Y is a hyperpolarization-activated channel

We chose to use hERG as a model channel, to explore the role of the voltage-sensing domain in modulating its rectification property. On transfection with hERG cDNA, CHO-K1 cells expressed a large potassium current with biophysical properties reminiscent of the IKr current in cardiomyocytes [6] (Fig. 1a). A slowly activating potassium current developed during depolarizations above -60 mV with maximum at a potential 0 mV in hERG-expressing cells (Fig. 1b). It opens with evident inactivation at more positive potential (Fig. 1a, and b). Analysis of the tail current allowed us to characterize the half-activation voltage (V1/2) which is -18.7 ± 1.1 mV (Fig. 1c, and i). The C-type inactivation gate of hERG contains 626GFG628 motif in the selectivity filter [4, 5]. As one of the key determinants of C-type inactivation, F627 regulates the asymmetrical constricted-like conformation of the selectivity filter [4] (Fig. 1d). The tyrosine substitution of F627 (F627Y) leads to an ion non-conducting channel under physiology solutions (Fig. 1a-e), consistent with previous studies [4, 31,32,33].

Fig. 1
figure 1

K525N&F627Y is a hyperpolarization-activated channel. a Representative currents of WT hERG overexpressed in CHO cells. The step voltage protocol (below) varies from -60 to +60 mV with a holding potential of -90 mV. The green arrow and red arrowhead indicate the measurement region of outward currents and tail currents, respectively. The 0 pA is indicated by a dashed line. b The normalized current-voltage (I-V) curve of WT hERG (n≥6) and F627Y (n≥6). Measured currents are indicated by the green arrow in Fig. 1a. c The normalized conductance-voltage (G-V) curve of WT hERG (n≥6). Measured currents are indicated by the red arrowhead in Fig. 1a. d Diagram of an hERG channel subunit that can be divided into a VSD (S1-S4) and a PD (S5-S6). K525 in the S4 helix and F627 in the selective filter is indicated by a red and purple star, respectively. The potential interacting residues (F431, C566, I607, and Y611) are also labelled with black dots. F431 is in S1, C566 is in S5, I607 and Y611 are in the pore helix. e Representative currents of F627Y. Step voltage protocol (below) varies from -165 to +30 mV with a holding potential at -70 mV. f Representative currents of K525N&F627Y. Step voltage protocol (below) varies from -130 to +30 mV with a holding potential at -70 mV. g The normalized I-V curve (n≥6) and h The normalized G-V curve (n≥6) of K525N&F627Y. i V1/2 values of WT hERG and K525N&F627Y (n=12). Error bars represent mean ± SEM

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We investigated channel properties of many double mutants that combined mutations of gating charge and F627Y (Fig. 1d). To our surprise, the nonfunctional single mutant of F627Y was rescued by the K525N mutation (Fig. 1f). Moreover, K525N&F627Y was activated by membrane hyperpolarization and mediated non-deactivated inward current (Fig. 1f-h, and Additional file 1: Fig. S1), in stark contrast to the wild-type (WT) hERG that was activated by membrane depolarization and conducted outward current (Fig. 1a, and b). Such behavior is reminiscent of the hyperpolarization-induced activation of D540K [23, 26] and V659P [27] of hERG, W434F-P475D of Shaker-IR [34], L226P of NachBac [28], and L271P&D312N of SKOR [29]. We observed K525N&F627Y was completely closed at physiological membrane potentials and began to conduct a slowly activated inward current as the membrane voltage was changed from -70 to -135 mV (Fig. 1f, g, and Additional file 1: Fig. S1). Such activation properties are exactly opposite to those of WT hERG, which was activated by more positive membrane potentials (Figs. 1a, and b; from -60 to +60 mV). The voltage dependence of the peak tail current for K525N&F627Y was fitted to a Boltzmann function, yielding a V1/2 of -103.2 ± 4.1 mV (Fig. 1h, and i), 84.5 mV more negative than that for WT (Fig. 1i). Also, K525N&G628S is a hyperpolarization-activated channel similar with K525N&F627Y (Additional file 1: Fig. S1). The gating polarity of K525N&F627Y and K525N&G628S is reversed to WT hERG (Fig. 1c, h, and Additional file 1: Fig. S1).

