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Department of Medicine, Division of Cardiology, Johns Hopkins University School of Medicine, Baltimore, MD 21205

Correspondence to Gordon F. Tomaselli: gtomasel{at}jhmi.edu

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
Calmodulin (CaM) regulates steady-state inactivation of sodium currents (Na_V1.4) in skeletal muscle. Defects in Na current inactivation are associated with pathological muscle conditions such as myotonia and paralysis. The mechanisms of CaM modulation of expression and function of the Na channel are incompletely understood. A physical association between CaM and the intact C terminus of Na_V1.4 has not previously been demonstrated. FRET reveals channel conformation-independent association of CaM with the C terminus of Na_V1.4 (CT-Na_V1.4) in mammalian cells. Mutation of the Na_V1.4 CaM-binding IQ motif (Na_V1.4_IQ/AA) reduces cell surface expression of Na_V1.4 channels and eliminates CaM modulation of gating. Truncations of the CT that include the IQ region abolish Na current. Na_V1.4 channels with one CaM fused to the CT by variable length glycine linkers exhibit CaM modulation of gating only with linker lengths that allowed CaM to reach IQ region. Thus one CaM is sufficient to modulate Na current, and CaM acts as an ancillary subunit of Na_V1.4 channels that binds to the CT in a conformation-independent fashion, modulating the voltage dependence of inactivation and facilitating trafficking to the surface membrane.

Abbreviations used in this paper: CaM, calmodulin; CT, carboxy terminus; DIC, differential interference contrast; FRET, fluorescence resonance energy transfer; Na_V, voltage-gated sodium channel.

	INTRODUCTION

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Voltage-gated sodium channels (Na_v) underlie the rising phase and influence the duration of action potentials in excitable cells such as neurons and cardiac and skeletal myocytes. Heritable defects in Na channel expression and gating are associated with myotonia (Yang et al., 1994; Wang et al., 2003; Wu et al., 2005), epilepsy (Kearney et al., 2001; Lossin et al., 2002), and sudden cardiac death (Keating and Sanguinetti, 2001). Na_v currents are regulated by the ubiquitous calcium-sensing protein calmodulin (CaM). The carboxy terminus (CT) of these channels contains a CaM-binding, so-called IQ motif (Mori et al., 2000; Deschênes et al., 2002). The Na channel IQ motif is homologous to CaM binding sites in canonical CaM-regulated channels, such as L-type Ca channels, which are evolutionarily related to Na channels.

Despite the conservation of a CaM-binding IQ motif in all Na_Vs, CaM regulation of Na currents is isoform specific (Deschênes et al., 2002; Herzog et al., 2003; Young and Caldwell, 2005). In vitro, cell-free association of CaM with the CT of Na_V channels has been demonstrated; however, such studies could be compromised by nonphysiological CT peptide conformations that exist under conditions that are required to solubilize the channel or channel fragments. Moreover, there is little known about channel state dependence of CaM binding, the number of CaM molecules required to regulate Na_V inactivation, and effects on channel function other than gating. Here we explore whether CaM binds to the CT of intact Na_V1.4 channels and if this interaction is conformation specific. We fused enhanced fluorescence protein to the cytoplasmic C termini of Na_V1.4 and CaM; the interaction of CaM with Na_V1.4-CT was monitored using fluorescence resonance energy transfer (FRET) in live cells. The data reveal an intimate spatial relationship between CaM and the Na_V1.4 CT that is conformation independent. CaM interaction with the CT of Na_V1.4 influences trafficking of the channel protein to the surface membrane and modulates steady-state inactivation. The fusion of a single CaM molecule to the channel near the IQ through a glycine linker was sufficient to modulate Na_V1.4 gating, suggesting that a single CaM binding to the CT of Na_V1.4 is sufficient for modulation of inactivation.

	MATERIALS AND METHODS

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Plasmid Construction
EYFP/ECFP Fused to Wild Type and Mutant Sodium Channels.
DNA fragments containing EYFP and ECFP were prepared by the addition of an in-frame insert containing EYFP/ECFP. Na_V1.4 was cloned into the EcoR1 site of mammalian expression vector GW1H. The fragments were cloned in frame to the CT of Na_V1.4 to create Na_V1.4-ECFP/EYFP. The EYFP/ECFP fragments were generated by PCR amplification of regions of pEYFP/pECFP (CLONTECH Laboratories, Inc.) vectors encoding the fluorescent protein with primers that contain an NheI site in the forward primer (5'-AATGAACAGCTAGCGTACCGGTCGCCACCATGG) and NotI in the reverse primer (5'-TTCTAGAGTCGCGGCCGCTT for EYFP and 5'-TCTAGAGTCGCGGCCGGAA for ECFP). The stop codon of Nav1.4 was replaced with an NheI site, and the EYFP/ECFP fragments were directionally cloned into this site and a NotI site in the GW1H. The IQ/AA mutants (I1727A/Q1728A) were made by site-directed mutagenesis of the Na_V1.4-ECFP/EYFP construct.

Construction of Na_V1.4-ECFP/EYFP Deletion Mutants.
Inserts containing the Na_V1.4 cDNA that were truncated at codons 1723 (Na_V1.4₁₇₂₃) or 1740 (Na_V1.4₁₇₄₀) in frame with either ECFP or EYFP, were generated by PCR using the forward primer Na_V1.4-BstZF (CTGCGTCAACACCACCACCT) and either one of the reverse primers Na_V1.4-1723NheR (1736bp) or Na_V1.4-1740NheR (1787 bp). The reverse primers used to prepare the 1723 and 1740 truncations were TCGAATCAGCTAGCACACACCTCCTCCTGCTTCC and TCGAATCAGCTAGCCACGGAGCGCTGCAGCAGG, respectively. The PCR products that generated the truncations were ligated into pGW1H-Na_V1.4 digested with BstZ17I and NheI. All the clones were sequence confirmed.

