Persistent Sodium Currents and Repetitive Firing in Motoneurons of the Sacrocaudal Spinal Cord of Adult Rats

doi:10.1152/jn.00335.2005

Persistent Sodium Currents and Repetitive Firing in Motoneurons of the Sacrocaudal Spinal Cord of Adult Rats

P. J. Harvey, Y. Li, X. Li and D. J. Bennett

Centre for Neuroscience, University of Alberta, Edmonton, Canada

Submitted 30 March 2005; accepted in final form 2 November 2005

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

Months after sacral spinal transection in rats (chronic spinalrats), motoneurons below the injury exhibit large, low-thresholdpersistent inward currents (PICs), composed of persistent sodiumcurrents (Na PICs) and persistent calcium currents (Ca PICs).Here, we studied whether motoneurons of normal adult rats alsoexhibited Na and Ca PICs when the spinal cord was acutely transectedat the sacral level (acute spinal rats) and examined the roleof the Na PIC in firing behavior. Intracellular recordings wereobtained from motoneurons of acute and chronic spinal rats whilethe whole sacrocaudal spinal cord was maintained in vitro. Comparedwith chronic spinal rats, motoneurons of acute spinal rats weremore difficult to activate because the input resistance was22% lower and resting membrane potential was hyperpolarized4.1 mV further below firing threshold (–50.9 ±6.2 mV). In acute spinal rats, during a slow voltage ramp, aPIC was activated subthreshold to the spike (at –57.2± 5.0 mV) and reached a peak current of 1.11 ±1.21 nA. This PIC was less than one-half the size of that inchronic spinal rats (2.79 ± 0.94 nA) and usually wasnot large enough to produce bistable behavior (plateau potentialsand self-sustained firing not present), unlike in chronic spinalrats. The PIC was composed of two components: a TTX-sensitiveNa PIC (0.44 ± 0.36 nA) and a nimodipine-sensitive CaPIC (0.78 ± 0.82 nA). Both were smaller than in chronicspinal rats (but with similar Na/Ca ratio). The presence ofthe Na PIC was critical for normal repetitive firing, becauseno detectable Na PIC was found in the few motoneurons that couldnot fire repetitively during a slow ramp current injection andmotoneurons that had large Na PICs more readily produced repetitivefiring and had lower minimum firing rates compared with neuronswith small Na PICs. Furthermore, when the Na PIC was selectivelyblocked with riluzole, steady repetitive firing was eliminated,even though transient firing could be evoked on a rapid currentstep and the spike itself was unaffected. In summary, only smallCa and Na PICs occur in acute spinal motoneurons, but the NaPIC is essential for steady repetitive firing. We discuss howavailability of monoamines may explain the variability in NaPICs and firing in the normal and spinal animals.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

Spinal motoneurons possess voltage-gated persistent sodium andcalcium currents [persistent inward currents (PICs)] that areactivated at low thresholds just above the resting membranepotential. These PICs play a major role in amplifying synapticinputs (Deisz et al. 1991; Prather et al. 2001) and sustainingrepetitive firing (Lee and Heckman 1998a,b; Schwindt and Crill1982). PICs in motoneurons are strongly facilitated by the monoaminesserotonin (5-HT: Hounsgaard and Kiehn 1989; Perrier and Hounsgaard2003) and norepinephrine (NE: Lee and Heckman 1999), consistentwith the dense monoamine innervation of motoneurons (Alvarezet al. 1998; Schroder and Skagerberg 1985). Most, but not all,5-HT and NE in the spinal cord derives from descending brainstem tracts, and accordingly motoneurons in brain stem-intactanimals (Hounsgaard et al. 1988a) and humans (Gorassini et al.1998; Kiehn and Eken 1997) exhibit bistable behaviors consistentwith large PICs. That is, PICs are large enough to produce sustaineddepolarizations (plateaus) and firing (self-sustained firing)that, because PICs are voltage-gated, can be turned on or offby brief excitatory or inhibitory inputs (bistable behavior).Spinal transection immediately eliminates such bistable behavior,likely because of the loss of brain stem–induced releaseof monoamines onto motoneurons because bistable behavior canbe recovered by exogenous application of monoamines (Conwayet al. 1988; Hounsgaard et al. 1988a). However, PICs are notcompletely eliminated by an acute spinal transection; they areusually just reduced enough to stop bistable behavior (Bennettet al. 2001).

