Clinical assessment, neurological and genetic testing

The patient was referred to the Section of Clinical Neurophysiology, Oslo University Hospital for neurophysiological evaluation of distal pain in her extremities. The patient underwent neurological and neurophysiological examinations, including QST (thermal thresholds), EMG/neurography and microneurography. The diagnosis of EM was based on the presence of episodic pain, warm and red feet and pain alleviated by cold, the absence of indicators of small fiber neuropathy in thermotesting and the absence of other causes for small fiber neuropathy like diabetes mellitus, polycythemia vera or medication (see Results for details, and [6]). A thorough medical history was inquired with focus on previous and family history of pain and details about actual pain symptoms, including start and evolution of pain, characteristics and intensity on a numeric scale from 0 to 10, occurrence of spontaneous episodic and evoked pain, eliciting and alleviating factors. The clinical and neurological examination consisted of an inspection of the extremities and of an evaluation of sensory function (light touch with cotton swab and a von Frey hair testing, pain sensation with a needle and vibration with a Rydel Seiffer tuning fork), and motor function (muscle strength and assessment of tendon reflexes from the upper and lower extremities).

Genetic testing was performed as previously described [8] and showed a heterozygous single-point mutation in SCN10A which was not found in 96 controls (it is also listed as very rare in the ExAC browser: http://exac.broadinstitute.org/variant/3-38783939-A-T). The study was approved by the regional ethical committee REK (Regional Committees for Medical and Health and Health ethics) South East, record-number S-07204a. The individual in this manuscript has given written informed consent (as outlined in PLOS consent form) to publish these case details.

Quantitative sensory testing

Threshold temperatures for the sensation of warmth, cold, heat pain and cold pain were determined using a computerized Thermotest (SENSElab, Somedic A/B, Hörby, Sweden) with a thermode size of 5 x 2.5 cm. Warmth detection threshold (WD), cold detection threshold (CD), heat pain detection threshold (HP) and cold pain detection threshold (CP) were determined from a baseline temperature of 32°C with a 1°C/s rate of change. The patient was instructed to push a signal-button when the relevant sensation was perceived. When this happened or if cut-off temperature (50 C and 10 C) was obtained, the temperature returned to baseline. WD, CD, HP, CP were determined from the thenar eminence, the dorsum of both feet and both legs at knee-level. For calculations of thresholds, an average of five recordings for WD and CD and the average of three recordings for HP and CP were used. The values were compared with normal values from the neurophysiological department of Rikshospitalet University Oslo.

EMG/neurography

A Keypoint EMG apparatus (Denmark) was employed, measuring motor amplitude, distal latency and conduction velocity of the median, ulnar, peroneal and posterior tibial nerves, and sensory amplitude and conduction velocity of the median, ulnar and sural nerves. EMG of proximal and distal muscles form the right leg was performed, assessing the properties of the motor unit potential as searching for possible signs of denervation. The values were compared to normal Keypoint data.

Microneurography recording technique

APs from single C-fibers were recorded by microneurography from the peroneal nerve at the level of the fibular head. Recordings from five EM patients without Nav mutations were used as controls and the data were compared to microneurography data from healthy controls which were published before (Namer et al 2009). The principle of microneurography has been described in detail previously [29] and is shown in Fig 1. Briefly, a tungsten electrode (Frederick Haer, Bowdoinham, ME, USA) was inserted into a fascicle of the peroneal nerve containing cutaneous C-fibers close to the knee. Individual C-fibers were identified by applying electrical pulses transdermally in the innervation area of the nerve on the foot dorsum, evoking APs with low conduction velocities (<2 m/s, Fig 1A). Two stimulation needles (0.15 mm diameter) were then inserted in the skin receptive field of the C-fibers of interest. The C-fibers were stimulated repetitively (0.25 Hz, 0.5 ms, 1–30 mA) via a constant current stimulator (DS7A; Digitimer, Hertfordshire, England, UK) through the stimulation needles and the resulting APs were recorded, amplified, processed online, and stored to a computer using custom-written Spike2 software and a micro1401 DAC (CED, Cambridge, UK, Fig 1B). The data were analyzed off-line by Drever software (Uppsala, Sweden).

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Fig 1.