Construction of Na_V1.4₁₇₄₀ -Glycine-CaM-EYFP.
Glycine (G₄)-linkered CaM was inserted into Na_V1.4₁₇₄₀-EYFP by cloning a PCR product of full-length CaM flanked by in-frame Nhe1 sites into an NheI site between the channel and fluorescent protein coding regions. The G₄-CaM insert was prepared by PCR using a calmodulin-containing plasmid as template and the forward primer 5'-attcatGCTAGCGGAGGAGGCGGGATGGCTGACACTGA-3' and the reverse primer 5'-attcatGCTAGCCTTCGCTGTCATCATTTGTAC-3'. The forward primer contains an in-frame Nhe1 site followed by four glycine codons and then the calmodulin start sequence, the reverse primer contains an Nhe1 site and the end of the calmodulin coding region without the stop codon. The G₄ construct was used to prepare the construct with CaM linkered with 14 glycines (G₁₄). The linker length was increased from 4 to 14 glycines by mutation of the 5' Nhe1 site to an AvrII site and the insertion of annealed oligonucleotides encoding 10 glycines and containing AvrII sticky ends.

Cell Culture and Transfection
Approximately 0.75 x 10⁶ human embryonic kidney cells (HEK293; American Type Culture Collection) were cultured in six-well tissue dishes in DMEM supplemented with FBS 10%, L-glutamine (2 mmol/liter), penicillin (100 U/ml), and streptomycin (10 mg/ml). The cells were cotransfected with β1 and plasmids encoding wild-type sodium channels Na_V1.4-EYFP, Na_v1.4-ECFP or mutant Na_V1.4_IQ/AA-ECFP, Na_V1.4_IQ/AA-EYFP, Na_V1.4₁₇₄₀-EYFP, Na_V1.4₁₇₂₃-EYFP, and wild-type ECFP/EYFP-CaM or mutant ECFP/EYFP-CaM₁₂₃₄ alone or in combination. Cells were transfected using Lipofectamine^TM 2000 (Invitrogen) according to the manufacturer's instructions and were studied 48–72 h post-transfection. The total amount of DNA for all transfections was kept constant.

Electrophysiology
HEK293 cells expressing wild-type or mutant tagged Na_V1.4 channels and CaM or CaM₁₂₃₄ were patch clamped with an Axopatch 200B patch-clamp amplifier using pipettes with tip resistances of 1–3 M and typical series resistance compensation of >90% to minimize voltage clamp errors. Transfected cells were identified for patch clamping by ECFP, EYFP, or GFP fluorescence. Current recording was initiated 10 min after establishing the whole-cell configuration to avoid time-dependent shifts in gating. The bath solution contained (in mM) 150 NaCl, 2 KCl, 2 CaCl₂, 1 MgCl₂, 10 glucose, and 10 Na-HEPES (pH 7.4). The patch pipette contained (in mM) 35 NaCl, 3.7 CaCl₂, 5 BAPTA, and 10 Cs-HEPES (pH 7.3). The free [Ca²⁺] in the pipette was 0.5 µM; the bath and pipette solutions were adjusted to same osmolarity using glucose.

For simultaneous FRET measurements cells were held at –140, –60, and –20 mV during the collection of emitted light. A standard two-pulse protocol (500 ms pulse from –140 to –50 mV and a 50-ms test pulse to –20 mV) was used to generate the steady-state inactivation curves. Recovery from inactivation was assessed with a two-pulse protocol with a 30-ms first pulse to –20 mV followed by a variable interpulse interval and a second 30-ms pulse to assay recovery from predominantly fast inactivated states. Entry into inactivated states was assessed by a variable first test pulse to –20 mV (1–10,000 ms), followed by a 10-ms interpulse interval and a second test pulse of 50 ms to –20 mV to assay entry into slowly recovering (intermediate and slow) inactivated states.

FRET Measurements
Measurements of single-cell FRET based on aggregate (nonspatial) fluorescence recordings with donor dequenching were performed as previously described (Erickson et al., 2001) with minor modifications. Donor dequenching experiments were performed using a CFP filter cube (D440/20M (excitation), 455DCLP (dichroic), D480/30M (emission; Chroma Technology Corp.) before and 5 min after intense illumination using a custom YFP photobleaching cube (Chroma Technology Corp.), consisting of a D535/50x excitation filter and a 100% mirror (in place of a dichroic mirror). In control experiments this bleaching protocol spared CFP fluorescence. Epifluorescence images were acquired with a PI1300 CCD camera (Princeton Instruments) mounted to the side port of Olympus IX70 inverted microscope (60 x 1.4 objective; oil) driven by Metamorph software (Version7.0, Molecular Devices). The exposure time was set during the prebleach image acquisition and was not changed throughout the acquisition. Intensities were measured from a user-defined region of interest within the area of YFP fluorescence. Each image was background adjusted by subtracting the average pixel intensity from a region in the same field located outside the cell. Donor dequenching FRET efficiency (E_EFF) was calculated using a previously described method (Erickson et al., 2001) in SigmaPlot (Systat Software Inc.). Movies of cell fluorescence intensities were recorded by stream acquisition (600 frames, 50-ms exposure time). The CaM and Na_V1.4 interaction was further studied using the nondestructive 3³ (three cube) FRET method, which has been previously used in CFP/YFP FRET to show interaction of CaM with the L-type Ca²⁺ channel. 3³ FRET is highly concordant with donor dequenching FRET, thus is used as a complementary method to verify results of donor dequenching FRET. 3³ FRET avoids the need for photolysis of the acceptor, thus reducing the possibility of artifactual changes in the quantum yield of the donor. The 3³ method measures the FRET ratio, a fractional increase in YFP emission due to FRET, by eliminating direct excitation of YFP and contaminating CFP emission using different filter cubes. 3³ FRET images were acquired with the following filter cubes (excitation, dichroic, emission): CFP filter cube (D440/20M, 455DCLP, D480/30M, Chroma Technology Corp.); the YFP filter cube (HQ500/20x, Q515LP, HQ505/30, Chroma Technology Corp.); and the FRET filter cube (D440/20M, Chroma Technology Corp.), 455DRLP (Omega Optical Inc. Brattleboro, VT), HQ535/30 (Chroma). The FRET ratio and FRET efficiency were calculated as previously described (Erickson et al. 2001).

