Activation and Inactivation of the Voltage-Gated Sodium Channel: Role of Segment S5 Revealed by a Novel Hyperkalaemic Periodic Paralysis Mutation

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The Journal of Neuroscience, June 15, 1999, 19(12):4762-4771

Activation and Inactivation of the Voltage-Gated Sodium Channel: Role of Segment S5 Revealed by a Novel Hyperkalaemic Periodic Paralysis Mutation
Saïd Bendahhou¹, Theodore R. Cummins²^,³, Rabi Tawil⁴, Stephen G. Waxman²^,³, and Louis J. Ptácek¹
¹ Howard Hughes Medical Institute, Eccles Institute of Human Genetics, University of Utah, Salt Lake City, Utah 84112, ² Departments of Neurology and Pharmacology, Yale University School of Medicine, New Haven, Connecticut 06510, ³ Neuroscience Research Center, Veterans Administration Medical Center, West Haven, Connecticut 06516, and ⁴ Department of Neurology, University of Rochester, Rochester, New York 14642

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Hyperkalaemic periodic paralysis, paramyotonia congenita, and potassium-aggravated myotonia are three autosomal dominant skeletalmuscle disorders linked to the SCN4A gene encoding the $alpha$ -subunitof the human voltage-sensitive sodium channel. To date, ~20 pointmutations causing these disorders have been described. We haveidentified a new point mutation, in the SCN4A gene, in a familywith a hyperkalaemic periodic paralysis phenotype. This mutationpredicts an isoleucine-to-phenylalanine substitution at position1495 located in the transmembrane segment S5 in the fourth homologousdomain of the human $alpha$ -subunit sodium channel. Introduction ofthe I1495F mutation into the wild-type channels disrupted themacroscopic current inactivation decay and shifted both steady-stateactivation and inactivation to the hyperpolarizing direction.The recovery from fast inactivation was slowed, and there wasno effect on channel deactivation. Additionally, a significantenhancement of slow inactivation was observed in the I1495F mutation.In contrast, the T704M mutation, a hyperkalaemic periodic paralysismutation located in the cytoplasmic interface of the S5 segmentof the second domain, also shifted activation in the hyperpolarizingdirection but had little effect on fast inactivation and dramaticallyimpaired slow inactivation. These results, showing that the I1495Fand T704M hyperkalaemic periodic paralysis mutations both haveprofound effects on channel activation and fast-slow inactivation,suggest that the S5 segment maybe in a location where fast andslow inactivationconverge.

Key words: Na channel; SCN4A; disorders; activation; slow inactivation; expression

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Naturally occurring mutations are a powerful tool to study the relationship between protein structure and function. They havebeen widely used in the past decade to study integral membraneproteins for which crystal structures are difficult to obtain.This has been successfully applied to the functional analysisof the voltage-gated sodium channels. The sodium channel $alpha$ -subunitis 260 kDa and associates with small $beta$ -subunits in muscle andbrain. According to sodium channel models, the $alpha$ -subunit is organizedin four homologous domains (I-IV), and each domain is representedby six membrane spanning segments (S1-S6) (Noda et al., 1984).Two fragments located between segments S5 and S6 (SS1-SS2) arebelieved to form the poreregion.

Over 20 single mutations affecting the human sodium channel gene SCN4A (encoding the human skeletal muscle isoform) have beenlinked to three autosomal dominant disorders: hyperkalaemic periodicparalysis (HyperKPP) (Ptácek et al., 1991; Rojas et al., 1991),paramyotonia congenita (PC) (Ptácek et al., 1992; McClatcheyet al., 1992), and potassium-aggravated myotonia (PAM) (Lercheet al., 1993; Ptácek et al., 1994). All channel domains carryat least one disease-causing mutation, and all transmembrane segmentsseem to be targeted, except the membrane spanning segments S2and S5 (for review, see Bulman, 1997). Many of these mutationshave been overexpressed in Xenopus oocytes or in mammalian heterologoussystems. These studies demonstrated the existence of many defectsin channel function that may underlie either muscle hyperexcitabilityor inexcitability, such as the presence of sustained inward current,shift in steady-state inactivation or activation, alteration ofchannel deactivation, modification of channel recovery from fastinactivation, and impairment of slowinactivation.

Five point mutations have been reported to affect the human sodium channel gene SCN4A causing HyperKPP: T704M (Cannon andStrittmatter, 1993; Cummins et al., 1993; Yang et al., 1994; Cumminsand Sigworth, 1996; Hayward et al., 1997), V781I (Baquero et al.,1995), A1156T (Yang et al., 1994), M1360V (Wagner et al., 1997),and M1592V (Hayward et al., 1997). A recent study of the V781Imutation in human embryonic kidney (HEK) 293 cells suggested thatthis mutation may be a benign polymorphism (Green et al., 1997).All of these HyperKPP mutations show a common feature; they arelocalized at the intracellular membrane interface. HyperKPP-causingmutations have not been found in the extracellular loops or inthe middle of any membrane spanning domain to date. We reporthere a novel missense mutation in the SCN4A in a patient withHyperKPP, causing the amino acid change from isoleucine to phenylalanineat position 1495 located within the putative transmembrane segmentS5 of domain IV. We have also performed additional comparativeexperiments on the most common HyperKPP mutation (T704M), locatedat the intracellular interface on the S5 segment of the sodiumchannel.

This is the first report of a naturally occurring mutation in the S5 segment, and naturally occurring mutations in this segmentmay allow a better understanding of the disease and define therole of segment S5 in sodium channelfunction.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Identification of a HyperKPP patient. The patient was examined by one of the authors (R.T.). The proband underwent a physicalexamination, a potassium-loading test, and electromyography. Allhuman tissue samples used in this project were obtained with theapproval of the Institutional Review Board at the University ofUtah Health SciencesCenter.