A: Microneurography setup. Action potentials are evoked electrically in the receptive field of the pierced fascicle, travel proximally along the peroneal nerve and are recorded at the fibular head. B: The interval between the first electrical stimulus and the arrival time of the evoked AP at the recording needle t₀ is set as reference conduction latency. Conduction latencies of subsequent pulses (Δt) are calculated relative to the first latency (Δt/t₀). C: Plot of the relative conduction latency (Δt/t₀) versus pulse number. The increase in Δt/t₀ indicates the slowing of the AP conduction upon repetitive stimulation.

https://doi.org/10.1371/journal.pone.0161789.g001

Response to natural stimulation and spontaneous activity

When a C-fiber was activated repetitively at low frequencies through stimulation needles in the receptive field of the recorded fibers, APs with stable conduction latencies were recorded. However, additional activity in this C-fiber, e.g. due to mechanical stimulation, induced a sudden increase in conduction latency, a phenomenon known as marking [29]. Such increase in latency is due to an activity-dependent slowing of conduction velocity (ADS) in C-fibers [30] and shown in Fig 1B and 1C. Marking was used to assess the responses in single C-fibers to natural (mechanical, heat) and electrical stimulation. Spontaneous activity of a fiber was judged by an abrupt increase of response latency followed by a gradual normalization (marking) without external stimulation or evidence of a unidirectional block.

Electrical stimulation protocols

After a 2 min pause in the electrical stimulation, activity dependent changes in conduction velocity were induced either by applying a low-frequency stimulation protocol (20 pulses at 0.125 Hz, 20 pulses at 0.25 Hz, and 30 pulses at 0.5 Hz) through the stimulation needles in the skin or a high-frequency protocol consisting of a train of 360 electrical pulses at 2 Hz. ADS was measured at the 3^rd, 10^th, 120^th and 360^th (last) pulse of the high frequency protocol. Total ADS was calculated as the relative increase in latency from the first pulse to the last in both protocols. By switching to the lower stimulation frequency of 0.25 Hz the total ADS gradually returns to baseline (“recovery phase”). During this phase we measured the response latency for the 10^th pulse at 0.25 Hz and normalized it to the total ADS (rate of recovery). The value was excluded if spontaneous activity interfered with ADS or rate of recovery.

Natural stimulation protocols

Fibers were tested for mechanical response by stimulating with a 75 g von Frey filament in the receptive fields. Fibers which responded to this stimulation by marking were classified as mechano-positive.

Heat response was assessed by using a feedback controlled bulb delivering a heat ramp to the skin, starting at 32°C with an increase of 0.25°C/sec up to a maximum of 50°C. Fibers responding by marking were classified as heat positive. Heat threshold was determined if possible.

Classification of C-fibers

The classification of single C-fibers was based on ADS and the response to natural stimulation. C-nociceptors were classified as CM-nociceptors if they were mechano-positive (von Frey 75 g) and had less than 3% total ADS in the low-frequency protocol, or as CMi-nociceptors if they were mechano-insensitive (von Frey 75 g) and had more than 5% total ADS in the low frequency protocol. The remaining C-nociceptors were classified as C-nociceptors of unknown type (not possible to classify as normal CM or CMi).

C-fibers were defined as sympathetic C-fibers if they had characteristic reversal of the initial ADS [31] in the high-frequency protocol and/or were activated by sympathetic stimulation.

Cell culture and transfection

Wistar rat pups (3–6 days of both sexes, bred at FAU Erlangen-Nuremberg, Germany) were anaesthetized with halothane (Sigma-Aldrich GmbH, Steinheim, Germany) and decapitated in accordance with ethical guidelines established by German animal protection law, approved by the animal protection committee of Regierung Mittelfranken, Germany, DIVA-number 095621001683, registered according to regulation (EG) number 1069/2009, DE09562000821. After decapitation, the backbone was removed rapidly and bisected longitudinally in ice-cold PBS. DRGs were removed, desheathed, cleaned and enzymatically dissociated in Dulbecco’s modified Eagle's Medium (DMEM, Gibco-Life technologies, New York, USA) supplemented with collagenase/protease for 45 min at 37°C. Cells were mechanically triturated with small diameter Pasteur pipettes in TNB medium (Biochrom AG, Berlin, Germany) and transfected using the nucleofector II (Lonza group Limited, Basel, Switzerland) according to the manufacturers protocol. Poly-D-Lysine (Sigma-Aldrich GmbH, Munich, Germany) coated cover slips were loaded with the cell suspension and after cells settled for 5–10 min TNB medium was added. DRGs were incubated at 37°C and 5% CO₂ for one day before experiments were performed.