Cell Surface Expression and Western Blot Analysis
The cells were cotransfected with equal amounts (0.5 µg/ml) of either wild-type Na_V1.4-EYFP or Na_V1.4₁₇₄₀-EYFP or Na_V1.4_IQ/AA-EYFP plasmids. The concentrations of plasmids were estimated spectrophotometrically and further confirmed by agarose gel electrophoresis (not depicted). The cells were grown to a similar level of confluence and then surface channels were biotinylated and total cell lysates were isolated; this includes biotin-labeled (cell surface) and unlabeled channels (the remainder). HEK293 cells were surface biotinylated for 1 h at 4°C using Sulfo-NHS-SS-Biotin (Pierce Biotechnology Inc.) 48 h after transfection. After quenching the excess biotin, cells were washed and lysed in 500 µl of 2% SDS, 50 mM EDTA with brief probe sonication. The total cell lysate was aliquoted and a fraction was used for purification of biotinylated proteins using Immobilized NeutrAvidin (Pierce Biotechnology Inc.) according to the manufacturer's protocol. The same volumes of total cell lysate and NeutrAvidin precipitates were run on the same SDS-PAGE (7%) gels, transferred to nitrocellulose membranes, and incubated with a monoclonal anti-Na channel antibody (Sigma-Aldrich, IgG₁ anti-mouse 1:500). The intensities of bands on the Western blots were quantified using Metamorph software (Version7.0, Molecular Device). The density of the biotinylated protein bands were normalized to their respective total lysate densities from the same gels. The intensity ratios (biotinylated proteins/total lysate proteins) were compared for each of the Na channel subunit variants expressed in the absence of CaM. For detection of CaM, HEK293 cells were transfected with ECFP-CaM (gift from D.T. Yue, Johns Hopkins University), ECFP-CaM₁₂₃₄, or ECFP alone (1 µg/ml). 48 h after transfection cells were lysed, briefly probe sonicated and proteins from the same volume of cell lysates were separated and analyzed by Western blotting with anti-CaM and anti-GFP antibodies (Covance).

Confocal microscopy
Approximately 0.75 x 10⁶ cells were plated and then transfected on coverslips in a six-well culture dish fixed in 4% formaldehyde 48 h after transfection. Fixed HEK293 cells expressing Na_V1.4-EYFP or the IQ mutant Na_V1.4_IQ/AA-EYFP fusion proteins were imaged using a confocal microscope (LSM510, Carl Zeiss MicroImaging, Inc.) with 63x/1.4 or 100x/1.4 oil differential interference contrast (DIC) plan apochromat objectives (Carl Zeiss MicroImaging, Inc.). EYFP was excited at 514 nm with an LSM510 Argon laser and emitted light was detected with a 530–600-nm band pass filter and beam splitter (HFT 405/514, mirror and NFT 515). Transmitted DIC images were obtained simultaneously.

Data Analysis
Electrophysiological, protein expression, and FRET data were expressed as the means ± SEM and inactivation data were fit to a Boltzmann function. Data for entry into inactivation and recovery from inactivation were fit to exponential functions. Significance was assessed using a t test (Microcal Origin, Microcal Software Inc.).

Online Supplemental Material
The online supplemental material (available at http://www.jgp.org/cgi/content/full/jgp.200709863/DC1) contains two figures. Fig. S1 summarizes the biophysical properties of Na_V1.4_IQ/AA in the presence of CaM and AIP. Fig. S2 illustrates the effect of the C-terminal truncation Na_V1.4₁₇₂₃ on channel trafficking by epifluorescence microscopy and Western blotting.

	RESULTS

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CT-Na_V1.4 Fusion Constructs Are Functionally Expressed and Interact with CaM
We have previously shown that CaM associates with wild type GST-tagged Na_V CT peptides in vitro (Deschênes et al., 2002), this work motivated studies of the interaction between the CT of intact Na_V channels and CaM in live cells using FRET. We designed channel fusions with fluorescent proteins linked to the CT, which is close in the linear amino acid sequence to the IQ motif, optimizing the possibility of FRET detection on CaM binding. One of the major concerns about fusion of a fluorophore to CT is the possibility of functional alterations of the sodium current by tagging the channel. The CT EYFP/ECFP-tagged Na_V1.4 channels were fully characterized and did not exhibit significant changes in current–voltage relationship or the voltage dependence of activation and steady-state inactivation compared with untagged wild-type channels expressed in HEK293 cells (Table I).