In motoneurons of acute spinal rats, the contributions of persistentsodium currents (Na PICs) and persistent calcium currents (CaPICs) to the total PIC have thus far not been quantified, andthus we do not know whether the loss of PICs with spinal transectionmainly results from of a loss of Ca PICs, or Na PICs, or both.We do know that with long-term spinal injury (chronic spinalrat), large PICs return (Bennett et al. 2001; Li and Bennett2003), and these include both large Na and Ca PICs of aboutequal size. Thus one of our objectives was to quantify the Naand Ca PICs in motoneurons of acute spinal rats and comparethese to the PICs found in chronic spinal rats (Li and Bennett2003) and other motoneurons of acutely isolated spinal cordslice preparations (motoneurons from different muscles. Turtle:Hounsgaard and Kiehn 1989; guinea pig: Hsiao et al. 1998; rat:Powers and Binder 2003). For this, we recorded PICs in motoneuronsin an in vitro preparation (Bennett et al. 2001), where thesacrocaudal spinal cord was acutely removed from normal adultrats (acute spinal).

Previously, the persistent sodium current (Na PIC) has beenargued to play a critical role in repetitive firing in motoneurons(Lee and Heckman 2001; Li et al. 2004a). Without a fast persistentinward current, like the Na PIC, repetitive firing is disruptedin motoneurons (Lee and Heckman 2001), as has been shown inother neurons (French et al. 1990; Urbani and Belluzzi 2000).In the course of quantifying the Na PICs in acute spinal rats,we found that, although on average the Na PIC was small, a considerablevariability existed in the Na PIC amplitude: some rats had littleor no Na PIC and others had moderately large Na PICs. Thus asecond objective of our study was to examine how variationsin the size of Na PICs affected the repetitive firing abilityof motoneurons. We found that the Na PIC was absolutely essentialfor repetitive firing, in that the few motoneurons that lackedNa PICs also had no ability to produce steady repetitive firingeven though they otherwise appeared to be healthy motoneuronswith normal fast sodium spikes.

This paper forms the basis for two companion papers (Harveyet al. 2005a,b) in which we examined how monoamine receptorsmodulate the Na PICs in the motoneurons of this study. There,we found that 5-HT application facilitated the Na PIC in acutespinal rats and, importantly, could rescue a cell that was initiallywithout firing ability, by producing a Na PIC and thereby enablingrepetitive firing (Harvey et al. 2005b). Furthermore, we showedthat 5-HT and NE receptor antagonists could completely eliminatethe Na PIC in both acute and chronic spinal rats (Harvey etal. 2005a). Thus despite the loss of brain stem–derivedmonoamines, spinal sources of monoamines (reviewed in Schmidtand Jordan 2000) must play a primary role in facilitating theNa PIC, and ultimately enable motoneurons to fire repetitively.

METHODS

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

Intracellular recordings were made from motoneurons in the invitro sacrocaudal spinal cord of both normal adult rats (femaleSprague-Dawley; 1–6 mo old, average age = 3.4 ±1.2 mo, n = 41) and spastic adult rats with chronic spinal cordinjury (3–5 mo old, average age = 4.0 ± 0.6 mo,n = 34). When the sacrocaudal cord was removed from normal ratsfor this in vitro recording, the cord was transected at theS₂ level at the time of removal; thus, these 41 rats were termedacute spinal rats. For the spastic chronic spinal rat, a completespinal cord transection was made at the S₂ sacral level whenthe adult rat was 40–55 days old (Bennett et al. 1999,2004). Usually, within 1 mo, dramatic spasticity developed inthe tail muscles, which are innervated by sacrocaudal motoneuronsbelow the level of the injury. Only rats >1.5 mo and <4mo after injury, and with clear spasticity, were used for invitro recording of the motoneurons (the 34 chronic spinal rats).Bennett et al. (1999, 2004) described the details of the chronicspinal transection and spasticity assessment. All experimentalprocedures were conducted in accordance with guidelines forthe ethical treatment of animals issued by the Canadian Councilon Animal Care, and approved by the University of Alberta HealthSciences Animal Policy and Welfare Committee.