ND7/23 neuroblastoma cells (kindly provided by Stephen G. Waxman) were maintained in DMEM medium (Gibco-Life technologies) containing 4.5 g/l Glucose, 10% fetal bovine serum (Biochrom AG) and 1% Penicillin/Streptomycin (PAA Laboratories GmbH). One day before transfection ND7/23 cells were plated on 3.5 cm dishes and transfected with Nanofectin (PAA Laboratories GmbH) according to the manufacturers protocol using 1 μg hNav1.8 in pIRESpuro3 vector and 0.5 μg EGFP-C1 (Clontech Laboratories, Inc., Mountain View, USA). Cells were recorded 20 to 30 h after transfection.

Whole-cell patch-clamp recordings

Whole-cell voltage and current clamp recordings were performed using glass electrodes with tip resistances of 1.5 to 2.2 MΩ, manufactured with a DMZ puller (Zeitz Instruments GmbH, Martinsried, Germany) and filled with an internal solution comprising for current-clamp recordings on DRGs (in mM): 135 K-Gluconate, 4 NaCl, 10 KCl, 10 HEPES, 2 Na₂ATP, 0.4 Na₃GTP (adjusted to pH 7.3 with KOH), and for voltage-clamp experiments on ND7/23 cells (in mM): 140 CsF, 10 NaCl, 10 HEPES, and 1 EGTA (adjusted to pH 7.38 with CsOH). Activation properties of Nav1.8 expressed in ND7/23 cells were determined using a pipette solution with low NaCl to shift the reversal potential to more depolarized voltages (in mM): 140 CsF, 2 NaCl, 10 HEPES, 10 TEA-Cl and 1 EGTA (adjusted to pH 7.38 with CsOH).

The external bathing solution contained for DRGs (in mM): 140 NaCl, 4 KCl, 1 MgCl₂, 2 CaCl₂, 10 HEPES, 5 Glucose (adjusted to pH 7.4 with NaOH), for ND7/23 cells (in mM): 140 NaCl, 1 MgCl₂, 1 CaCl₂, 10 HEPES, 10 Glucose, 10 TEA-Cl (pH 7.4, adjusted with NaOH). In experiments with ND7/23 cells, endogenous TTXs Navs were suppressed by adding 1 μM TTX (Biotrend, Wangen/Zurich, Switzerland) to the bath solution.

Only small (< 25 μm) DRGs were chosen for recordings. Size was measured as the maximal diameter of the cells on an image taken with a digital camera at the patch clamp setup. Recordings were performed at room temperature (22 ± 1°C). Current-clamp recordings were sampled at 20 kHz (low-pass filter 6 kHz) using an Multiclamp 700B amplifier in conjunction with a Digidata 1322A interface and pClamp10 software (all from Molecular Devices, Sunnyvale, USA). A HEKA EPC-10 USB operated with Patchmaster software (HEKA electronics, Lambrecht, Germany) was used for voltage-clamp signal recording, low-pass (< 10 kHz) filtering and digitizing (100 kHz).

Pipette potential was zeroed prior to seal formation and capacitive transients were compensated using C-fast for pipette-capacity correction and subsequently C-slow for cell-capacity compensation, the series resistance was compensated by at least 50%. The absolute peak current (pA) was divided by the capacitance as determined by C-slow compensation to obtain current densities. For voltage-clamp recordings, leak pulses were applied following the test pulse, and mean leak current was subtracted digitally online corresponding to the P/4 leak pulse procedure.