View larger version (47K): [in this window] [in a new window] [Download PPT slide]   Figure 1. NaV1.4-EYFP expression. (A) NaV1.4-EYFP expression in HEK293 cells. Epifluoresecence image and intensity profile of an HEK293 cell expressing NaV1.4-EYFP and NaVβ1subunits. The peaks in the fluorescence profiles indicate membrane targeting. (B) A family of NaV1.4-EYFP currents elicited by the voltage protocol shown in the inset. (C) Western blot of total cell lysates from NaV1.4-EYFP–transfected (1 µg/ml) HEK293 cells and nontransfected controls. Lysates isolated 48 h after transfection, separated by Western blot, and probed with an anti-NaV antibody exhibit a band near 197 kD representing NaV1.4-EYFP expression.

View larger version (29K): [in this window] [in a new window] [Download PPT slide]   Figure 2. ECFP-CaM overexpression in HEK293 cells. (A) Epifluorescence image and intensity profile of an HEK293 cell expressing ECFP-CaM alone shows uniform cytosolic expression of CaM. (B) Immunoblot of HEK293 lysates probed with an anti-CaM antibody demonstrates endogenous CaM, ECFP-CaM, and ECFP-CaM1234 (left). Immunoreactive ECFP, ECFP-CaM, and ECFP-CaM1234 are shown with an anti-GFP antibody. (C) Epifluoresecence image and intensity profile of NaV1.4-EYFP coexpressed with ECFP-CaM in HEK293 cells; the peaks indicate membrane targeting. In the top panel, the cell is excited with 535-nm light and the bottom panel is the same cell excited with 440-nm light showing enrichment of ECFP-CaM at the cell membrane when coexpressed with NaV1.4-EYFP.

View larger version (39K): [in this window] [in a new window] [Download PPT slide]   Figure 3. CaM modulation of inactivation gating of NaV1.4. (A) A representative family of NaV1.4-EYFP currents elicited by the steady-state inactivation protocol shown in the inset. Currents were recorded at a test pulse of –20 mV after a 500-ms conditioning pulse from –140 to +30 mV. The bottom panel shows the steady-state inactivation curves of NaV1.4 EYFP expressed in HEK293 cells alone () or coexpressed with ECFP-CaM (•) or ECFP-CaM1234(), and in the presence of both ECFP-CaM and EYFP-CaM1234 (). The data are means ± SEM and fit to Boltzmann function. (B) A representative family of NaV1.4-EYFP currents in the presence of AIP290-309 elicited by the steady-state inactivation protocol in (A). The CaM anti-peptide AIP290-309 added to the pipette solution abolishes the CaM-induced shift in the steady-state inactivation of NaV1.4-EYFP (), AIP290-309 in the absence of overexpression of CaM induces a rightward shift in the V1/2 of steady-state inactivation (•). In IQ/AA mutant channels, AIP290-309 induces a rightward shift in the V1/2 of steady-state inactivation of NaV1.4IQ/AA-EYFP () compared with the absence of AIP290-309 (). (C) Effect of AIP290-309 on the normalized current–voltage relationships of NaV1.4IQ/AA-EYFP and NaV1.4-EYFP currents. The top panels are representative raw current records of NaV1.4 and mutant NaV1.4IQ/AA channels with AIP290-309 (protocol in the inset). The normalized current–voltage (IV) relationships for NaV1.4-EYFP in absence () and presence of AIP290-309 (•), and for NaV1.4IQ/AA-EYFP () reveal that peak IV relationship for NaV1.4IQ/AA is significantly shifted in the depolarizing direction in presence of AIP290-309 (). (D) The recovery of the channels from inactivation measured using the protocol in the inset reveal that rec of NaV1.4IQ/AA in presence of AIP290-309 () is significantly shorter than that of NaV1.4IQ/AA in the absence of AIP290-309 (). The rec of NaV1.4 is not significantly different in the absence () and presence of AIP290-309 (•). (E) The entry of the channels into inactivation was measured using the protocol in the inset. The entry of NaV1.4IQ/AA is decreased in the presence of AIP290-309(), the entry of NaV1.4 (•) in the presence of AIP290-309 is not significantly different from NaV1.4 in the absence of AIP290-309().

Inclusion of the CaM anti-peptide (AIP290-309) in the pipette solution mitigates the CaM-induced shift in the steady-state inactivation curve (V_1/2 = –63.7 ± 0.2 mV, n = 7) in cells coexpressing Na_V1.4- EYFP and ECFP-CaM (Fig. 3 B). These data are consistent with the peptide effectively competing with CaM binding to the CT of Na_V1.4 and supports the hypothesis that CaM binding to the CT is essential for modulation of the voltage dependence of inactivation gating. In the absence of CaM overexpression, AIP290-309 induced a +7-mV shift in the steady-state inactivation curve (V_1/2 = –58.5 ± 0.2 mV, n = 7) compared with cells expressing only Na_V1.4-EYFP (Fig. 3 B). AIP290-309 may be acting by displacement of endogenous CaM from the channel or through inhibition of CaM binding to other sites on Na_V1.4 or other effector proteins. However, in cells expressing Na_V1.4_IQ/AA, AIP290-309 induces an +12-mV shift in the steady-state inactivation curve (V_1/2 = –61.1 ± 0.1 mV, n = 10) compared with cells expressing Na_V1.4_IQ/AA in the absence of AIP (V_1/2 = –73.9 ± 0.2 mV, n = 7; Fig. 3 B). AIP290-309 has several distinct effects on gating of Na_V1.4_IQ/AA that are not observed in the wild-type channel. AIP290-309 shifts the peak current–voltage relationship to right in Na_V1.4_IQ/AA (Fig. 3 C). Channel recovery from inactivated states and entry into slowly recovering inactivated states were evaluated using the pulse protocols in the insets of Fig. 3, D and E, respectively. AIP hastens recovery (_rec) from fast inactivation state in IQ/AA mutant channels without affecting the wild-type channel (Fig. 3 D). AIP290-309 significantly reduces _rec from 5.5 ± 0.1 ms (n = 7) to 4.5 ± 0.7 ms in Na_V1.4_IQ/AA (n = 10, Fig. 3 D) and decreases _entry from 1592.80 ± 127.4 ms (n = 6) to 815.3 ± 98.2 ms (n = 7, Fig. 3 E). In contrast, AIP290-309 did not significantly alter _rec or _entry of wild-type Na_V1.4 (Fig. 3, D and E). Thus the IQ/AA mutation unmasks effects of AIP290-309 that are independent of CaM binding to the channel.