Genetic analysis. Genomic DNA was extracted from peripheral blood leukocytes and amplified using PCR as described previously(Ptácek et al., 1992). Single strand conformation polymorphism(SSCP) analysis was performed on amplified DNA using a protocoldescribed previously (Ptácek et al., 1992). The primers usedwere as follows: 5'-CCTCCTCCTCTTCCTGGTCAT-3' (Nb forward) and5'-GGGCTCGCTGCTCTCCTCTGT-3' (Nbreverse).

Cell culture and transfection. HEK 293 cells were grown in DMEM supplemented with penicillin, streptomycin, and 10% fetalcalf serum (Life Technologies, Gaithersburg, MD) and maintainedat 37°C with 5% CO₂. The calcium-phosphate precipitation technique(Graham and Van Der Eb, 1973) was used for both transient andstable transfections. HEK 293 cells were grown on a 35 mm culturedish (Corning, Corning, NY) and transfected at 30% confluence.Approximately 15 hr after transfection, the media was changed.Stably expressing cell lines were produced using the expressionvector pRc-CMV encoding either wild-type (WT) human skeletal musclevoltage-gated sodium channel or the corresponding I1495F mutantconstruct (Bendahhou et al., 1995).

Construction of hSkM1-I1495F and hSkM1-T704M. The hSkM1-I1495F was constructed using the megaprimer PCR method of site-directedmutagenesis (Sarkar and Sommer, 1990). Wild-type cDNA (hSkM1)was used as a template for the first round of PCR to generatetwo megaprimers (1.3 kb). The reaction was primed with an oligo-nucleotideencoding a region corresponding to nucleotides (nt) 3736-3755of the full-length channel sequence 5'-GGCTCAATGTCAAGGTCAAC-3'and the oligo encoding sequence (nt 4550-4569) 5'-TGGAGTAGGTGAACATGACC-3'(reverse). The first round PCR reaction protocol was as follows:2 min at 94°C for one cycle; 20 sec at 94°C, 20 sec at 60°C, and1 min at 75°C for 30 cycles; and 5 min at 72°C for onecycle.

The second megaprimer set was generated using oligo-nucleotides (nt 4550-4570) 5'-GGTCATGTTCACCTACTCCA-3' and (nt 5079-5098)5'-TGGGCAAGTCCAGTGTGATG-3' (reverse). The first round PCR reactionprotocol for this primer set was as follows: 2 min at 94°C forone cycle; 20 sec at 94°C, 20 sec at 50°C, and 1 min at 75°C for30 cycles; and 5 min at 72°C for onecycle.

The primer contained a nucleotide substitution T4561C (indicated above by an italic letter), which results in the amino acidsubstitution I1495F. The second round of PCR was primed usingfirst round products (megaprimers) and the primers 5'-GGCTCAATGTCAAGGTCAAC-3'(forward) and 5'-TGGGCAAGTCCAGTGTGATG-3' (reverse). The followingprotocol was used for the second round PCR: 2 min at 94°C forone cycle; 20 min at 94°C, 20 sec at 54°C, and 90 sec at 72°Cfor 30 cycles; and 5 min at 72°C for one cycle. A 1.3 kb productwas isolated from a 1% agarose gel using the Qiagen (Hilden, Germany)gel extraction kit, cut with SseI restriction enzyme and ligatedto the appropriately cut fragment of wild-type hSkM1 (the pRc-CMV-hSkM1construct was initially cut with SseI enzyme to separate a 10kb band from the 1.3 kb wild-type band) to construct the full-lengthmutated channel hSkM1-I1495F.

All PCR reactions were performed in DNA Engine Tetrad (MJ Research, Watertown, MA). DNA sequencing was performed using eitherApplied Biosystems (Foster City, CA) dRhodamine dye terminatorsor Applied Biosystems Prism BigDye Terminators and cycle sequencingwith Taq FS DNA polymerase. DNA sequence was collected and analyzedon an Applied Biosystems Prism 377 automated DNA sequencer. Allprimers were synthesized on a 394 automated DNA synthesizer (AppliedBiosystems) following standard ABIprocedures.

The hSkM1-T704M construct was engineered as described previously (Yang et al., 1994)

Electrophysiology. Recordings were conducted in the whole-cell configuration (Hamill et al., 1981) at room temperature (22°C)using an Axopatch 200B amplifier (Axon Instruments, Foster City,CA) and an EPC-9 amplifier. Data acquisition and analysis wereperformed with pClamp6 (Axon Instruments) or Pulse and Pulsefit(Heka Elektronik, Lambrecht/Pfalz, Germany), and Igor Pro (WaveMetricsInc., Lake Owego, OR) programs. Pipettes (Kimax; Kimble GlassInc.) of 0.8-1.5 M $Omega$ were prepared using a Sutter (Novato, CA)P-87 puller and were heat-polished before use. The pipette tippotential was adjusted to zero for each experiment. To minimizespace-clamp problems caused by the electrical coupling betweenHEK 293 cells, only isolated cells with a soma size of 10-30 µmwere selected for recordings. Cells were not considered for analysisif the initial seal resistance was <5 G $Omega$ or if the cells had highleakage currents (holding current of >0.1 nA at $-$ 80 mV), membraneblebs, or an access resistance >3 M $Omega$ . Linear leak subtraction,based on the resistance estimates from 4-6 hyperpolarizing pulsesapplied before the depolarizing test potential, was used for allvoltage-clamprecordings.