Under physiological solutions (external: 5 mM K+ and 140 Na+ versus internal: 145 mM K+), the reversal potential of WT hERG and K525N&F627Y was around -60 mV (Additional file 2: Fig. S2); and it changed to about 0 mV (Additional file 2: Fig. S2) while symmetric potassium solutions were applied (external and internal: 145 mM K+). Therefore, the reversal potential of WT hERG and K525N&F627Y was strictly determined by the potassium gradient between the extracellular (external) solution and intracellular (internal) solution. K525N&F627Y and K525N&G628S remained a potassium channel with a limited permeability to sodium and NMDG (Figs. 2a, and Additional file 2: Fig. S2), which is similar to WT hERG (Fig. 2b).

Fig. 2
figure 2

K525N&F627Y is a K+ selective channel. a Analysis of relative K+ permeability over Na+, or NMDG+ of K525N&F627Y based on Erev measurement (n≥6). b Analysis of relative K+ permeability over Na+, or NMDG+ of WT hERG based on Erev measurement (n≥6). Error bars represent mean ± SEM

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K525N&F627Y is inhibited by hERG channel blockers

hERG channel physiologically conducts ions through the alpha (α) pore [6]. However, the omega (Ω) pore would be created by mutating some gating charges in the S4 of voltage-gated ion channels, especially the first gating charge [35,36,37]. K525S has been reported that it can create an extra Ω pore in hERG [38]. Therefore, a question is raised on whether the hyperpolarization-activated conductance of K525N&F627Y is indeed carried by the hERG channel, and if true, whether it is still carried by the α pore. To address these questions, we first investigated the K525N&F627Y current sensitivity to some hERG channel blockers. Dofetilide and E4031 are both classical blockers through sitting in the central cavity of the α pore [39,40,41]. We found that both dofetilide (Fig. 3a-c) and E4031 (Fig. 3d-f) also significantly inhibited the inward current of K525N&F627Y. The sensitivity of K525N&F627Y to both blocker is dramatically reduced compared with wild-type hERG, which might be attributed to an inability of the open gate to trap blockers in the pore at hyperpolarized potentials [40]. The similar phenomenon was also observed for the D540K mutant [40]. The G-V curve of K525N&F627Y was dramatically left-shifted in the presence of either dofetilide (Fig. 3g-i) or E4031 (Fig. 3j-l). Given that dofetilide and E4031 often act as blocker binding in the α pore [39, 41], and the K525N&F627Y channel shares the same ion selectivity and permeability as the WT hERG channel (Figs. 2, and Additional file 2: Fig. S2), it is reasonable to speculate the inward current of K525N&F627Y is still through the α pore as WT hERG.

Fig. 3
figure 3

K525N&F627Y is inhibited by dofetilide and E4031. a Representative currents of K525N&F627Y with or without 10 μM dofetilide. Inward currents were elicited with -135 mV (the protocol see below). b histogram of I/I0 at -135mV with or without dofetilide (n≥6). c I-V curves of K525N&F627Y with or without dofetilide (n≥6). d Representative currents of K525N&F627Y with or without 3 μM E4031. e histogram of I/I0 at -135mV with or without E4031 (n≥6). f I-V curves of K525N&F627Y with or without E4031 (n≥6). g Representative step currents of K525N&F627Y with or without dofetilide. The step voltage protocol (below) varies from -165 to +30 mV. h The G-V curve (n≥6) and i V1/2 values (n≥6) of K525N&F627Y with or without dofetilide. j Representative step currents of K525N&F627Y with or without E4031. k The G-V curve (n≥6) and l V1/2 values (n≥6) of K525N&F627Y with or without E4031. Error bars represent mean ± SEM. *P<0.05, **P<0.01; ***P<0.001, two-tailed Student’s t-test

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K525N perturbs the channel closed state, presents an open and an inactivated state

To explore the hyperpolarization-activated gating mechanism of K525N&F627Y, we characterized the channel properties of K525N. K525 is proximate to the S3-S4 linker that regulates hERG activation gate [42, 43]. Unlike WT hERG, K525N produced an instantaneous current that was observed upon hyperpolarization as well as depolarization (Fig. 4a, and d). K525N still exhibited properties of a depolarization-activated channel, and tail currents at -150 mV were progressively larger as if the membrane potential was depolarized (Fig. 4a, b, and Additional file 3: Fig. S3). The tail current demonstrated compromised deactivation, and half of the maximum conductance remained at -150 mV (Fig. 4a, and b). K525N can not be fully closed even if the voltage is -170 mV (Fig. 4a, and b). The G-V curve of K525N is dramatically left-shifted compared with WT hERG (Fig. 4b), giving a V1/2 of -95.6 ± 3.9 mV and -19.3 ± 2.1 mV for K525N and WT, respectively (Fig. 4c). An inwardly rectifying current was still detected at more positive potentials (-46.2 ± 3.9 mV) with a maximum current recorded at more negative potentials than WT hERG (6.0 ± 0.8 mV) (Fig. 4d-f). With further depolarization, the current of K525N amplitude decreased progressively (Fig. 4d, and e), which is due to the channel voltage-dependent inactivation. Thus, K525N perturbed channel closure and preserved the channel activation state and inactivation state.