To further elucidate role of the IQ region in CaM binding and channel function, we studied deletion mutants with and without the IQ motif of the Na_V1.4 CT region. Deletion mutations of the Na_V1.4 CT that preserve the IQ motif (e.g., Na_V1.4₁₇₄₀-EYFP) expressed in HEK293 cells display fluorescence enrichment at the cell perimeter. Line scans of fluorescence intensity are consistent with surface membrane expression of this truncation mutant (Fig. 4 A). Further qualitative analysis of Western blots of purified biotinylated Na_V1.4₁₇₄₀ protein demonstrates expression of the truncated channels at the surface membrane (Fig. 4 B). The family of currents elicited by voltage-clamp pulses of the deletion mutant Na_V1.4₁₇₄₀ is similar to intact Na_V1.4 (Fig. 4 C). The normalized current–voltage (Fig. 4 C) relationships of the Na_V1.4₁₇₄₀ mutant and wild-type channels are nearly identical with the peak current amplitudes at –20 mV. _rec from fast inactivation of truncated channel is 1.7 ± 0.1 ms (n = 5), not significantly different from wild-type channel (1.9 ± 0.1 ms, n = 5; Fig. 4 D). Similarly, truncation of the nonstructured part of CT in Na_V1.4 distal to the IQ region does not significantly alter _entry (1165 ± 17 ms, n = 6), compared with the wild-type channel (1088 ± 20 ms, n = 5; Fig. 4 E). The steady-state inactivation curve of Na_V1.4₁₇₄₀ reveals a V_1/2 of –62.7 ± 0.1 mV (n = 6) and coexpression of ECFP-CaM with Na_V1.4₁₇₄₀ shifts the V_1/2 5 mV (V_1/2 = –68.0 ± 0.1 mV, n = 8, P < 0.04) in the hyperpolarizing direction (Fig. 4 F). Overexpression of ECFP-CaM₁₂₃₄ with Na_V1.4₁₇₄₀ does not shift the availability curve compared with Na_V1.4₁₇₄₀ expression alone (–64.6 ± 0.04 mV, n = 5; Fig. 4 F). Thus the deletion mutant Na_V1.4₁₇₄₀ retains the basic biophysical properties of Na_V1.4 channels and CaM-induced modulation of steady-state inactivation (Table I). These data suggest that the nonstructured distal portion of the CT (after amino acid 1740) is not critical for modulation of channel gating by CaM. In contrast, deletion after amino acid 1723, which includes the entire nonstructured region and the IQ motif of CT-Na_V1.4 (Na_V1.4₁₇₂₃), generated no current (Fig. 4 G). Thus the region containing the IQ motif in Na_V1.4 is essential to functional expression of the channel.

View larger version (37K): [in this window] [in a new window] [Download PPT slide]   Figure 4. NaV1.41740-EYFP preserves CaM-dependent modulation of steady-state inactivation. (A) Epifluoresecence image and intensity profile of NaV1.41740-EYFP expressed with NaVβ1in an HEK293 cell; the peaks indicate membrane targeting. (B) A Western blot of biotinylated surface proteins purified with streptavidin and probed with an anti-NaV antibody (left lane). Total channel proteins are cell lysates that include biotin-labeled (cell surface) and unlabeled channels (the remainder) (right lane). The deletion mutant channel runs just above 197 kD. (C, left) Representative families of NaV1.4-EYFP and NaV1.41740-EYFP currents are similar. (bottom) The normalized IV relationships for NaV1.4-EYFP () and NaV1.41740-EYFP () are not significantly different. (D) Recovery from inactivation of NaV1.41740-EYFP () and NaV1.4-EYFP () are not significantly different. (E) Entry into inactivation of NaV1.41740-EYFP () and NaV1.4-EYFP () are not significantly different. (F) The steady-state inactivation curve of NaV1.41740-EYFP () is shifted in the hyperpolarizing direction by ECFP-CaM () but not by ECFP-CaM1234 (). (G) A truncation of the CT including the IQ region, NaV1.41723-EYFP, eliminates channel function. The data expressed as the means ± SEM and inactivation data are fit to a Boltzmann function.

View larger version (36K): [in this window] [in a new window] [Download PPT slide]   Figure 5. Properties of NaV1.41740-glycine-CaM. (A) Representative raw current records of truncated NaV1.4 channels with CaM linked to the CT by 4 (top, NaV1.41740–G4–CaM) or 14 (bottom, NaV1.41740–G14–CaM) glycine residues. The IV relationships reveal no significant differences between the channels linked to CaM and wild-type NaV1.4 (right). (B) Recovery from inactivation of NaV1.41740–G4–CaM () and NaV1.41740–G14–CaM () are slower than that of wild-type, full-length NaV1.4 (). (C) The rates of entry into inactivated states are similar in NaV1.41740–G4–CaM (), NaV1.41740–G14–CaM (), and wild-type NaV1.4 () channels. (D) Overexpression of wild-type CaM (•) but not CaM1234 () shifts the steady-state inactivation curve in the hyperpolarizing direction compared with NaV1.41740–G4–CaM () or wild-type NaV1.4 () expressed alone. (E) The steady-state inactivation curve of NaV1.41740–G14–CaM () is unaffected by overexpression of CaM () or CaM1234 ().