Pulse protocols. Steady-state activation was studied by measuring the peak sodium conductance (G_Na) during a 25 msec testpulse to various test potentials from $-$ 120 mV holding voltage.G_Na was calculated from G_Na = I_Na/(V $-$ V_rev), where I_Na is thepeak sodium current during the test depolarization (V), and V_revis the sodium reversal potential. Data were normalized to maximumpeak conductance (G_max) and fit to a two-state Boltzmann distribution:G_Na/G_max = (1 + exp[ze(V $-$ V_0.5)/kT])¹, where V_0.5 is the potential for half-maximal activation, k isthe Boltzmann constant, z is the apparent gating charge, T theabsolute temperature, and kT/e = 25 mV at 22°C.

To study steady-state fast inactivation, cells were held at prepulse potentials ranging from $-$ 130 or $-$ 120 to +20 mV for 200msec and then subjected to a 0 mV test pulse for 25 msec. Normalizedpeak currents were plotted versus prepulse potentials, and curveswere fitted by the Boltzmann function: I/I_max= (1 + exp[ze(V $-$ V_0.5)/kT])¹, where I_max is the current recorded at 0 mV after the most hyperpolarizingprepulse, and k, T, z, and e are the same as describedabove.

For the development of fast inactivation, the holding potential was $-$ 100 mV. A series of prepulses ranging from $-$ 80 to $-$ 50mV for increasing durations were applied before a test pulse at $-$ 20 mV for 20 msec to determine the fraction of current inactivatedduring theprepulse.

Recovery from fast inactivation was studied by prepulsing the cells to $-$ 20 mV for 20 msec to inactivate all of the current,and then recovery potentials from $-$ 140 to $-$ 60 mV for increasingrecovery durations were applied before the test pulse to $-$ 20 mV(20 msec) to assay the fraction of current recovered. Normalizedpeak current amplitudes were plotted and fitted to a single-exponentialfunction (a₀ + a₁ exp( $-$ t/t)), and the time constant wasdetermined.

Steady-state slow inactivation. The first step consists of holding the cells at potentials ranging from $-$ 130 to 10 mV in 10mV steps for 50 sec. A 30 msec recovery pulse to $-$ 100 mV and a20 msec test pulse to $-$ 10 mV were given before the holding potentialwas incremented again. The holding potential was incremented by10 mV immediately after each recovery pulse-test pulse sequence.We term this protocol sequential because the channels are notallowed to recover from slow inactivation for each test pulse;the expectation is that the sequential changes in holding potentialwill mimic changes in holding potential of longer durations. Theshort hyperpolarizing recovery pulses can be used to remove fastinactivation just before a test pulse to measure slow inactivationprocesses (Simoncini and Stühmer, 1987). The peak current elicitedby the test pulse to $-$ 10 mV was plotted as a fraction of the maximumcurrent. Steady-state slow inactivation data were fitted witha Boltzmann function as described for fastinactivation.

Slow inactivation recovery. Cells were held at $-$ 20 mV for at least 15 min to allow slow inactivation to reach steady-stateequilibrium. Short recovery times were monitored with individualrecovery pulses. Once every 50 sec, the cells were allowed torecover at $-$ 100 mV for increasing durations (from 1 to 500 msec),followed by a 20 msec test pulse to $-$ 10 mV. After the last shortrecovery pulse sequence, the cells were held at $-$ 20 mV for anadditional 50 sec, after which the holding potential was switchedto $-$ 100 mV and recovery was monitored in a continuous recording,with $-$ 10 mV test pulses at 0.5 sec intervals for 10 sec, thenat 5 sec intervals for 110 sec, and finally at 15 sec intervalsfor 5 min. This protocol allowed us to monitor a complete recoveryprofile to >7min.

Twenty-four hours after plating stable lines or 36 hr after transfection, culture dishes containing cells were transferredto the stage of an inverted microscope. The culture media wasremoved and replaced with a bathing solution containing (in mM):140 NaCl, 4 MgCl₂, 2 CaCl₂, and 10 Na-HEPES, pH 7.3. The internalpipette solution was (in mM): 130 CsCl, 4 MgCl₂, 2.5 EGTA, 5 NaCl,and 10 HEPES, pH 7.3. We have not observed significant differencesin the sodium current properties when CsF is used instead ofCsCl.

Values represent means ± SEM. Statistical data were obtained using ttest.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Evaluation of patient

The patient is a 48-yr-old man who initially noted episodic weakness induced by rest after exercise. The attacks had onsetat age 16 and are not affected by cold temperatures or dietarychanges. His episodes of weakness were associated with crampingpain in his muscles. No symptoms suggestive of myotonia were reported;he has no paradoxical eye closure myotonia or lid lag myotonia.Similarly, no percussion or action myotonia is noted in his limbs.He has developed progressive fixed weakness in his proximal lowerextremities, and significant wasting in his quadriceps muscles.In addition to the striking atrophy of his quadriceps and hamstrings,he had significant calf hypertrophy, as well as well developedupper extremity musculature. The level of creatine kinase waselevated at 523 IU/l (normal is 0-243 IU/l). The patient evaluationincluded an electromyogram, which showed no evidence of myotonicdischarges. The patient was challenged with a sugar-free potassiumchloride solution. This resulted in a peak potassium level (6.1mmol/l; normal is 3.4-4.7 mmol/l) ~90 min after ingestion, witha concomitant loss of strength noted in his grip, as well as moredramatically in his hip flexors and kneeextensors.

The patient was treated variously over the years with acetazolamide, thiazide diuretics, or tocainide. None of these pharmacologicalinterventions prevented the attacks. Although both parents aredeceased and their affected status is not known, he has an affectedolder brother andnephew.