Fig. 4
figure 4

K525N perturbs the channel closure and preserves the open and inactivated state. a Representative step currents of K525N elicited with a complicated protocol. The step voltage protocol (below) varies from -150 to +60 mV with a holding potential of -70 mV. Since channels were instantaneously open at -70 mV, a -170 mV was applied before the step trying to close the pore gate and to detect the activation kinetics. A -150 mV followed the step to detect tail currents. b The G-V curve (n≥6) and c V1/2 of activation values (n≥6) of K525N. d Representative step currents of K525N elicited with an easier protocol. The step voltage protocol (below) varies from -150 to +60 mV. e The G-V curve (n≥6) and f the voltage at the peak current (n≥6) of K525N. Error bars represent mean ± SEM. ***P<0.001, two-tailed Student`s t-test

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The gating polarity of K525N is pharmacologically reversed by E4031 and cisapride

Both E4031 and cisapride bind in the central cavity of the PD near the inactivation gate of hERG channel [39, 41, 44]. To further explore the role of the inactivation in the gating polarity of hERG, we studied the influence of E4031 and cisapride on the channel properties of K525N. In the presence of E4031 at 3 μM (> IC100 = 1 μM on WT hERG in CHO cells [45]) and Cisapride at 10 μM (> IC100 = 1 μM on WT hERG in CHO cells [46]), the outward current was almost completely blocked (Fig. 5a, and d). However, a partial inward current of K525N remained (Fig. 5a, and d), showing the peak current was more sensitive to E4031 and cisapride than the steady-state current (Fig. 5b, c, e, and f). The residual inward current (Fig. 5a, and d) is reminiscent of that of K525N&F627Y (Fig. 1f). The tail current of the residual inward current was increased as the membrane potential decreased from -100 mV (Fig. 5g, and h). The G-V curve can be fitted by a Boltzmann function with the V1/2 of -147.0 ± 12.7 mV and -119.6 ± 5.4 mV for K525N with E4031 and cisapride, respectively (Fig. 5g, and h). E4031 and cisapride converted a depolarization-activated channel of K525N into a hyperpolarization-activated channel.

Fig. 5
figure 5

The gating polarity of K525N is switched by E4031 and cisapride. a Representative step currents of K525N with or without 3 μM E4031. Green arrows indicate peak currents, and red arrowheads indicate steady-state currents. b I-V curves of peak currents (n≥6) and c steady-state currents (n≥6) of K525N with or without E4031. d Representative step currents of K525N with or without 10 μM cisapride. Green arrows indicate peak currents, and red arrowheads indicate steady-state currents. e I-V curves of peak currents (n≥6) and f steady-state currents (n≥6) of K525N with or without cisapride. G-V curves of K525N with or without g E4031 and h cisapride. Error bars represent mean ± SEM

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The extracellular interaction between the VSD and PD is critical for functions of K525N&F627Y

The extracellular and intracellular interaction of the voltage-sensing domain and the pore domain regulate voltage-gated ion channel functions including the hERG channel [18, 20, 22, 24, 25, 47]. The VSD-PD interaction is the mechanism that confers voltage-dependent inactivation in hERG, and whether the hyperpolarization channel of K525N&F627Y can be regulated by the extracellular interaction of the VSD and the pore is not clear. Based on the cryo-EM structure of hERG (PDB:5VA1) [6], we observed the extracellular interaction is potentially composed of the F431 on the S1, C566 in the S5, I607, and Y611 on the pore helix [6, 19, 22] (Fig. 6a). These potential interaction sites are flanked by K525 in the S4 and F627 in the selective filter (Fig. 6a). Mutating F431, C566, I607, and Y611 to the alanine with K525N&F627Y background did not change the expression pattern of hERG on the plasma membrane (Additional file 4: Fig. S4). With mutations of F431A, C566A, and Y611A, K525N can not rescue the current of F627Y at all. The mutation of I607A also partially disrupted the rescue effect of K525N on F627Y, and the inward current of K525N&F627Y&I607A was significantly reduced (Fig. 6b-d). Mutations of other residues beyond this region, such as I409A, barely affected functions of K525N&F627Y (Additional file 4: Fig. S4). F431A, C566A, and Y611A eliminated the current of K525N as well (Additional file 4: Fig. S4). Therefore, the potential interaction between the VSD and PD is also involved in the hyperpolarization-activated properties of K525N&F627Y.