In vitro preparation

Details of the in vitro procedures have been described in previouspublications (Bennett et al. 2001; Li and Bennett 2003; Li etal. 2004b). Briefly, normal and chronic spinal rats were anesthetizedwith urethane (0.18 g/100 g; maximum of 0.45 g per rat for rats>250 g), and the whole caudal cord between the T₁₃ and L₆vertebrae (corresponding to spinal L₆ to cauda equina) was exposedand continuously wetted with modified artificial cerebrospinalfluid (mACSF). The rat was administered pure oxygen with a maskfor 5 min before quickly removing the cord and immersing itin a dissection chamber containing mACSF. All spinal roots wereremoved except for the S₄ and Ca₁ ventral roots, and the dorsalsurface of the cord was glued (super glue; RP 1500, AdhesiveSystems) onto a small piece of nappy paper to improve stability.After a total time of 1.5 h in the dissection chamber at roomtemperature (20°C), the cord was transferred to a recordingchamber containing normal ACSF (nACSF) maintained at 24°Cand continuously flowing at >5 ml/min. The cord was securedat the bottom of the recording chamber with the ventral sideup by pinning the nappy paper to which it was glued onto theSylgard base. After allowing an hour in the recording chamberto wash out any residual anesthetic or kynurenic acid, the bathingsolution was switched to nACSF containing a cocktail of fastsynaptic transmission blockers (AP5, CNQX, strychnine and picrotoxin).The nACSF was oxygenated in an elevated 200-ml source bottleand run through the recording chamber. This nACSF running outof the recording chamber was continuously collected, filtered,and returned to the source bottle using a peristaltic pump.Because of the large volume (200 ml) being recycled in thisway and the small volume of the cord (<0.05 ml), a significantaccumulation of metabolic byproducts was not likely.

Intracellular recording

Intracellular recording methods were as described in Li andBennett (2003). Briefly, sharp intracellular electrodes weremade from thick-walled glass capillary tubes (1.5 mm OD; WarnerGC 150F-10) using a Sutter P-87 micropipette puller and filledwith a mixture of 1 M K-acetate and 1 M KCl. Electrodes (Fig. 1A)were bevelled down from an initial resistance of 40–60to 25–30 M ${Omega}$ using a rotary beveller (Sutter BV-10). Thebevel and wide electrode shaft gave good current-passing capabilities,and the sharp tip of the bevel was critical for breaking throughthe tough pia and connective tissue in these adult rats, beforepenetrating the motoneurons. A stepper-motor micromanipulator(660, Kopf) was used to advance the electrodes through the tissueand into cells. Motoneurons were identified through antidromicstimulation of the S₄ and Ca₁ ventral roots, which were wrappedaround Ag·AgCl electrodes above the recording chamberand sealed with high-vacuum grease. Only motoneurons with astable penetration, resting potential below –60 mV, andantidromic spike height >60 mV from rest were included inthis study. Data were collected with an Axoclamp 2b intracellularamplifier (Axon Instruments, Burlingame, CA) running in discontinuouscurrent clamp (DCC, switching rate 5–8 kHz, output bandwidth5.0 kHz) or discontinuous single-electrode voltage clamp (SEVC;gain 0.8 to 2.5 nA/mV) modes.

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FIG. 1. Intracellular motoneuron recording methods for rat in vitro sacrocaudal cord. A: electron microscope image of a bevelled intracellular electrode tip. Electrode was bevelled by holding the tip against a rotating stone (at 22°), while continuously monitoring its resistance with saline on the stone, until the resistance dropped to 25–30 M ${Omega}$ . Scale bar = 200 nm. B: intracellular recording in discontinuous current clamp (DCC) mode of motoneuron from a chronic spinal rat. Bottom: slow triangular current ramp (0.4 nA/s). Middle: membrane potential with repetitive firing, showing extrapolated leak potential (thin line). Note subthreshold acceleration (arrowhead), self-sustained firing (positive ${Delta}$ I = 0.8 nA; dashed lines, onset and offset of firing), and afterpotential (double arrow). Top: firing frequency (horizontal line indicates 6 Hz). Note hysteresis in firing frequency. C: instantaneous firing frequency (F) from triangular current ramp in B, plotted against current (I). F-I slope measured by regression analysis of linear region of F-I plot was 4 Hz/nA in this cell. D: same motoneuron as B, during slow triangular voltage ramp from –80 to –40 mV and back to –80 mV (3.5 nA/s; top) in single-electrode voltage clamp (SEVC) mode. At persistent inward current (PIC) onset (VSTART), current (bottom) deviated from the extrapolated leak current (thin line). PIC amplitude estimated from maximum difference between leak current and actual current, shown with downward arrow. E: same data as D, with current filtered and plotted against voltage (I-V plot). Note negative-slope region (NSR) in I-V relation.