Identification of nucleotide alterations in the patient DNA

DNA from the patient was amplified using primers for exon 24 as described in Materials and Methods. An aberrant SSCP conformerwas noted in this patient and his brother. Sequence analysis ofthe aberrant conformer revealed a T4561C mutation (data not shown)of the SCN4A gene that predicts an isoleucine-to-phenylalaninechange at position 1495 in the human skeletal muscle sodium channel $alpha$ -subunit. This mutation was absent in 106 normal unrelated individuals.This amino acid is located in the membrane spanning segment S5of domain IV and is perfectly conserved among all voltage-gatedsodium channels sequenced to date from Drosophila to human (Fig.1).

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Figure 1. Alignment of the segment IV-S5 of the sodium channel. Segment S5 of domain IV deduced amino acid sequence of the voltage-gated sodium channel from human skeletal muscle (hSkM1), human cardiac muscle (hSkM2), rat brain type II (RII), eel electroplax, squid giant axon (Squid), TTX resistant from dorsal root ganglia (DRG), jellyfish, and Drosophila para, along with isoleucine 1495-to-phenylalanine substitution. This figure shows that isoleucine 1495 is well conserved among voltage-gated sodium channels.

Fast inactivation

A common feature of the majority of the naturally occurring mutations causing HyperKPP or PC is a sustained or noninactivatingsodium current. To check for the presence of this component inthe hSkM1-I1495F channels, cells were first held at $-$ 120 mV andthen depolarized to different potentials for 25 msec. Figure 2illustrates the behavior of wild-type channels (Fig. 2A) and thehSkM1-I1495F (Fig. 2B) expressed in HEK 293 cells, in responseto increasing depolarizing pulses. The mutant channels revealan additional sustained sodium current. This is better illustratedin Figure 2C in which two normalized current traces (at $-$ 10 mV)from wild-type and I1495F channels are superimposed to show thedefect in the fast inactivation decay. Increasing the test pulseduration to 100 msec also shows the presence of this prolongedinward sodium flow (Fig. 2D). However, when currents were recorded10 min after rupturing into the cell, the sustained inward currentwas absent (data not shown). This may indicate that the prolongedinward current seen during the first minutes of recording is subjectto modulation. Whatever the reason, early recordings indicatethat the S5 segment may be involved in channel inactivation.

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Figure 2. Effect of I1495F mutation on macroscopic currents. Cells were held at $-$ 120 mV, and inward sodium currents were elicited by 10 mV voltage steps from $-$ 80 to 20 mV for WT (A) and I1495F (B). C shows normalized current traces from WT and I1495F mutant recorded at $-$ 10 mV. D, An example of superimposed current recordings from WT and I1495F channels using the same pulse protocol as in A-C for a 100 msec duration.

The inactivation phase was fitted with a single exponential at different voltages. A single-exponential function was sufficientfor fitting wild-type currents, whereas a two-exponential functionwas necessary to obtain an accurate fit of sustained I1495F currents(Fig. 3A). The HyperKPP current decay exhibits two components:one that is fast with a time constant slightly faster than WTthroughout the range of potentials tested, and the second decayingwith a slow time constant representing the sustained channelsshown in the traces in Figure 2, C and D (Fig. 2B-D).

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Figure 3. Inactivation kinetics of I1495F. A, Time constant of fast inactivation for WT (filled circles, n = 39) and I1495F (open circles, n = 14) showing an additional slow component (open squares, n = 14) for the HyperKPP mutant channels. B, Steady-state fast inactivation. HEK 293 cells were subjected to a protocol described in Materials and Methods to generate the inactivation curves for WT (filled circles, n = 43) and I1495F (open circles, n = 31).

A sustained sodium current could be the result of an increase in the "window current" caused by a positive shift of the steady-stateinactivation, a negative shift of the activation curve, or both.To test for changes in steady-state fast inactivation, cells wereheld over a range of potentials for 200 msec, which allows thechannels to undergo fast inactivation without allowing the channelsto slowly inactivate, and then depolarized to a test pulse (0mV) to measure the fraction of channels that did not fast inactivate.Figure 3B shows that the mutant channels inactivate at more hyperpolarizingpotentials than the wild type. The midpoint of inactivation wasshifted by $-$ 10 mV (WT, V_0.5 = $-$ 62.1 ± 4.9 mV; n = 43; I1495F,V_0.5 = $-$ 72.3 ± 4.3 mV; n = 31), and this significant shift (p< 0.001) was not transient. This hyperpolarizing shift of theinactivation curve has not been reported in a pure HyperKPP mutantbut was rather seen in mutations occurring at position 1448, R1448P,C, H (Chahine et al., 1994; Yang et al., 1994), or S (S. Bendahhou,T. R. Cummins, H. Kwiecinski, S. G. Waxman, and L. J. Ptácek,unpublished observations), causing PC. However, there is no significantchange (p = 0.1) in the slope of the inactivation curve for I1495Fchannels (WT, z = 3.9 ± 0.7; n = 26; I1495F, z = 3.7 ± 0.5; n= 30) as reported for the different substitutions at position1448 of the human skeletal muscle sodiumchannel.

Steady-state activation

As mentioned above, a sustained inward sodium current could result from a negative shift in the voltage dependence of theactivation. Figure 4A shows the current-voltage relationship forWT and I1495F channels. The I1495F channels activate at more negativepotentials. This shift is better seen by transforming the current-voltagerelationship to a conductance-voltage curve (Fig. 4B). The steady-stateactivation is significantly shifted (p < 0.001) to the left forthe hSkM1-I1495F by ~8 mV (WT, V_0.5 = $-$ 17.7 ± 3.0 mV; n = 47;I1495F, V_0.5 = $-$ 25.5 ± 3.7 mV; n = 31). There was no significantchange (p = 0.05) in the apparent gating charge between the twoconstructs (WT, z = 4.2 ± 0.6; n = 47; I1495F, z = 4.0 ± 0.4;n = 31). In addition to its role in channel inactivation (indicatedby the presence of sustained current flow and the shift in theinactivation curve), our data also suggest an involvement of theS5 segment of domain IV in channel activation.