Fig. 6
figure 6

F431A, C566A, I607A, and Y611A impair the inward current of K525N&F627Y. a The cryo-EM structure of hERG (PDB: 5VA1) [6] highlighted with K525 (blue), F627 (yellow), and potential key residues (red in the S1 helix, and green in the S5-P region) of the extracellular interaction face between the VSD and the PD. The top view and side view of the interaction region are zoomed out and shown in the Right panel. b Representative step currents of F431A, C566A, I607A, and Y611A on top of K525N&F627Y, respectively. c Normalized I-V curves (n≥6) and d current density (n≥6) of F431A, C566A, I607A, and Y611A on top of K525N&F627Y, respectively. Error bars represent mean ± SEM. **P<0.01; ***P<0.001, two-tailed Student’s t-test

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K525N&S631A is a “leak” channel

Previously, S631A was reported as an “inactivation-alleviation” mutant [48, 49]. Consistently, we found that the inactivation was absent even at +50 mV in S631A [48, 49] (Fig. 7a, and c). We first combined S631A with K525N to create K525N&S631A and recorded the channel behavior at a large range of membrane potentials (Fig. 7b). Interestingly, K525N&S631A was a “leak” channel with substantial inward and outward currents (Fig. 7b, and c). The inward current of K525N&S631A was different from K525N, as a saturated current was achieved at negative potentials (Fig. 7b, and c). However, K525N&S631A is still a depolarization-activated channel with the voltage dependence similar to K525N (Fig. 7d). ICA-105574 is a potent activator of hERG by alleviating the inactivation [50,51,52]. In the presence of ICA-105574, K525N also behaved as a “leak” channel (Fig. 7e), and the inward current was saturated at negative potential as well (Fig. 7f). ICA-105574 left-shifted the G-V curve of K525N channel at potential more negative than -80 mV significantly (Fig. 7g). Thus, the VSD and the PD together could also reshape hERG to a “leak” channel.

Fig. 7
figure 7

K525N&S631A is a “leak” channel. a Representative step currents of S631A, and b K525N&S631A. c I-V curves (n≥6) of S631A, K525N, and K525N&S631A, respectively. Steady-state currents indicated by green arrows in Fig. 7a and b were quantified. d G-V curves of S631A, K525N, and K525N&S631A, respectively. e Representative step currents and f I-V curves (n≥6) of K525N with or without 10 μM ICA-105574. g G-V curves of K525N with or without 10 μM ICA-105574. In the presence of ICA-105574, the G-V curve was fitted by the Boltzmann equation (blue line). Error bars represent mean ± SEM

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Discussion

The VSD is involved in switching the gating polarity of hERG

Both hERG and HCN belong to CNBD-family channels, sharing a similar structure [6, 8, 9]. Recently, several studies have revealed that the structural basis for the different polarities of the depolarization-activated channel and hyperpolarization-activated channel is associated with the pore domain of hERG [23, 26, 27]. D540K in the S4-S5 linker [23, 26] and V659P in the S6 helix [27] of hERG mediate the inward current that is gradually larger as if the membrane potential decreases. K540 interacts with R665 in the S6 helix to couple the VSD with the PD, underlying the mechanism of hyperpolarization-dependent opening of D540K [23]. V659P introduces a kink that disrupts the coupling between the VSD and the PD [27]. In the Shaker channel, the combination of L434F and P475D, two residues in the PD, converts it to the hyperpolarization activated channel as well [34]. Whether the VSD is involved in determining the gating polarity of hERG? In HCN-EAG chimera channels, the substitution of serine in helix breaking transition in the S4 with a bulky hydrophobic amino acid flips the gating polarity from inward to outward-rectifying [53], suggesting the VSD may be critical to the gating polarity. The S3-S4 linker is important for stabilizing the closed conformation of hERG relative to the open state [42, 43, 54]. As the first gating charge, K525 stabilizes the closed state of hERG. Mutations of K525 would disturb the pore gate closure, and left-shift the voltage dependence dramatically [43, 54,55,56,57,58]. We found herein K525N also impairs the pore gate closure and preserves the open and inactivated state. When cooperating with F627Y, a mutation in the inactivation gate [4, 31, 32], K525N successfully inverted the polarity of voltage dependence (Fig. 1e-h). Therefore, the VSD is also involved in modulating the gating polarity of hERG.