Drugs and solutions

Two kinds of ACSF were used in these experiments: mACSF, designedto minimize potential excitotoxicity, was used in the dissectionchamber before recording, and nACSF in the recording chamber.Composition of the mACSF was (in mM) 118 NaCl, 24 NaHCO₃, 1.5CaCl₂, 3 KCl, 5 MgCl₂, 1.4 NaH₂PO₄, 1.3 MgSO₄, 25 D-glucose,and 1 kynurenic acid. nACSF was composed of (in mM) 122 NaCl,24 NaHCO₃, 2.5 CaCl₂, 3 KCl, 1 MgCl₂, and 12 D-glucose. Bothtypes of ACSF were saturated with 95% O₂-5% CO₂ and maintainedat pH 7.4. A synaptic transmission blocking cocktail was usuallyadded to the nACSF; it consisted of 50 µM D(–)-2-amino-5-phosphonopentanoicacid (AP5; Tocris), 10 µM 6-cyano-7-nitroquinoxaline-2,3-dione(CNQX; Tocris), 1 µM strychnine (Sigma), and 100 µMpicrotoxin (Tocris) to block N-methyl-D-aspartate (NMDA), AMPA,glycine, and GABA_A receptors, respectively. Additional drugswere added as required, including 0.5–2 µM TTX (AlamoneLabs) to block voltage-gated Na channels, 15 µM nimodipine(Tocris) or 400 µM Cd²⁺ (Sigma) to block voltage-gatedL-type Ca channels, and 20 µM riluzole (Tocris) to blockpersistent sodium currents.

Persistent inward currents in current- and voltage-clamp recording

Slow triangular current ramps (0.4 nA/s) were applied to themotoneurons to measure firing and basic cell properties (Fig. 1B).The input resistance was measured during the ramp over a 5-mVrange near rest and subthreshold to PIC onset. The firing level,or spike voltage threshold (V_th), was averaged from five consecutivespikes starting with the second spike on the up ramp, and wastaken as the potential at which the rate of change of membranepotential (dV/dt) first exceeded 10 V/s (Li et al. 2004a). Thespike overshoot (>0 mV) was calculated as the average peakdepolarization during the action potential from these same fivespikes. Bistable behavior was quantified by measuring self-sustainedfiring ( ${Delta}$ I): that is, when the motoneuron continued to fire atless current than was initially required to recruit firing.This was quantified during current ramps by subtracting thecurrent at derecruitment (I_end) from the current at recruitment(I_start), so that ${Delta}$ I = I_start – I_end. A subthreshold activationof the PIC (e.g., subthreshold plateau) was identified by extrapolatingto higher potentials the linear subthreshold current-voltagerelation (Fig. 1B, thin line) from a region $≥$ 5 mV below spikevoltage threshold and comparing this to the actual depolarization.In motoneurons with large PICs, the plateau potential was seenas a subthreshold acceleration (Fig. 1B, arrowhead) in membranepotential before the first spike, and a long after-depolarizationafter cessation of firing (Fig. 1B, double arrow). Instantaneousfiring frequency (F) as a function of current (F-I relation)was computed using a custom Linux-based program (G.R. Detillieux,Winnipeg, Canada) from the current ramp recordings (Fig. 1C).The F-I slope was calculated for linear regions of the F-I relationusing a regression. Minimum firing rate was determined by takingthe average of the last interspike interval from two to threeconsecutive current ramps or from threshold current steps inthe case of motoneurons that did not fire during normal slowcurrent ramps. Antidromic spike height was measured after stimulationof the ventral roots while the cell was at rest.

Slow triangular voltage ramps (3.5 mV/s), from approximately–80 to –40 mV and back to –80 mV, were usedto quantify the PICs (Fig. 1D). During the increasing portionof the ramp, the current initially increased linearly with voltagebecause of the passive leak conductance. A linear relation wasfit in this region (10 mV below the PIC onset) and extrapolatedinto more depolarized potentials (Fig. 1D, thin line labeledleak current). With further depolarization, there was a downwarddeviation from this extrapolated leak current, as the PIC wasactivated (at V_START). The PIC was quantified as the peak amplitudeof this downward deviation (initial peak on up ramp; Fig. 1D,downward arrow). Large PICs caused an outright negative slopein the current response [Fig. 1E; negative-slope region (NSR)in the I-V relation]. Smaller PICs produced a downward deflectionin the current response (flattening of I-V slope) without producinga NSR (as in Fig. 2B). A linear current response, not deviatingdownward from the leak current line (linear I-V relation), wastaken to indicate the absence of any PIC (as in Fig. 5B). Theonset voltage of the PIC, V_START, was defined as the voltageat which the slope of the I-V relation was reduced to halfwayfrom the leak current slope (maximum slope) to the minimum positiveslopes (halfway to 0 in the case of cells with a NSR). Thisis different from the onset voltage that we previously definedfor the PIC, V_on, which was simply the voltage at which theI-V slope first reached zero (Li and Bennett 2003). However,V_on is not possible to pick in cells without an NSR. Thus wedo not use V_on.