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Figure 4. WT and I1495F activation parameters. The pulse protocol for constructing the current-voltage relationship is described in Materials and Methods. A, The current-voltage curves for WT (filled circles, n = 47) and I1495F (open circles, n = 31) were normalized for a better appreciation of the shift between the two relations. B, Currents were converted to conductance, and fit was made according to the Boltzmann function described in Materials and Methods. Symbols are the same as in A.

Deactivation, development, and recovery from fast inactivation in I1495F

A defect in channel deactivation may favor prolonged action potentials, as shown in a model of muscle membrane excitability(Featherstone et al., 1998). To examine this, tail currents, resultingfrom a brief 40 mV pulse preceding a command potential rangingfrom $-$ 120 to 0 mV, were recorded, and traces were fitted witha single-exponential function. As shown in Figure 5, kineticsof deactivation of the I1495F channels are not different fromWT channels. However, when testing for recovery from fast inactivation,the fraction of channels recovered after a prolonged $-$ 80 mV conditioningpulse was smaller for I1495F channels than for the WT channels(Fig. 5B), suggesting a slower recovery from fast inactivationfor the mutant channels. The time constants for slow recoveryfrom fast inactivation are illustrated in Figure 5C, which plotsthe time constant at each potential tested. However, developmentof fast inactivation seems to be enhanced at negative voltagesin the I1495F channels, indicating that closed-state inactivationis enhanced in the I1495F mutation.

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Figure 5. Deactivation, development, and recovery from inactivation for I1495F. A, Tail currents were elicited by a 0.5 msec test pulse to 40 mV, followed by repolarization pulses ranging from $-$ 120 to 0 mV. Resulting currents were fitted by a single-exponential decay and expressed as function of the voltage for WT (filled circles, n = 20) and for I1495F (open circles, n = 20). B, To assess the rate of recovery from fast inactivation, the following protocol was applied to HEK 293 cells: channels were fast inactivated during 200 msec using 0 mV voltage pulse, then they were allowed to recover at different voltages ( $-$ 80 mV test pulse is shown as an example) for an increasing time, and finally a 0 mV test pulse was applied to test for the fraction of the channels recovered. Peak currents obtained using the test pulse were normalized to the peak current obtained during the inactivating pulse for WT (filled circles, n = 14) and I1495F (open circles, n = 26). C, Data for development of inactivation (squares) and recovery from fast inactivation (circles) were fitted to a single-exponential function and plotted as a function of the development-recovery pulse voltage. The averaged time constants from WT (filled symbols, n = 10) and I1495F (open symbols, n = 7) are shown.

I1495F enhances slow inactivation

It has been proposed that a disruption of slow inactivation is also necessary to account for the extended duration of paralysisseen in patients with HyperKPP (Ruff, 1994). Subsequently, itwas demonstrated that the rT698M mutation does indeed impair slowinactivation of the rat SkM1 sodium channel (Cummins and Sigworth,1996). Slow inactivation is functionally distinct from fast inactivation.The time constant for entering and leaving the slow inactivatedstate is on the order of tens of seconds rather than millisecondsas for fast inactivation (Ruff et al., 1988). Results from I1495Fslow inactivation experiments are shown in Figure 6. Our datashow that steady-state slow inactivation (s) is not impairedfor I1495F channels as reported for the rat T698M mutation (Cumminsand Sigworth, 1996), but in contrast, is enhanced with the I1495Fmutant (WT, V_0.5 = $-$ 61.6 ± 2.8 mV; z = 2.7 ± 0.2; n = 8; I1495F,V_0.5 = $-$ 76.7 ± 2.6 mV; z = 1.8 ± 0.1; n = 8) (Fig. 6A). Both midpointand apparent gating charge are significantly different (p < 0.002).However, development of slow inactivation at $-$ 20 mV (Fig. 6B)and recovery from slow inactivation at $-$ 100 mV (Fig. 6C) do notseem to be significantly altered by the I1495F mutation.

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Figure 6. I1495F enhances slow inactivation. A, Steady-state slow inactivation in hSkM1 WT (filled circles, n = 8) and I1495F (open circles, n = 8) after 50 sec conditioning pulse ranging from $-$ 130 to 10 mV. B and C show development of slow inactivation and recovery from slow inactivation, respectively, as a function of time for WT (filled circles, n = 7) and I1495F (open circles, n = 7) channels. Protocols are as described in Materials and Methods.

The T704M mutation

The T704M is the most common HyperKPP mutation and is located at the intracellular interface on the S5 segment of domain II.Although the corresponding mutation has been extensively studiedin the rat clone (rT698M; Cannon and Strittmatter, 1993; Cumminset al., 1993; Cummins and Sigworth, 1996; Hayward et al., 1997),the T704M mutation in the human clone has not been fully characterized(Yang et al., 1994). For example, it is not known whether theT704M mutation alters deactivation or slow inactivation of humanskeletal muscle sodium channels. Hence, we were interested inthe comparison of the T704M and I1495F mutations in the humanbackground and in the same expressionsystem.