The hyperpolarization-activated mechanism of K525N&F627Y

The PD of the hERG channel contains the intracellular activation and extracellular inactivation gate [6]. Both gates are intimately regulated by the VSD (Fig. 8a) [6]. In the closed state at the rest membrane potential, the voltage sensor is located intracellularly, leading to the activation gate being closed and the inactivation gate being open [1, 6, 11]. Upon depolarization, the voltage sensor slides outwardly, inducing the activation gate to gradually open (Fig. 1a, and c) via the intracellular S4-S5 linker. Whereas the inactivation gate would keep open at a voltage lower than 0 mV, and close at higher voltages (Fig. 1a, and b). How the gating polarity of hERG is reversed in K525N&F627Y? K525 is the first gating charge of hERG [6], and eliminating the first gating charge may prohibit S4 from sliding down completely at hyperpolarization and prevent full closure of the activation gate [13, 59]. Since K525N left-shifts the voltage dependence significantly and eliminates the closed state of the channel (Fig. 4a, and b), the S4 might be located extracellularly, preventing full closure of the activation gate and resulting in a “leaky open” state in K525N&F627Y (Fig. 8b). The inactivation gate may still open at hyperpolarizing potentials, resembling the Shaker-IR-L434F-P475D channel [34]. However, as the membrane potential depolarizes, the inactivation gate gradually close (Fig. 8). K525N&F627Y only exhibits the open and the inactivated state without the closed state. Therefore, it is the inactivation gate that determines the ion conductance of K525N&F627Y, which is reminiscent of the Shaker-IR-L434F-P475D channel [34], and the voltage-dependent gate in the MthK potassium channel [60].

Fig. 8
figure 8

Suggested model for the inverted gating polarity of K525N&F627Y. a Upon depolarization, WT hERG sequentially forms three states, the closed, the open, and inactivated state. As the membrane potential depolarizes, S4 (yellow) of hERG slides extracellularly and slowly drives the activation gate open (red) via the S4-S5 linker (grey). Channels transit from a closed state into an open state that mediates an outward K+ current. Once the membrane potential is higher than 0 mV, S4 further translocates extracellularly, and channels are inactivated. Channels reach the inactivated state that is non-conductive to ions. The non-canonical coupling pathway between the VSD and PD is critical for the hERG channel function. b K525N&F627Y preserves two states of hERG, the open and the inactivated state. When the membrane potential is higher than -70 mV, S4 (yellow) usually sits extracellularly. Channels stay in the inactivated state that is non-conductive to ions. Once the membrane potential hyperpolarizes, S4 would translocate mildly toward the intracellular, and relieve the inactivation gate. Channels transit into a “leaky open” state that mediates an inward K+ current

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Non-covalent interactions of the VSD and PD in Kv channels

Two tetrameric architectures identified amongst Kv channels: domain-swapped channels, such as Shaker, Kv1.2, and Kv7.1, and non-domain-swapped channels, such as hERG, HCN, and KvAP [6]. In domain-swapped channels, the VSD from one subunit is in close contact with the PD from the adjacent subunit, forming an extensive inter-subunit non-covalent interface. In non-domain-swapped channels the VSD and PD from the same subunit closely contact with a non-covalent interface as well. The non-covalent interface is located at the extracellular region of the VSD and PD. The non-covalent interface of domain-swapped channels is similar with that of non-domain-swapped channels, which is supported by the Shaker channel [20] and hERG [25]. In Shaker K+ channel, the voltage sensor is coupled with the selective filter (VS-SF coupling) through the extracellular interaction chain composed of the S4, S5, P-Loop, and SF [20]. The L366H in the S4 restores the K+ conduction abrogated by W434F in the PD of the Shaker-IR channel. The disruption of the functional connection between contiguous residues in the S4-S5-(P-Loop)-SF chain is sufficient to decrease the K+ conduction of L366H:W434F [20]. A kinematic chain of residues that couples the VSD to PD consists of S4/S1 and S1/S5 subunit interfaces in hERG [25]. The movements of VSD electromechanically propagates to the constriction of the SF following the S4-S1-S5-(P-Loop)-SF route relevant for the C-type inactivation [25]. These paths in hERG resemble those for the Shaker channel, suggesting the presence of a common underlying mechanism of electromechanical coupling across the superfamily of Kv channels.