View larger version (11K): [in this window] [in a new window] [Download PPT slide]   Figure 6. In vivo association of CaM with CT-NaV1.4 by FRET. (A) Donor dequenching FRET in live HEK293 cells expressing the indicated channel constructs. The top three bars in the graph are the FRET efficiencies of control experiments in cells not expressing channels, but expressing ECFP alone, ECFP and EYFP, or the linked chameleon (ECFP-EYFP). NaV1.4-EYFP coexpressed with ECFP or ECFP-CaM1234, or NaV1.4IQ/AA coexpressed with ECFP-CaM yield no detectible FRET. NaV1.4-EYFP coexpressed with ECFP-CaM exhibits significant FRET (>5% efficiency). (B) Peak current densities of expressed NaV1.4 and NaV1.4IQ/AA channels used for FRET measurements. The densities of NaV1.4-EYFP coexpressed with ECFP-CaM or ECFP-CaM1234, or NaV1.4IQ/AA coexpressed with ECFP-CaM are not significantly different from the current density of NaV1.4-EYFP coexpressed with ECFP alone. (C) Interaction of CaM and NaV1.4 assayed by the 33 FRET method. This nondestructive technique confirms the proximity of the fluorophores and the production of FRET in cells expressing NaV1.4-EYFP and ECFP-CaM by a FRET ratio of almost 2. (D) Cells coexpressing NaV1.4-EYFP and ECFP-CaM are held at different membrane voltages to populate different channel conformations. FRET is comparable in cells held at –140 and –60 mV, and is present but reduced at a holding voltage of –20 mV.

The association of CaM with the CT of Na_V1.4 was tested with a complementary, nondestructive FRET measurement technique, 3³ FRET (Erickson et al., 2001). Expression of CT-Na_V1.4-EYFP with ECFP-CaM resulted in a FRET ratio (FR) of >1, with a mean FRET efficiency 8.2% (n = 12; Fig. 6 C), confirming the association of CaM to the CT-Na_v1.4. Consistent with the donor dequenching FRET results, the 3³ FRs were <1 in cells expressing the Na_V1.4_IQ/AA channel with CaM (Fig. 6 C). Thus FRET is the result of a specific CaM–channel interaction at the IQ motif.

To understand the mechanism of modulation of inactivation of Na_V1.4 we examined the voltage dependence of the interaction of CaM and its proximity to the CT fluorescent Na channel tag. We measured donor dequenching FRET between Na_V1.4-EYFP and ECFP-CaM while holding the channels at three different potentials: –140 mV (favoring closed channels), –60 mV (V_1/2 of the inactivation curve), and –20 mV (favoring inactivated channels). Coexpressing ECFP-CaM and Na_V1.4-EYFP enhanced the ECFP signal in patch-clamped cells held at –140 mV, leading to a mean 22.7 ± 2.0% (n = 15) FRET efficiency, which is significantly (P < 0.0006) higher than the FRET efficiency of unpatched cells (Fig. 6 D). Similarly, at a holding voltage of –60 mV, a mean FRET efficiency of 25.4 ± 1.8% (n = 9) was observed (Fig. 6 D). However, holding at –20 mV yielded a FRET efficiency (9.9 ± 2.3%, n = 15) similar to FRET of unpatched cells (Fig. 6 D). CaM does not appear to dissociate from the channel in the closed or inactivated conformations.

CaM Influences Channel Trafficking
CaM binding to the CT of Na_V1.4 under resting conditions and studies describing reduced current density by expressed Na_V channel isoforms that have been mutated to impair CaM binding (Cormier et al., 2002; Herzog et al., 2003) suggest that CaM binding influences channel trafficking and surface expression. In addition to calmodulation of steady-state inactivation of Na_V1.4, we assessed whether CaM influenced channel trafficking and expression. Lysates isolated from cells expressing wild-type or mutant Na_V1.4_IQ/AA channel proteins were separated on SDS-PAGE gels (Fig. 7 A) and band intensities were measured to estimate the level of total channel expression. To assess effect of CaM binding on surface expression, cells expressing wild-type or mutant Na_V1.4_IQ/AA channels were labeled with membrane-impermeable biotin and purified with streptavidin beads. The band intensities of biotinylated proteins, representing cell surface expression, were normalized to the respective total channel protein expression and plotted in Fig. 7 B. The Na_V1.4_IQ/AA mutant exhibits significantly (P 0.05, n = 4) reduced surface expression compared with wild-type Na_V1.4 and the truncation mutant distal to the IQ, Na_V1.4₁₇₄₀ (Fig. 7 B). Truncation of Na_V1.4 further upstream at residue 1723 (Na_V1.4₁₇₂₃) eliminates channel function (Fig. 4 G) but does not eliminate cell surface expression, as detected by Western blot and epifluorescence microscopy (Fig. S2, available at http://www.jgp.org/cgi/content/full/jgp.200709863/DC1). The data suggest that the CaM binding region of the intact CT of Na_V1.4 is essential for functional cell surface channel expression. To further examine trafficking of the IQ mutant channel, Na_V1.4-EYFP or Na_V1.4_IQ/AA-EYFP were expressed in HEK293 cells, and the cellular channel protein distribution was examined with confocal microscopy. Fluorescence from EYFP-fused wild-type channels was distributed in both the periphery and center of the cell, consistent with trafficking from perinuclear membranes to cell surface (Fig. 7 C). In contrast, signals from the Na_V1.4_IQ/AA-EYFP mutant channels were predominantly in the perinuclear region, indicating mutant channels are synthesized but remain trapped in intracellular membranes (Fig. 7 D). Compared with the wild-type Na_V1.4 channel, more Na_V1.4_IQ/AA channels remain internalized, consistent with the reduced surface expression of the Na_V1.4_IQ/AA protein observed in Western blot analysis (Fig. 7, A and B). Although the IQ/AA mutation interferes with cell surface trafficking of Na_V1.4, truncation of the CT proximal to IQ generates nonfunctional channels that are expressed on the cell surface. It is possible that the IQ/AA mutation creates a signal that mediates retention in subcellular membranes such as the ER. This mutation-mediated retention signal is eliminated by truncation of the IQ motif (i.e., Na_V1.4₁₇₂₃), resulting in normal surface membrane trafficking of nonfunctional channels. Either the IQ motif itself or CaM binding to IQ promotes a structure of this region of the CT, likely involving residues between 1723 and 1740, that is trafficked to the cell surface.