Voltage protocols were carried out after current stabilization. Standard current-voltage (I-V) curves were recorded using 100-ms pulses from a holding potential of −120 mV to a range of potentials (-100 to +80 mV) in 10 mV steps. Conductance-voltage curves were obtained by calculating the conductance (G) at each voltage (V) using the equation G = I/(V − V_rev), with V_rev being the reversal potential, determined for each cell individually. Conductance-voltage curves were fitted with a Boltzmann equation: G_Na = G_Na,max/(1 + exp [(V_m − V_half)/k]), where G_Na is the voltage-dependent sodium conductance, G_Na,max is the maximal sodium conductance, V_half is the potential at which activation is half-maximal, V_m is the membrane potential, and k is the slope factor. Steady-state fast inactivation was determined by applying a 500 ms pulse with various potentials (ranging from -130 mV to +10 mV in 10 mV steps) and determining the remaining available current using a depolarizing pulse to 0 mV. Currents were normalized to the maximum inward current. Inactivation decay time constants were determined by single-exponential fits to the current decay of the current obtained with the activation protocol. We provide all single, processed recordings shown in the data figures in S1 and S2 Files.

Statistics

An unpaired two-sample Student’s t-test was used to test for statistical significance for the patch-clamp data. Data are presented as mean ± standard error of the mean (SEM) unless otherwise specified.

Microneurography data were processed using Statistica version 26. Due to the exploratory design and the small size and distribution of the data obtained from microneurography, descriptive data (median and 25th and 75th percentiles) are presented and significance testing was performed using the non-parametric Mann-Whitney-U-test.

A patient carrying the Nav1.8 M650K mutation shows clinical signs of erythromelalgia

We describe here a 53 year old woman with symptoms beginning at the age of 35 for whom genetic testing revealed the heterozygous amino acid substitution M650K, Methionine (M) to Lysine (K), in her SCN10A gene encoding for Nav1.8 [8]. No additional mutation was identified in her other sodium channel or candidate genes. Her father and sister report burning feet, but were not diagnosed with EM, nor genetically tested. The patient has previously suffered from migraine-like attacks and has had neck problems. Her present symptoms are described as episodes of painful warm feet several times a week, predominantly in the evenings and early night. The feet are red and feel warm, but the skin temperature appears normal upon clinical examination. Her symptoms are worse after physical activity and after exposure to heat (e.g. warm floors). Her pain is superficial and of a burning and pressing character, only located in the feet, predominantly the soles. Pain intensity was rated up to 5 on a numeric rating scale from 0 to 10 where 0 is no pain and 10 maximal pain. The patient does not receive medication but her pain is relieved by cooling. Therefore she often walks barefooted or submerges the feet and legs in cold water. She had normal findings by EMG/neurography and QST (thermal thresholds) (see Tables 1 and 2) and also no abnormalities in her clinical and neurological findings, except for a reduced sensibility for light touch (von Frey test) on the feet from the toes to just above the ankle. As we observed normal nerve conduction results for the sural nerves we excluded a large fiber sensory neuropathy.

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Table 1. Results of QST (thermal thresholds) of the IEM patient carrying the Nav1.8/M650K mutation.

https://doi.org/10.1371/journal.pone.0161789.t001

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Table 2. Sensory nerve conduction properties of the sural nerve of the IEM patient carrying the Nav1.8/M650K mutation.

https://doi.org/10.1371/journal.pone.0161789.t002

Patient’s nociceptors show low rate of spontaneous activity

We examined a total of 25 C-fibers of this patient by microneurography, including 20 C-nociceptors (ten CM-nociceptors, eight CMi-nociceptors, two C-nociceptors of unknown type, Table 3), two sympathetic C-fibers and three fibers that could not be identified. In order to assess the specific impact of the Nav1.8 M650K mutation, we chose to compare our findings in this patient with previously published EM patients without identified Nav mutations (23 CM-nociceptors, eight CMi-nociceptors, 14 C-nociceptors of unknown type and 11 sympathetic C-fibers). For direct comparison with a healthy control group we included data of previously published healthy age matched controls [32].

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Table 3. Basic sensory and axonal properties of CM and CMi-fibers.

https://doi.org/10.1371/journal.pone.0161789.t003

Two nociceptors with biophysical properties typical for CMi-nociceptors, showed a response to mechanical stimuli. These nociceptors were interpreted as mechanical sensitized CMi-nociceptors. In contrast to the mechanical sensitization in CMi-nociceptors, the mechanical responses of six of the ten CM nociceptors were reduced in comparison to mechanical responses of healthy subjects: CM-nociceptors could only be activated by the first stimulus, and the response itself was small and not of a typical bursting character.