K525N and drug treatment

LQT2-associated mutations broadly distribute in every domain of hERG [2, 30, 61]. A comprehensive study analyzing 226 different LQT mutations reported that 32% resided in transmembrane and pore domains [61]. Deficient protein trafficking to the cell membrane is the dominant mechanism for most of the mutations associated with LQT2 [3, 62]. The trafficking defect mutants can be pharmacologically corrected by culturing in the presence of pore-blocking drugs such as E4031 [62, 63]. Although K525N is still functional on the cell surface (Fig. 4), many channel functional properties are different from WT hERG. Neither activators nor inhibitors of hERG can restore the functions of K525N (Figs. 5 and 7). Therefore, our study suggests alternative treatments should be developed for LQT2 patients carrying the K525N mutation. In addition, LQT2 syndrome in patients with K525N&R528P [30] may not be pathologically attributed to the K525N, since K525N is a gain-of-function mutant of hERG.

Conclusions

This work characterized the role of a long-QT syndrome type-2-related mutation in the voltage-sensing domain, K525N [30], in modulating the gating polarity of hERG. Completely different from WT hERG, K525N together with F627Y reversed a depolarization-activated channel into a hyperpolarization-activated channel. K525N&F627Y conducted ions upon hyperpolarization and was non-conducted under depolarization. A Boltzmann fitting curve of the tail current gave a V1/2 is about -103.2 mV. The non-deactivated inward current conducted by K525N&F627Y was still sensitive to hERG channel blockers. Pharmacologically, a hyperpolarization-activated channel was also achieved by blocking K525N with E4031 and cisapride. Furthermore, we discovered that the extracellular interaction between the S1 helix and the S5-P region was crucial for the involvement of the VSD in modulating the gating polarity of hERG.

Methods

Mutagenesis

The hERG construct was a gift from M. Sanguinetti (University of Utah), which has been described in our previous work [64]. hERG mutants were generated with QuikChange lightning II site-directed mutagenesis kit (Agilent) and confirmed by DNA sequencing. Primers used for site-directed mutagenesis are listed below.

mutation

Forward primer

Reverse primer

K525N

gatcgggctgctgaacactgcgcggctg

cagccgcgcagtgttcagcagcccgatc

F627Y

ctcaccagtgtgggctacggcaacgtctc

gagacgttgccgtagcccacactggtgag

G628S

cagtgtgggcttcagcaacgtctctcccaac

gttgggagagacgttgctgaagcccacactg

F431A

ccctactcggctgccgccctgctgaaggagac

gtctccttcagcagggcggcagccgagtaggg

C566A

cgcactggctagccgccatctggtacgccatc

gatggcgtaccagatggcggctagccagtgcg

I607A

ctgggcggcccctccgccaaggacaagtatg

catacttgtccttggcggaggggccgcccag

Y611A

cctccatcaaggacaaggctgtgacggcgctctac

gtagagcgccgtcacagccttgtccttgatggagg

I419A

catcctgctgctggtcgcctacacggctgtcttc

gaagacagccgtgtaggcgaccagcagcaggatg

S631A

gcttcggcaacgtcgctcccaacaccaac

gttggtgttgggagcgacgttgccgaagc

K525R

ctgatcgggctgctgcggactgcgcggctg

cagccgcgcagtccgcagcagcccgatcag

K525C

ctgatcgggctgctgtgtactgcgcggctgctg

cagcagccgcgcagtacacagcagcccgatcag

K525S

gagctgatcgggctgctgagtactgcgcggctg

cagccgcgcagtactcagcagcccgatcagctc

K525M

gatcgggctgctgatgactgcgcggc

gccgcgcagtcatcagcagcccgatc

K525P

gatcgggctgctgccgactgcgcggctg

cagccgcgcagtcggcagcagcccgatc

K525A

gatcgggctgctggcgactgcgcggctg

cagccgcgcagtcgccagcagcccgatc

K525V

gatcgggctgctggtgactgcgcggctg

cagccgcgcagtcaccagcagcccgatc

K525E

ctgatcgggctgctggagactgcgcgg

gccgcgcagtctccagcagcccgatcag

Cell culture and transient transfection

Chinese Hamster Ovary (CHO) cells were grown in 50/50 DMEM/F12 (Cellgro, Manassas, VA) with 10% fetal bovine serum (FBS) and 2 mM L-glutamine (Gibco, Carlsbad, CA). To express ion channels, cells were split 24 hours before transfection, plated in 60-mm dishes, and transfected with Lipofectamine 3000™ reagent (Invitrogen, Carlsbad, CA), according to the manufacturer’s instruction. At 24 hours after transfection, cells were split and re-plated onto coverslips coated with poly-L-lysine (Sigma-Aldrich, St. Louis, MO). A plasmid for cDNA of GFP (Amaxa, Gaithersburg, MD) was co-transfected to aid the identification of transfected cells by fluorescence microscopy.