View larger version (40K): [in this window] [in a new window] [Download PPT slide]   Figure 7. Influence of CaM on NaV1.4 channel expression and localization. (A) Western blots of lysates from HEK293 cells transfected with wild-type NaV1.4 and mutant NaV1.4IQ/AA channels reveal a reduction in surface expression of NaV1.4 protein by the IQ/AA mutation compared with wild type with no significant change in immunoreactive protein in total cell lysates. The protein is detected with the antibodies described in Fig. 1. (B) The ratio of cell surface expression to total expression of NaV1.4IQ/AA is significantly (P 0.05, n = 4) reduced compared with wild-type NaV1.4 and NaV1.41740. (C) Confocal images of NaV1.4-EYFP expressed in HEK293 cells. EYFP-fused wild-type channels are distributed in both the periphery and center of the cell. The right panel is a DIC image and bottom panel is the merge of the DIC and fluorescence images. (D) In contrast, NaV1.4IQ/AA mutant channels fused to EYFP are predominantly distributed in the perinuclear region of the cell, indicating mutant channels are synthesized but remain trapped in internal membranes. The images are as described in C.

	DISCUSSION

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

CaM acts as a channel subunit binding to a C-terminal IQ motif, and a calcium sensor for calcium-dependent inactivation of Ca_V1.2 (Peterson et al., 1999; Zuhlke et al., 1999; Erickson et al., 2001; Van Petegem et al., 2005). An homologous IQ binding domain is present in all Na_v1 sodium channel isoforms; however, CaM's interaction with Na_V channels and its functional effects appear to be isoform specific (Mori et al., 2000; Deschênes et al., 2002; Kim et al., 2004; Young and Caldwell., 2005; Choi et al., 2006). To begin to understand the isoform-specific functional effects of Ca²⁺/CaM/CaMK on Na_V1 isoforms and the role of the IQ motif and alternate sites of CaM and apo-CaM interaction we have examined the effect of CaM binding to the CT of skeletal muscle channel, Na_V1.4.

CaM Is Tethered to Intact Na_v 1.4 through an IQ Motif
Our data conclusively demonstrate tethering of CaM to the CT of intact Na_V1.4 channels in live cells. Deletion mutations of the Na_V1.4 CT that preserve the IQ motif (Na_V1.4₁₇₄₀) generated currents that had voltage dependences and kinetics of activation and inactivation that were similar to wild-type Na_V1.4 (Fig. 4, C and F). In contrast, deletion of the entire nonstructured region and part of the terminal -helix including the IQ motif (Na_V1.4₁₇₂₃) exhibit no current (Fig. 4 G), indicating that the region containing the IQ motif and CaM binding to this motif in Na_V1.4 is indispensable for normal sodium channel functional expression. CaM tethering to the IQ region was further confirmed by the absence of an effect of CaM₁₂₃₄ on the CaM-induced shift in gating of Na_V1.4 (Fig. 3 A). In contrast, the effects of AIP290-309 (CaM anti-peptide) are more complex and independent of CaM binding to the channel at the IQ motif (Fig. 3, B–E). AIP290-309 alters the gating of wild-type and IQ/AA mutant Na_V1.4 channels. Inactivation of Na_V1.4_IQ/AA is destabilized by AIP290-309 independent of the presence of CaM overexpression (Fig. S1), whereas, steady-state inactivation of Na_V1.4 is shifted to depolarized potentials by AIP290-309 with no effect on the IV curve or recovery from inactivation. The effects of AIP290-309 on wild-type Na_V1.4 gating are eliminated by overexpression of CaM (Fig. 3 B). Whether AIP290–309 interacts with the channel directly and the site(s) of that interaction remain uncertain. The effects of AIP290-309 on Na_V1.4_IQ/AA do not appear to be the result of a general inhibition of endogenous CaM function as overexpression of CaM does not mitigate the AIP290-309–induced changes in Na_V1.4_IQ/AA gating.