Fast inactivating sodium currents are observed in cells expressing either the WT (Fig. 7A) or the T704M channels (Fig. 7B).The voltage dependence of activation and conductance was significantlydifferent (p < 0.005) between WT (V_0.5 = $-$ 19.0 ± 1.7 mV; n = 28)and T704M (V_0.5 = $-$ 26.9 ± 1.8 mV; n = 26) in HEK 293 cells (Fig.7C,D). The apparent gating charge was also significantly different(p < 0.005) between WT (z = 3.7 ± 0.1; n = 15) and T704M (z =3.0 ± 0.2; n = 13) channels. The shift in activation is similarto what has been reported previously for T704M channels (Yanget al., 1994) and for rT698M channels (Cummins et al., 1993),and to the shift in activation caused by the I1495F mutation.It has been proposed that the HyperKPP mutations increase theprobability that the channels gate in a noninactivating mode,increasing the size of the sustained current throughout the activationrange (Cannon and Strittmatter, 1993). To examine this, we measuredthe sustained current at the end of 40 msec depolarizations. At0 mV, where window currents are not expected to contribute tothe sustained current, we did not find any difference betweenthe size of the sustained currents in WT (0.4 ± 0.8% of peak;n = 8) and T704M (0.3 ± 0.7% of peak; n = 10) cells. In contrast,at $-$ 50 mV, where window currents can contribute to the persistentcurrent, the sustained currents were larger in T704M cells (0.5± 0.2% of peak; n = 10) than in WT cells (0.1 ± 0.2% of peak;n = 8). We found no difference (p = 0.3) between steady-statefast inactivation of WT ( $-$ 70.5 ± 1.2; z = 4.0 ± 0.1; n = 31) andT704M ( $-$ 73.6 ± 1.1; z = 3.6 ± 0.1; n = 29) channels (Fig. 7D).We were careful to measure steady-state fast inactivation at thesame time point in the recording for both WT and T704M channels.We have shown previously that there is no difference between ratWT and rat T698M channels in terms of the voltage dependence ofsteady-state fast inactivation (Cummins et al., 1993; Cumminsand Sigworth, 1996).

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Figure 7. Effect of the T704M mutation on hSk6M1 currents. Family of traces from representative HEK 293 cells expressing either WT (A) or T704M (B) channels. The currents were elicited by 40 msec test pulses to various potentials from $-$ 60 to 30 mV. Cells were held at $-$ 100 mV. C, Peak current-voltage relationship for WT (filled squares, n = 8) and T704M (open squares, n = 7). D, The steady-state fast inactivation curves for WT (filled circles, n = 12) and T704M (open circles, n = 10) channels with 500 msec inactivating prepulses are shown. Cells were held at prepulse potentials over the range of $-$ 130 to 10 mV before a test pulse to $-$ 10 mV for 20 msec. Current is plotted as a fraction of peak current. Currents were converted to conductance, from the current-voltage curve shown in Figure 7C, for WT (filled squares, n = 8) and T704M (open squares, n = 7), and fit was made according to the Boltzmann function.

We also compared tail current kinetics of WT and T704M under the same conditions as those used for the I1495F. We found thatthe time constant of deactivation was slower in the T704M thanin the WT channels (Fig. 8A,B), in contrast to the I1495F mutantin which deactivation was not affected. This suggests that theT704M mutation alters the transition between the closed and openstates. Our data on the recovery from fast inactivation show thatthe T704M recovers from fast inactivation in a manner similarto the I1495F mutant. However, development of fast closed-stateinactivation seems to be unaffected by the T704M mutation (Fig.8C), whereas the I1495F exhibits a faster development of closed-stateinactivation.

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Figure 8. Deactivation, development, and recovery from fast inactivation for the T704M. The protocols used for the T704M are the same as those described for the I1495F mutation in Figure 5. A, Tail current traces obtained from WT and T704M channels at $-$ 70 mV. B, Time constants of tail current as shown in A were plotted as a function of the test potential for WT (filled circles, n = 5) and T704M (open circles, n = 6). C, Development of fast inactivation (squares) and recovery from fast inactivation (circles) for WT (filled symbols, n = 8) and T704M (open symbols, n = 7) were obtained as described in Figure 5.

Because the rat T698M and the I1495F mutations have altered slow inactivation and because the T704M is located at the intracellularinterface of the S5 segment of domain II, we tested whether slowinactivation of human skeletal muscle sodium channels was affectedby the T704M mutation. Results from slow inactivation experimentsare shown in Figure 9. Although most of the WT current is slowinactivated after 5 min at 0 mV (Fig. 9A), >50% of the T704M currentremains available for activation under the same conditions (Fig.9B). We measured the voltage dependence of slow inactivation using50 sec sequential depolarizations (Fig. 9C). We observed a significantimpairment of slow inactivation for T704M channels compared withWT channels. For WT channels, slow inactivation is nearly completeat 0 mV, with 6 ± 3% (n = 8) of the current available for activationafter the 30 msec recovery pulse. In contrast, at 0 mV, 50 ± 10%(n = 7) of the T704M current is available for activation afterthe 30 msec recovery pulse.

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Figure 9. Slow inactivation is impaired in T704M cells. Changes in peak sodium current for representative WT (A) and T704M (B) cells in response to changes in the holding potential. Cells were allowed to stabilize for 20 min at $-$ 80 mV before beginning the test protocol. The protocol involved holding the cell at a specific potential for 5 min, while once every 15 sec the membrane potential was stepped to $-$ 100 mV for 30 msec and then to 0 mV for 20 msec. The peak current elicited by the test pulse to 0 mV is plotted. C, The steady-state slow inactivation curves for WT (filled circles, n = 8) and T704M (open circles, n = 7) cells are shown. D, Normalized Na current in representative WT (filled circles, n = 5) and T704M (open circles, n = 6) cells recovering from slow inactivation. The time axis is logarithmic. The recovery protocol required ~45 min to complete and had two phases: short recovery times were obtained with individual recovery pulses, long recovery times were obtained in a continuous recording. E, Development of slow inactivation is shown to be slower for the T704M (open circles, n = 5) than for the WT channels (filled circles, n = 5). Cells were held at $-$ 100 mV for an increasing conditioning time. Details of the protocol are described in Materials and Methods.