Spontaneous activity was observed in one CM- and one CMi-nociceptor (10.0% of total C-nociceptors) of the M650K patient. Due to the indirect assessment of spontaneous activity in microneurography via the marking method it is not possible to give exact measures about the frequencies of spontaneous discharges, but from the pattern of markings spontaneous activity appeared to be of lower frequency when compared to markings obtained during mechanically or heat induced bursting. In recordings from the EM control group, 42.2% of the C-nociceptors fired spontaneously (5 CM, 4 CMi, 10 C-nociceptors of unknown type). Thus, the patient carrying the M650K mutation displayed fewer spontaneously active fibers compared to EM patients without Nav mutation.

Patient’s CMi nociceptors display enhanced ADS

Conduction velocity and ADS at the low-frequency protocol in CM- and CMi-nociceptors were comparable to EM-controls (see Table 3). Conduction velocity and ADS of the two sympathetic C-fibers of the M650K patient were normal (Table 2) and in the range of the sympathetic fibers of the EM-controls.

However, in contrast to what was displayed during the low frequency protocol, the CMi-nociceptors of the patient carrying the M650K mutation displayed more ADS during 2 Hz stimulation compared to the EM-controls and healthy subjects, even during the first pulses of the protocol (Table 4 and Fig 2A–2C, lower panel). Two CMi-fibers of the M650K patient showed an abnormal increase in ADS at the end of the high-frequency protocol (Fig 2A). There were no noticeable differences between the CM-fibers of the three groups (Table 4).

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Fig 2. ADS during 2 Hz stimulation protocol of CMi-nociceptors in the M650K patient (A) and EM controls without Nav mutations (B) and age-matched healthy controls (C).

The lower panel shows the first 15 pulses of the upper panel (subset indicated with gray shadow in the upper panel). Note the prominent abnormal progressive increase in ADS in the last part of the stimulation in two of the CMi-nociceptors from the M650K patient (red), none in EM patients without mutation and only one less pronounced in age-matched healthy controls showed this behavior.

https://doi.org/10.1371/journal.pone.0161789.g002

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Table 4. ADS and recovery of the C-nociceptors during high-frequency protocol.

https://doi.org/10.1371/journal.pone.0161789.t004

Thus, ADS in the patient with the M650K mutation is enhanced compared to controls and to patients with EM without Nav mutation already during the first pulses of the 2 Hz stimulation and leads to an abnormal progressive increase in ADS towards the end of the 2 Hz stimulation in two CMi-nociceptors.

Nav1.8 M650K mutation reduces sensory neuron firing rate

The mutation M650K which was found in our patient is located at the intracellular side of DIIS1 in the linker between DI and DII of Nav1.8 (Fig 3A). In order to assess the impact of the mutation on cellular excitability, we transiently transfected dissociated rat pup DRGs with Nav1.8 or its M650K mutation. Surprisingly, neurons transfected with the M650K mutation produced significantly fewer APs compared to WT when stimulated with a 500 ms square current pulse (Fig 3B). Single step evoked APs revealed that transfection of the M650K mutation broadened the AP half width at 0 mV from 4.9 ± 0.4 ms to 7.0 ± 0.9 ms (Fig 3C and 3D, p<0.05 in a two sided t-test). Resting membrane potential remained unaffected (-41.0 ± 0.8 mV for WT versus -43.2 ± 1.6 mV for the M650K mutation, not significantly different). Thus, the Nav1.8 M650K mutation broadens APs and decreases the neuronal firing rate when transfected into DRG neurons.

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Fig 3. The M650K mutation decreases the firing rate of DRG neurons.

A: Schematic overview of a eukaryotic Nav showing the four domains DI to DIV, each consisting of the transmembrane segments S1 to S6. The rare genetic variant M650K in Nav1.8 (red dot, [8]) is located at the adjacent intracellular side of DII/S1. B: Number of APs evoked by 500 ms square step current injections to WT (black markers) or M650K (red markers) transfected cells (n = 18 and 19). * < 0.05 in a 2-sided t-test C: Example of an AP recorded from a WT (black trace) and a M650K (red trace) transfected DRG neuron evoked by a 5 ms depolarizing pulse. Injected current was twice threshold current. D: The AP half width was significantly broader in M650K than in WT transfected neurons (n = 13 and 19). *< 0.05 in a 2-sided t-test.

https://doi.org/10.1371/journal.pone.0161789.g003

Nav1.8 M650K shifts voltage dependence of steady-state fast inactivation to more hyperpolarized potentials

To assess Nav characteristics that may lead to the observed broadened AP, we transiently transfected Nav1.8 and its M650K mutation into ND7/23 cells. By adding 1 μM TTX to the bath solution we blocked all endogenous Nav currents and thus recorded Nav1.8 in isolation using voltage-clamp (Fig 4). Expression of Nav1.8 was not affected by the mutation (current density at +10 mV was -162 ± 15 pA/pF for WT (n = 10) and -171 ± 11 pA/pF for M650K (n = 12), shown in S1 Fig).