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FIG. 2. Motoneurons from acute spinal rats have small PICs. A: recording of a motoneuron in acute spinal rat that did not exhibit any self-sustained firing during a triangular current ramp ( ${Delta}$ I = 0 nA). B: voltage-clamp recording from same cell with slow voltage ramp starting at –80 mV (horizontal mark). Note small PIC that induces an inflection (flattening) in current response. C: different motoneuron from acute spinal rat with small subthreshold acceleration in membrane potential before the 1st spike and small afterdepolarization after cessation of firing (arrowhead). Firing frequency increased linearly with current, and there was a small amount of self-sustained firing ( ${Delta}$ I > 0 nA; see METHODS). D: voltage ramps for cell in C showing PIC inducing a small NSR associated with self-sustained firing ability. E: motoneuron from chronic spinal rat showing much greater self-sustained firing (greater ${Delta}$ I), and nonlinearity (acceleration) in firing frequency induced by Ca PIC onset (double arrow). F: large PICs and NSR associated with self-sustained firing in E. Scale bars in A apply to C and E. Scale bars in D also apply to F.

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FIG. 5. Variability in repetitive firing ability is related to Na PIC amplitude. All recordings (A–F) are from motoneurons of acute spinal rats with 15 µM nimodipine present to block Ca PICs (same format as Fig. 2). A: motoneuron that was unable to initiate repetitive firing with standard slow current ramps, although it had a full-height spike (inset) in response to antidromic stimulation (up arrow). B: motoneurons with poor firing ability, as in A, lacked Na PICs (linear current response to voltage ramp; same cell as in A). C: typical motoneuron for acute spinal rats, with small subthreshold acceleration (arrowhead) and repetitive firing (top of spikes clipped), but no self-sustained firing ( ${Delta}$ I = 0 nA). D: these typical motoneurons had small Na PICs that only caused a flattening in the current response to a voltage ramp and no NSR. Note that V_START occurs below firing level (V_th). E: extreme motoneuron that had self-sustained firing ( ${Delta}$ I > 0 nA) and relatively low minimum firing rate (<6 Hz). Note large subthreshold acceleration (arrowhead) and after-potential (double arrow), indicating underlying Na plateau. F: same motoneuron as in E had a Na PIC large enough to induce an NSR. Horizontal marks at left of frequency plots indicate 10 Hz.

Data analysis

Data were analyzed in Clampfit 8.0 (Axon Instruments), and figureswere made in Sigmaplot 8.0 (Jandel Scientific). Data are shownas mean ± SD. A Student's t-test was used to test forstatistical differences, with a significance level of P <0.05.

RESULTS

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

Resting membrane potential of motoneurons in acute spinal rats is more hyperpolarized relative to the firing threshold than in chronic spinal rats

The whole sacrocaudal spinal cord was removed from 41 normaladult rats (1–6 mo old) and maintained in vitro. Becausethe cord was transected at the time of removal, this was termedthe acute spinal condition. Sharp intracellular recordings weremade from a total of 58 motoneurons in these acute spinal rats.These motoneurons were compared with a further 42 motoneuronsthat were likewise recorded in vitro, but their cords were takenfrom 34 rats that had undergone a sacral spinal cord transectionover 1.5 mo previously (chronic spinal condition). In controlmotoneurons recorded before application of TTX or nimodipine,the average resting membrane potential (V_m) was about 2 mV morehyperpolarized in acute spinal rats (–72.7 ± 5.8mV; n = 28) than in chronic spinal rats (–70.6 ±7.2 mV; n = 20), although this was not significant because ofthe large variability between cells. Likewise, the average spikevoltage threshold (V_th) was about 2 mV more depolarized in acutespinal rats (V_th = –50.9 ± 6.2 mV) than in chronicspinal rats (V_th = –52.9 ± 7.4 mV, measured duringcurrent ramp as in Fig. 1B), although again this was not significant.However, the difference V_th – V_m was significantly largerin acute spinal rats (21.6 ± 5.9 mV) than in chronicspinal rats (17.4 ± 6.2 mV). Thus motoneurons in acutespinal rats rested further from threshold (hyperpolarized byabout 4 mV) than in chronic spinal rats.