In resting cells, wild-type CaM increased the donor dequenching FRET signal in tagged, presumably inactivated Na_V1.4 channels (Fig. 6, A and C). Changing the membrane voltage did not eliminate FRET, suggesting that CaM is tethered to the CT of Na_V1.4 in all channel conformations; however, the proximity of the fluorophores may be different in channels subjected to depolarized voltages for extended periods of time (slow inactivated states). In any case, these data confirm the importance of the IQ motif in the CT for CaM binding and modulation of the voltage dependence of gating of Na_V1.4 channels. This is in contrast to a previously proposed mechanism of gating for voltage-gated cardiac sodium channels, Na_V1.5 (Shah et al., 2006), where CaM has been proposed to bind to the IQ motif at resting Ca²⁺ levels, but later dissociates from the CT upon Ca²⁺ binding, thus enabling the CaM-free IQ motif to interact with an EF hand motif in the CT of the channel. However we observed wild-type Na_V1.4 and mutant Na_V1.4_IQ/AA are both regulated by Ca²⁺ in the presence of endogenous CaM (unpublished data). Moreover, CaM-mediated regulation of Na_V1.4 is lost in the absence of Ca²⁺, consistent with Ca²⁺-dependent CaM regulation of Na_V1.4 gating (Deschênes et al., 2002). Finally, Na_V1.4_IQ/AA mutant channels are not regulated by CaM but retain sensitivity to Ca²⁺, thus at least one form of Ca²⁺-mediated regulation of channel gating does not require an interaction between the IQ motif and the EF hand. The loss of FRET between CaM and Na_V1.4_IQ/AA and the absence of an interaction between wild-type Na_V1.4 and CaM₁₂₃₄ indicates that CaM-Ca²⁺ binds to the CT via the IQ motif. CaM-Ca²⁺ regulation of channel gating is mediated principally through Ca²⁺ binding to CaM complexes with IQ in the Na_V1.4-CT.

A Functional Model for the Regulation of Na_V1.4 Channel Gating by CaM
The conformation-independent tethering of CaM to the IQ motif is central to the model presented. Additional electrophysiogical evidence supports the idea that CaM does not dissociate from the IQ motif in Na_V1.4. First, overexpression of CaM₁₂₃₄ does not eliminate the CaM-mediated effect on steady-state inactivation, indicating its only CaM-mediated regulation (Fig. 3 A). Second, overexpression of both CaM and CaM₁₂₃₄ shows similar regulation to that exhibited by CaM alone (Fig. 3 B), indicating that the Ca²⁺ binding–deficient CaM₁₂₃₄ does not displace CaM. Finally, among the variable length glycine–linkered CaM fused to CT only the linker length that allows CaM to reach IQ region exhibits CaM modulation of gating, indicating one CaM molecule is sufficient for regulation of inactivation (Fig. 5, D and E). Overall the data are consistent with CaM being tethered to the CT-Na_V1.4 during normal gating.

The IQ motifs are highly conserved across Na_V isoforms, suggesting an important functional role for these regions. It is conceivable that the cytoplasmic tail of Na_V1.4 exists in a disordered form under basal depolarized conditions, when subjected to more polarized voltages, the cytoplasmic tail could be more structured due to an increase in helicity, leading to an altered binding relationship of CaM and the IQ motif (Fig. 6 D). It is possible that the binding of CaM to the more structured CT facilitates interactions with other cytoplasmic domains at pore mouth that participate in and stabilize inactivation. Further structural characterization of the Na_V1.4-CT and its interactions with CaM are required to critically test this hypothesis and will aid in understanding the role of CaM binding in various cardiac and muscular disorders.

Role of CaM Binding in Surface Expression of Na_V1.4
We demonstrate that CaM participates in the modulation of cell surface expression of intact Na_V1.4 channels by interaction with the IQ motif similar to other channels such as KCNQ1 (Ghosh et al., 2006), SK4 channels (Joiner et al., 2001; Lee et al., 2003), and KCNQ2/Q3 potassium channels (Wen and Levitan., 2002). It has been suggested that CaM behaves as an obligate subunit of the calcium channel, Ca_V1.2, altering both function and expression of this subunit. Similarly, CaM acts as an obligate subunit of some Na_V1 channels, necessary for proper folding (Kim et al., 2004). Our data reveal that mutations in the CaM binding motif reduce total and cell surface expression of Na_V1.4. More proximal truncations of the channel that include the IQ motif (Na_V1.4₁₇₂₃, Fig. 3 G and Fig. S2) support a role for other regions of the CT of the Na channel in both function and expression. It is possible that the IQ/AA mutation leads to defects in proper channel folding; thus the role of CaM could be in stabilization of proper channel folding and facilitating trafficking of the channel to the cell surface. CaM regulation of channel trafficking to the cell surface and its role in the early stages of channel formation could be a general phenomenon further adding to the diversity of the CaM signaling on ion channel function.

Our data demonstrate an intimate relationship between intact Na_V1.4 channels and CaM that influences channel gating and functional expression, and that a single CaM molecule is sufficient to regulate Na_V1.4 inactivation gating. In live cells, CaM is associated with CT-Na_V under resting conditions and CaM remains tethered to the CT-Na_V over a wide range of voltages, indicating no significant displacement of CaM from any channel conformation. The Na_v1.4_IQ/AA mutant eliminates the proximity of CaM to CT-Na_V1.4 and reduces Na_V1.4 surface expression. Thus CaM is tethered to CT-Na_V1.4 at the IQ motif and is essential for normal inactivation gating of Na_V1.4, functions to stabilize channel conformation, and promotes membrane trafficking of the channel protein.

	ACKNOWLEDGMENTS

 
We acknowledge financial support from the National Institutes of Health (RO1HL50411). Gordon F. Tomaselli holds the David J. Carver Professorship in Medicine at the Johns Hopkins University.

Angus C. Nairn served as editor.

Submitted: 31 July 2007
Accepted: 24 January 2008

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