We also measured the time course for recovery from slow inactivation. The fraction of current was measured for recovery timesranging from 1 msec to >400 sec, as has been described previously(Cummins and Sigworth, 1996). The T704M channels recovered fromslow inactivation much faster than did the WT channels (Fig. 9D).With a recovery time of 100 msec, only 11 ± 4% (n = 5) of theWT current recovers, whereas 66 ± 9% (n = 5) of T704M currentrecovers. The initial rate of recovery for the T704M channelsis similar to that for the recovery from fast inactivation. Figure9E shows the time course for the development of slow inactivationfor WT and T704M channels. At $-$ 20 mV, the time constant was significantly(p < 0.05) smaller for WT channels (3.9 ± 0.7 sec; n = 5) thanfor T704M channels (12.0 ± 2.9 sec; n = 5). These data show thatthe T704M mutation disrupts slow inactivation in human SkM1 channelsin an identical manner to the effect of the rT698M mutation onrat SkM1 channels but distinct from the I1495F mutation in whichslow inactivation was particularlyenhanced.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Over 20 point mutations in the SCN4A gene causing either HyperKPP, PC, or PAM have been described. The mutations are dispersedthroughout the channel. However, three locations may be consideredas "hot spots" according to the number of patients carrying mutations:the interdomain III-IV, cytoplasmic membrane interface, and segmentS4 in domain IV. Few patients were reported with mutations inthe transmembrane segments. No disease-causing mutation in segmentsS2 or S5 has been reported todate.

In the present study, we report a new family with the HyperKPP phenotype, which was unusual in that it was associated withmuscle cramp and no myotonia was seen clinically or electrophysiologically.Scanning the sodium channel gene in the patient's DNA with SSCPanalysis and sequencing revealed a T-to-C transition at position4561 of the SCN4A gene (in exon 24), resulting in the amino acidchange isoleucine 1495 to phenylalanine located in the S5 segmentof domain IV of the sodium channel $alpha$ -subunit. This is the firstdisease-causing mutation located in this transmembrane segment.Expression of the I1495F mutation in HEK 293 cells revealed alterationsin channel function that could account for the onset of HyperKPPin our patient. Comparing I1495F and T704M mutations revealeda prominent role of the S5 segment in channel activation, as wellas in fast and slowinactivation.

Macroscopic inward sodium current from cells expressing I1495F showed that this substitution results in a sustained currentat a wide range of physiological voltages. A two-exponential functionwas needed to fit the decay phase of the mutant macroscopic current,whereas a single exponential was sufficient for WT current decayfitting. The slowly decaying component measured in I1495F suggeststhat the S5 segment of domain IV is involved in channel inactivation.This behavior is surprising because I1495F is embedded in themembrane, presumably far from the intracellular membrane interfaceand also far from the III-IV linker, a strong candidate for thefast inactivation gate of the sodium channel (Stühmer et al.,1989; West et al., 1992). This mutation may have indirectly disrupteda structure directly involved in channel inactivation. Indeed,Mitrovic et al. (1996) and McPhee et al. (1998) reported recentlyan involvement of the cytoplasmic linker IV/S4-S5 in channel fastinactivation. In another study, a similar conclusion was reachedby scanning the linker IV/S4-S5 of the hSkM1 by cysteine mutagenesis(Lerche et al., 1997).

We did not observe large sustained currents in T704M channels at 0 mV but only at more negative voltages at which window currentsmight occur. Although initially we do observe larger sustainedcurrents in I1495F channels, these currents appear to run down,and after 10 min in the whole-cell configuration, we do not findany difference in the size of WT and I1495F sustained currents.This may indicate that sustained currents in skeletal muscle sodiumchannels can be modulated, and some of the disease-causing mutationscould possibly affect this modulation. Recently, it has been shownthat G-proteins modulate sustained currents in brain sodium channels(Ma et al., 1997).

Inactivation, especially at negative potentials, is significantly enhanced in the I1495F construct but not affected in T704M;this is indicated by a 10 mV hyperpolarizing shift in the steady-statefast inactivation of I1495F compared with WT and the faster developmentof inactivation at negative voltages ( $-$ 80 to $-$ 60 mV, Fig. 5C).This is the first HyperKPP mutation causing a negative shift inthe voltage dependence of channel availability and conductance.However, the M1360V mutation responsible for HyperKPP and PC (Wagneret al., 1997) causes a $-$ 13 mV shift in channel availability only.The activation curve was not changed by the M1360V mutation, incontrast to the I1495F and T704M mutations that shifted the voltagedependence of activation toward negative potentials. Cummins etal. (1993) found a similar result for the rat T698M mutation (equivalentto the human T704M causing HyperKPP). A $-$ 12 mV shift in the voltagedependence of activation was reported to underlie the increasein the sustained sodium flow, mainly by increasing the windowcurrent between $-$ 75 and $-$ 40 mV, a voltage range in which sustainedcurrent is observed in HyperKPP musclefibers.

The similarity observed here between the I1495F and T704M mutations in the activation curve may suggest a role of the S5 segments(at least in domain II and IV) in channel activation. However,although myotonia is prominent in patients with the T704M mutation,the patient with the I1495F mutation did not exhibit myotonia.This suggests that enhancement of activation is not sufficientto cause myotonia. Interestingly, another mutation in the S4-S5linker of domain II, I693T, also shifts activation in the negativedirection and induces weakness but apparently not myotonia (Plassart-Schiesset al., 1998).