The membrane input resistance (R_m), measured near rest, wasalso significantly lower in acute spinal (5.2 ± 2.3 M ${Omega}$ )compared with chronic spinal (6.7 ± 2.9 M ${Omega}$ ) rat motoneurons.During current ramps, acute spinal rat motoneurons requiredsignificantly more current to fire (3.7 ± 2.5 nA) comparedwith chronic spinal rat motoneurons (1.8 ± 1.2 nA), consistentwith the lower input resistance and higher spike threshold relativeto rest (V_th –V_m) in acute spinal rats. Thus motoneuronsin acute spinal rats were more difficult to activate than inchronic spinal rats.

The spike height and overshoot (absolute value over 0 mV), asmeasured during current ramps, were not significantly differentin acute and chronic spinal rats (92.0 ± 8.7 and 19.3± 7.3 mV, respectively, in acute spinal rats vs. 88.3± 10.5 and 17.7 ± 7.3 mV in chronic spinal rats).

Normal motoneurons have small, but variable, PICs after acute spinal transection

When a slow voltage ramp was applied to a motoneuron in theacute spinal rat, the recorded current increased relativelylinearly in the subthreshold region near rest, because of thepassive leak current (Fig. 2B, thin line), but at more depolarizedlevels between –60 and –45 mV, the current usuallydeviated downward from the linearly extrapolated leak current(Fig. 2B, downward arrow from thin line). This downward deviationfrom the leak current was used as an estimate of the net PIC.For acute spinal rats, this PIC was 1.11 ± 1.21 nA (n= 28; Fig. 3C), which was significantly smaller than the netPIC for chronic spinal rats (2.79 ± 0.94 nA, n = 7; Fig. 3C;PIC measured in all cases at its peak on the upward currentramp, at downward arrow in Fig. 2, B, D, and F). The averageonset voltage, V_START, for the acute spinal rats was –57.2± 5.0 mV (Fig. 3B).

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FIG. 3. TTX-sensitive Na PICs and TTX-resistant Ca PICs in motoneurons of acute spinal rats. A: current response to voltage ramp before and after TTX application, with leak current shown with thin line (as in upward ramp of Fig. 2D). PICs indicated by downward arrows. Notice reduction in PIC with TTX, leaving only a TTX-resistant PIC (Ca PIC). B: filtered data from A with the leak current (thin line in A) subtracted (leak-subtracted current), and plotted against voltage. Trace labeled total PIC is the leak-subtracted current in normal artificial cerebrospinal fluid (nACSF), and trace labeled Ca PIC is the leak-subtracted TTX-resistant current in A, which is Cd²⁺-sensitive (data not shown). Trace labeled Na PIC is difference between total PIC and Ca PIC (TTX-sensitive PIC). C: averages of total PIC, Na PIC, and Ca PIC peak amplitudes from all acute and chronic spinal rats tested with TTX, each significantly larger in chronic spinal rats.

Among acute spinal rat motoneurons, the amplitude of the PICwas highly variable. Some motoneurons (25.0%, n = 7/28) hadsmall PICs that only produced an inflection in the current response,lowering the slope, but not producing an NSR (Fig. 2B). A further28.6% (n = 8/28) of motoneurons did not exhibit detectable PICsat all, in that the current response was linear (data not shown,but see Fig. 5B). Finally, the remaining motoneurons (46.4%,n = 13/28), had PICs large enough to produce an NSR in the currentresponse (Fig. 2D), although the depth of this NSR of these13 cells was usually small (0.84 ± 0.63 nA) and significantlysmaller than in a comparable population of motoneurons fromchronic spinal rats (1.70 ± 0.55 nA; Fig. 2F). Usually,the PIC amplitudes from all motoneurons of a given rat weresimilar, and the above variability was caused by large between-ratvariations (see DISCUSSION).