Electrophysiological recording

Whole-cell voltage-clamp recording was carried out at room temperature in CHO cells with an Axopatch-200B amplifier (Molecular Devices, Sunnyvale, CA). The electrodes were pulled from borosilicate glass capillaries (World Precision Instruments, Sarasota, FL). When filled with the intracellular solution, the electrodes had resistances of 3-5 MΩ. The pipette solution contained (mM): KCl 145, MgCl2 1, EGTA 5, HEPES 10, and MgATP 5 (pH 7.3 with KOH). During the recording, constant perfusion of the extracellular solution was maintained using a BPS perfusion system (ALA Scientific Instruments, Westbury, NY). The extracellular solution contained (mM): NaCl 140, KCl 5, CaCl2 2, MgCl2 1.5, HEPES 10, and glucose 10 (pH 7.4 with NaOH). Signals were filtered at 1 KHz and digitized using a DigiData 1550B with pClamp 11.2 software (Molecular Devices, Sunnyvale, CA). Series resistance was compensated by 60-80%.

Determination of relative permeability (P X/P K)

The permeability of TMEM175 for Na+ and NMDG+ relative to K+ was estimated based on the Goldmann-Hodgkin-Katz current equation s[65] and the measured Erev using “bi-ionic” conditions:

$$\frac{P_X}{P_K}=\frac{{\left[{K}^{+}\right]}_i{e}^{\left({}^{ FV}\!\left/ \!{}_{ RT}\right.\right)}-{\left[{K}^{+}\right]}_e}{{\left[{X}^{+}\right]}_e-{\left[{X}^{+}\right]}_i{e}^{\left({}^{ FV}\!\left/ \!{}_{ RT}\right.\right)}}$$

Where R, T, F, and V are the gas constant, absolute temperature, Faraday`s constant, and the reversal potential, respectively. In the whole-cell recording, the pipette solution is (in mM): KCl 145, EGTA 5, and HEPES 10 (pH 7.3 with KOH). The sodium solution is (in mM): NaCl 145, EGTA 5, and HEPES 10 (pH 7.3 with NaOH). The NMDG solution is (in mM): NMDG 145, EGTA 5, and HEPES 10 (pH 7.3 with HCl). Erev was determined using a pre-open at 0 mV step protocol in response to extracellular solutions.

Data and statistical analysis

Patch-clamp data were processed using Clampfit 11.2 (Molecular Devices, Sunnyvale, CA), and then analyzed in Origin 2018 (OriginLab, Northampton, MA). Voltage-dependent activation curves were fit with the Boltzmann equation: G=Gmin+(Gmax-Gmin)/(1+exp(V-V1/2)/S)), where Gmax is the maximum conductance, Gmin is the minimum conductance, V1/2 is the voltage for reaching 50% of the maximum conductance and S is the slope factor. Data are presented as means ± SEM. Significance was estimated using paired two-tailed students’ t-tests.

Availability of data and materials

All data generated or analyzed during this study are included in this published article and its supplementary information files.

Abbreviations

CNBD:

Cyclic nucleotide-binding domain

hERG:

human Ether-a-go-go Related Gene

VSD:

Voltage-sensing domain

LQT2:

Long-QT syndrome type 2

PD:

Pore domain

I Kr :

Rapidly activating delayed rectifier potassium current

ECG:

Electrocardiogram

Kv:

Voltage-gated potassium channel

HCN:

Hyperpolarization-activated and cyclic nucleotide-gated

CHO:

Chinese Hamster Ovary

WT:

Wild-type

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Acknowledgements

We appreciate the encouragement and helpful comments provided by Dr. P. Li`s laboratory and Dr. Z. Gao`s laboratory colleagues.

Funding

This work was supported by grants from the National Natural Science Foundation of China (32100621, 82273913, and 82200368), Guangdong Basic and Applied Basic Research Foundation (2022A1515010851), Zhongshan Municipal Bureau of Science and Technology (220418134367984, and CXTD2022013), China Postdoctoral Science Foundation (2022M713264), Department of Science and Technology of Guangdong Province (2019B090904008, and 2021B0909050003).