Defective deactivation may well account for sodium channel disease, as reported in our own study on the R1448S mutation (Bendahhou,Cummins, Kwiecinski, Waxman, and Ptácek, unpublished observations)and studies from other laboratories (Richmond et al., 1997; Featherstoneet al., 1998). These studies together have shown that a defectin sodium channel deactivation, along with altered inactivation,may lead to a destabilization of membrane repolarization resultingin prolonged action potentials. Whereas the T704M mutation significantly(p < 0.001) slowed deactivation, the I1495F mutation had muchless of an effect compared with WT. We investigated also the rateof recovery from fast inactivation in WT, I1495F, and T704M. Whereasthe I1495F has a slower recovery rate than WT (most prominentat $-$ 80 mV), the T704M mutation did not significantly alter therate of recovery from fastinactivation.

It has been proposed that both fast and slow inactivation must be disrupted to trigger sustained currents in HyperKPP patients(Ruff, 1994). We found that slow inactivation was differentiallydisrupted in the I1495F and T704M mutants. Slow inactivation appearsto be incomplete in T704M channels; after prolonged depolarizationslasting 20 min or more, more than one-third of T704M channelsfail to become slow inactivated and are available for activationafter a brief (e.g., 30 msec) hyperpolarization. This disruptionof slow inactivation, in combination with enhanced window currents,are expected to result in sustained currents, such as those observedin the muscle of patients with HyperKPP. In the I1495F channels,in contrast, slow inactivation is dramatically enhanced; thisis shown by the left shift in the steady-state slow inactivation.This is the first disease-causing mutation shown to enhance sodiumchannel slow inactivation. However, Wang and Wang (1997) haveshown in site-directed mutagenesis that a mutation in S6 segmentof domain I can cause enhancement in slow inactivation of therat muscle homolog. An enhancement of slow inactivation couldcontribute to weakness in thispatient.

Because the patient with the I1495F mutation did not exhibit myotonia, our data on slow inactivation suggests that disruptionof slow inactivation could be crucial to the development of myotoniain HyperKPP patients. However, slow inactivation does not appearto be impaired by PC mutations associated with myotonia (Haywardet al., 1997; Richmond et al., 1997).

The HyperKPP mutation described here is the first substitution occurring in the putative membrane spanning segment IV-S5.This segment has not previously been shown to be involved in eitherthe activation or inactivation process of the sodium channel.Mutations in the S5 segments and in the S4-S5 linker have alreadybeen shown to alter gating of voltage-sensitive potassium channels(Zagotta and Aldrich, 1990; McCormack et al., 1991; Kirsch etal., 1993; Holmgren et al., 1996; Shieh et al., 1997). An involvementof the S5 segments of the sodium channels in both activation andinactivation may well explain the mutant channel behavior inHyperKPP.

Recent studies have focused on the role of the S4-S5 and S3-S4 linkers of domain IV in sodium channel inactivation. This wasshown by either studying disease-causing mutations, scanning mutagenesis(McPhee et al., 1998), cysteine scanning mutagenesis (Lerche etal., 1997), or by peptide insertion (Dib-Hajj et al., 1997). Onone hand, the S3-S4 linker of domain IV may affect the couplingbetween activation and inactivation by altering the movement ofS4 segment in the membrane (Chahine et al., 1994; Dib-Hajj etal., 1997). The S4-S5 linker, on the other hand, is a good candidatefor interacting with the Ile-Phe-Met motif of the inactivationgate (Lerche et al., 1997; McPhee et al., 1998). These studiesconcluded that the loop S4-S5 plays a prominent role in sodiumchannel fast inactivation but gave no indication of the role ofthe S5 segment in the inactivation process. We hypothesize, basedon our data and those reported for the role of the loop S4-S5and the S4 segment in channel inactivation, that the membranespanning segment S5 of domain IV interacts closely with the activationmechanism.

It has been proposed that paralysis can still occur in HyperKPP without impaired slow inactivation (Cannon, 1994). However,it was predicted that, without disruption of slow inactivation,there would be an asynchronous cycling of the muscle fibers betweenexcitable and inexcitable states during the episodes of paralysis.In contrast to most patients with HyperKPP who typically havepainless episodes of paralysis, the patient with the I1495F mutationexperienced crampy pain during the attacks of weakness. Therefore,we propose that intermittent activation of affected muscle fibersduring attacks of weakness might contribute to the crampy painassociated with the I1495F mutation. Because the I1495F mutationenhances slow inactivation, our results demonstrate that the manifestationof HyperKPP does not necessarily require disruption of slowinactivation.

  FOOTNOTES

Received Jan. 20, 1999; revised April 1, 1999; accepted April 1, 1999.

This work was supported by a Muscular Dystrophy Association grant and by the Paralyzed Veterans of America and Eastern ParalyzedVeterans Association. We are grateful to Dr. F. Sigworth for supportingsome of the work on the T704M mutation. We also thank the DNASequencing Facility at the University of Utah, supported in partby National Cancer Institute Grant #5P30CA42014. We thank Drs.M. Sanguinetti, J. Richmond, and D. Featherstone for criticalreading of thismanuscript.
Drs. Bendahhou and Cummins have contributed equally to thiswork.

Correspondence should be addressed to Louis J. Ptácek, Howard Hughes Medical Institute, Eccles Institute of Human Genetics,University of Utah, Building 533, Room 4425, Salt Lake City, UT84112.

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