Consistent with the small PICs in motoneurons of acute spinalrats, they also had little or no self-sustained firing ( ${Delta}$ I small;see METHODS). That is, the ${Delta}$ I in acute spinal rats was 0.16 ±0.44 nA, which was significantly smaller than in chronic spinalrats ( ${Delta}$ I = 0.57 ± 0.42 nA; Fig. 2E) and not significantlydifferent from zero, consistent with previous reports of bistablebehavior being minimal in acute spinal rats (Bennett et al.2001; Li et al. 2004a). Furthermore, in acute spinal rats, thefiring frequency varied relatively linearly with current (Fig. 2C),in contrast to chronic spinal rats where there was at timesan abrupt acceleration in firing (nonlinearity; Fig. 2E, doublearrow) that has previously been shown to be caused by the onsetof a large Ca PIC (Li et al. 2004a).

Although ${Delta}$ I was generally low in acute spinal rats, an NSR inthe total PIC was linked to self-sustained firing. Of the motoneuronsthat had an NSR, 11/13 exhibited some small degree of self-sustainedfiring, with an average ${Delta}$ I = 0.34 ± 0.40 nA. For the sevencells with a PIC but no NSR, however, there was, on average,no significant self-sustained firing (average ${Delta}$ I = 0.00 ±0.27 nA). Finally, the cells that did not exhibit appreciablePICs never had self-sustained firing (n = 8/8); indeed, repetitivefiring did not usually occur at all in these cells (see Fig. 5A).

Persistent sodium and calcium currents make up the total PIC in acute spinal rats

The PICs in motoneurons of acute spinal rats resulted from twomajor currents: a TTX-sensitive Na PIC and a nimodipine-sensitivepersistent Ca PIC (mediated by nimodipine-sensitive L-type calciumchannels). That is, TTX (2 µM) reduced the PIC significantlyby 40.8 ± 10.1% (n = 7; Fig. 3A), suggesting that nearlyone-half the PIC was caused by Na PICs. This TTX-sensitive currentwas directly measured by subtracting the current response beforeand after TTX as shown in Fig. 3B (trace labeled Na PIC); itwas 0.44 ± 0.36 nA and had an onset voltage of –61.3± 3.6 mV (V_START in Fig. 3, A and B). The remaining PICin TTX was quantified by subtracting the leak current (see METHODS;Fig. 3B, middle trace, labeled Ca PIC). This remaining TTX-resistantPIC was 0.78 ± 0.82 nA (or 59.2% of the total PIC), hadan onset voltage of –54.5 ± 3.6 mV, and was mediatedby calcium currents (Ca PIC) because it was blocked by the nonspecificcalcium channel blocker cadmium (400 µM, n = 4), as inchronic spinal rat motoneurons (Li and Bennett 2003). Nimodipine(15 µM) and TTX (2 µM) also completely blocked thePIC (n = 7), so the Ca PIC was mediated by the nimodipine-sensitiveL-type calcium channel [likely by the low-threshold CaV(1.3)L-type Ca channel, Xu and Lipscombe 2001]. Thus as in motoneuronsof chronic spinal rats (Li and Bennett 2003), the PIC in acutespinal rat motoneurons consists of only two major currents,a Na PIC and Ca PIC, both of which were initiated subthresholdto spike threshold (–50.9 mV).

The reduction of the PIC by 2 µM TTX (as in Fig. 3) wasrapid and occurred just before the block of all fast sodium-spikingability in the motoneuron (at about 2 min after application),supporting the idea that the main action of TTX on the PIC wasto directly block the sodium channels underlying the Na PICin the motoneuron. TTX also blocks any spike-mediated transmitterrelease onto motoneurons, and thus may possibly have indirecteffects on the Ca PIC, if the Ca PIC depends on this transmitterrelease (e.g., 5-HT release). However, this indirect effectshould be slow, because of the slow actions of such neuromodulatorson the Na PIC (>10 min; Harvey et al. 2005a,b) and is thusunlikely to have affected the above results, considering therapid action of TTX. Furthermore, as detailed below, the Caand Na PICs do not depend on neuronal activity in the spinalcord in general, because they persist for many hours with allfast synaptic transmission blocked with CNQX, AP5, strychnine,and picrotoxin (without TTX; see METHODS). Thus we interpretthe TTX-sensitive PIC as a Na PIC on the motoneuron, as shownpreviously in chronic spinal rats (Li and Bennett 2003).