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Fig 4. Voltage-dependence of activation and deactivation of Nav1.8 is unaltered by the M650K mutation.

A: Pulse protocol and representative voltage-clamp recordings of hNav1.8 WT and hNav1.8 M650K expressed heterologously in ND7/23 cells. Traces were digitally low pass filtered for display.B: Conductance-voltage relations for WT (black circles, n = 10) and the Nav1.8 M650K mutation (red circles, n = 12) are shown. Solid lines represent Boltzmann-fits to the mean data points. C: Pulse protocol for deactivation measurements and representative recordings of hNav1.8 WT and hNav1.8 M650K mutant expressed heterologously in ND7/23 cells. D: Deactivation time constants as derived from single exponential fits of current decay during repolarization for WT (black circles, n = 13) and M650K (red circles, n = 15) at various voltages.

https://doi.org/10.1371/journal.pone.0161789.g004

Nav1.8 activated and inactivated within 20 ms (Fig 4A) and introduction of the M650K mutation did not alter voltage-dependence of activation (Fig 4B). The voltage of half maximal activation derived from Boltzmann fits to the conduction-voltage curves revealed a V_half = -2.1 mV ± 2.68 mV (WT) and -4.7 mV ± 1.53 mV (M650K) and a slope of 11.75 mV and 11.46 mV for WT and M650K, respectively. Broader APs like those recorded in M650K transfected DRG neurons may be due to slowed deactivation kinetics. We assessed deactivation using a brief depolarization of 1 ms to +20 mV in order to fully activate all expressed channels, followed by hyperpolarizing pulses to potentials between -120 mV and 0 mV (Fig 4C). Time constants derived from a single exponential fit to the deactivating currents were not significantly different between WT and M650K mutation at all potentials tested (Fig 4D). The remaining mean persistent current measured between 80 and 100 ms during the test pulse were not affected by the mutation (S2 Fig).

In contrast, the voltage-dependence of steady-state fast inactivation was significantly shifted to more hyperpolarized potentials (Fig 5A). Mean V_half revealed by Boltzmann-fits for WT and M650K mutant were -66.0 mV ± 6.5 mV and -73.8 mV ± 2.2 mV (slope: -9.03 mV and -9.66 mV), respectively (Fig 5B). Inactivation decay kinetics, as determined by a single exponential fit to current decay using depolarizing pulses (as shown in Fig 4A) did not show any differences between WT and the M650K mutation (Fig 5C).

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Fig 5. The M650K mutation shifts steady-state fast inactivation to more hyperpolarized potentials.

A: Voltage dependence of steady-state fast inactivation as determined with the indicated pulse protocol. Black circles indicate WT (n = 7–8) and red circles the M650K mutation (n = 7–8). B: Distribution of the V_half determined by Boltzmann fits to each cell. Mean is indicated as an open square, the median is depicted as a line inside the box, the boxes indicate 50% confidence interval and whiskers indicate 95% confidence interval. C: Time constants of single exponential fits of currents evoked with the pulse protocol shown in Fig 4A did not differ between WT and M650K mutation at any investigated voltage.

https://doi.org/10.1371/journal.pone.0161789.g005

Recovery from fast inactivation as determined by an increasing inter-pulse interval at -120 mV and at -70 mV for periods between 1 ms and 512 ms did not reveal any significant changes induced by the M650K mutation (n = 13 for WT and n = 11 for M650K, S3 and S4 Figs). Similarly, slow inactivation as measured following a 30s pre-pulse revealed no shift of its voltage-dependence nor its slope (n = 6 for WT and n = 3 for M650K, S5 Fig). Thus, our electrophysiological results show a broadened AP and a shift of steady-state fast inactivation to more hyperpolarized potentials.