Author information

Author notes

  1. Zhipei Liu, Feng Wang, Hui Yuan, and Fuyun Tian contributed equally to this work.

Authors and Affiliations

  1. School of Pharmacy, Zunyi Medical University, Zunyi, 563000, China

    Feng Wang, Hui Yuan, Guimei Yang, Zhaobing Gao & Ping Li

  2. Zhongshan Institute for Drug Discovery, Zhongshan, 528400, China

    Zhipei Liu, Feng Wang, Hui Yuan, Fuyun Tian, Chuanyan Yang, Fei Hu, Yiyao Liu, Meiqin Tang, Meixuan Ping, Chunlan Kang, Ting Luo, Guimei Yang, Mei Hu, Zhaobing Gao & Ping Li

  3. Center for Neurological and Psychiatric Research and Drug Discovery, Shanghai Institute of Materia Medica, Chinese Academy of Sciences, Shanghai, 201203, China

    Zhipei Liu, Fuyun Tian, Chuanyan Yang, Fei Hu, Meixuan Ping, Zhaobing Gao & Ping Li

  4. School of Basic Medicine and Clinical Pharmacy, China Pharmaceutical University, Nanjing, 210009, China

    Chuanyan Yang

  5. School of Pharmaceutical Sciences, Southern Medical University, Guangzhou, 510515, China

    Meiqin Tang & Chunlan Kang

  6. University of Chinese Academy of Sciences, Beijing, 100049, China

    Meixuan Ping, Zhaobing Gao & Ping Li

  7. School of Pharmaceutical Sciences, Guizhou Medical University, Guiyang, 550025, China

    Ting Luo

  8. Pharmacology Laboratory, Zhongshan Traditional Chinese Medicine Hospital, Guangzhou University of Chinese Medicine, Zhongshan, 528401, China

    Mei Hu

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  1. Zhipei Liu
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  2. Feng Wang
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  3. Hui Yuan
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Contributions

Conceptualization: ZL, FT, and PL; Methodology: ZL, FW, HY, and FT; Supervision: ZG, and PL. ZL, FW, FT, CK, TL, and GY performed whole-cell patch-clamp recordings. HY, CY, FH, YL, MT, MP, and MH generated mutants of hERG. FT, ZG, and PL wrote the paper with input from all authors. All authors read and approved the final manuscript.

Corresponding authors

Correspondence to Zhaobing Gao or Ping Li.

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Supplementary Information

Additional file 1: Fig. S1.

K525N&G628S is a hyperpolarization-activated channel. a The expression pattern of hERG-EGFP, and F627Y-EGFP in CHO cells stained with Dil dye (red). b The representative ramp current of K525N&F627Y. The ramp protocol (below) ranges from -130 to +30 mV in 5 seconds with a holding potential at -100 mV. c Representative currents of G628S. d Representative currents of K525N&G628S. e The G-V and e the I-V curve of K525N&G628S.

Additional file 2: Fig. S2.

K525N&G628S is a K+ selective channel. a Representative current traces with ramp protocols and b histogram of the reversal potential of K525N&F627Y in the presence of different bath solutions. c Representative current traces and d histogram of the reversal potential of WT hERG channel in the presence of different bath solutions. e Representative current traces and f histogram of the reversal potential of K525N&G628S in the presence of different bath solutions. g Analysis of relative K+ permeability over Na+, or NMDG+ of K525N&G628S based on Erev measurement (n≥6). Error bars represent mean ± SEM.

Additional file 3: Fig. S3.

Various K525 mutations disturb channel closure. a G-V curves of K525 mutants.

Additional file 4: Fig.

 4. I419A did not impair the inward current of K525N&F627Y. a The expression pattern of K525N&F627Y&F431A-EGFP, K525N&F627Y&C566A-EGFP, K525N&F627Y&I607A-EGFP, and K525N&F627Y&Y611A-EGFP in CHO cells stained with Dil dye (red). b The cryo-EM structure of hERG (PDB: 5VA1) highlighted with K525 (blue), F627 (yellow), and F431 (red) and I419 (green) residues amongst the potential interaction face between the VSD and PD. The top view and side view of the interaction region are zoomed out and shown in the Right panel. c Representative step currents of K525N&F627Y, and K525N&F627Y&I419A, respectively. d Current density (n≥6) of K525N&F627Y, and K525N&F627Y&I419A, respectively. Representative currents of e K525N, f K525N&F431A, g K525N&C566A, and h K525N&Y611A. Error bars represent mean ± SEM. **P<0.01; ***P<0.001, two-tailed Student’s t-test.

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Liu, Z., Wang, F., Yuan, H. et al. An LQT2-related mutation in the voltage-sensing domain is involved in switching the gating polarity of hERG. BMC Biol 22, 29 (2024). https://0-doi-org.brum.beds.ac.uk/10.1186/s12915-024-01833-0

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BMC Biology

ISSN: 1741-7007

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