The Na PIC was also measured by first applying nimodipine (15µM) to block the Ca PIC (Fig. 4A). The remaining PIC innimodipine was purely a Na PIC (seen after leak current subtractionin Fig. 4B), because it was quickly and completely blocked by2 µM TTX (nimodipine + TTX traces in Fig. 4, A and B).The motoneuron in Fig. 4, A and B, had a particularly largePIC and clearly shows the PIC components. Figure 4, C and D,shows a motoneuron with a PIC more typical of acute spinal rats.On average, the Na PIC measured in nimodipine was 0.55 ±0.74 nA (n = 31 motoneurons), and its onset voltage (V_START= –62.3 ± 6.2 mV) was significantly lower thanthe spike threshold (V_th = –50.9 ± 6.2 mV). ThisNa PIC was 49.5% of the total PIC measured without nimodipine(1.11 ± 1.21 nA, n = 28). Thus the Ca PIC blocked bynimodipine was, on average, 50.5% of the total PIC. This isclose to the proportion of the PIC eliminated by a completecalcium channel block with cadmium (400 µM; 69.7 ±12.8%; significant reduction; n = 3) and the proportion remainingafter addition of TTX (59.2%), suggesting again that the CaPIC is mediated by nimodipine-sensitive L-type calcium channels.Comparing across all cells in acute spinal rats, the Na PIC(peak Na PIC measured on upward ramp, as usual) was not significantlycorrelated with the input conductance measured at rest (correlationcoefficient r = 0.06, n = 31, P = 0.7).

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FIG. 4. Ca PIC is blocked by nimodipine, leaving only a TTX-sensitive Na PIC in motoneurons from acute spinal rats. A: same format as Fig. 3A, but with 15 µM nimodipine added 1st to block L-type calcium channels mediating the Ca PIC. Downward arrows indicate amplitude of total PIC before nimodipine (left) and Na PIC in nimodipine (right). Addition of TTX blocked Na PIC, leaving linear current response. B: filtered and leak-subtracted currents from A, plotted against voltage (I-V plots, as in Fig. 3B), showing total PIC in nACSF, Na PIC in nimodipine, and block of all PICs in nimodipine and TTX. C and D: same format as A and B, but from different acute spinal rat motoneuron with smaller, more typical Na PIC remaining in nimodipine. TTX was not added in this motoneuron.

Using nimodipine to isolate and quantify the Na PIC is particularlyconvenient for several reasons: 1) the PIC measured in nimodipinewas clearly blocked by TTX and very similar to the TTX-sensitivecurrent measured before nimodipine application in other cells(0.55 ± 0.74 nA compared with 0.44 ± 0.36 nA;Figs. 4B vs. 3B); 2) fast sodium spikes were not affected bynimodipine (see Li et al. 2004a

) and thus the relation betweenthe Na PIC and firing could be studied; and 3) multiple motoneuronrecordings and Na PIC estimates could be obtained in the samepreparation, unlike with estimating the Na PIC by direct TTXapplication, where no further motoneurons could be located andidentified in TTX, because the antidromic ventral root activationof the motoneurons was irreversibly blocked. Thus the nimodipine-resistantPIC was used as the standard method of quantifying the Na PICin this and in our companion papers (Harvey et al. 2005a

In nimodipine, the majority of motoneurons (58.8%; n = 20/34)had a small Na PIC that was not large enough to produce an NSRin the current trace, but instead only produced a flatteningor inflection, as in Fig. 5D. A few motoneurons had a largeenough Na PIC to produce an NSR (11.8%; n = 4/34), as in Fig. 5F.The remaining cells (29.4%, 10/34) exhibited no detectable NaPIC, with a relatively linear I-V relation, as in Fig. 5B.

Na PIC and Ca PIC are both much larger after chronic injury

The sodium and calcium components of the PIC in motoneuronsof chronic spinal rats were much larger than those measuredin acute spinal rats. Consistent with our earlier observations(Li and Bennett 2003), the total PIC in chronic spinal rat motoneuronswas 2.79 ± 0.94 nA (n = 7 cells before TTX application;see Fig. 3C and large PIC in Fig. 2F), and this was reducedin TTX by 0.97 ± 0.46 nA (34.8%; TTX-sensitive Na PIC),leaving a 1.82 ± 0.78 nA calcium PIC (65.2% of total)that was nimodipine-sensitive. Likewise, when nimodipine wasadded alone to motoneurons of chronic spinal rats, the remainingPIC (Na PIC estimate in nimodipine) was 1.31 ± 0.93 nA(n = 19), which was similar to the Na PIC measured by directapplication of TTX (0.97 ± 0.46 nA). Either method ofestimating the Na and Ca PICs gave currents in chronic spinalrats that were more than double those in acute spinal rat motoneurons(Na PIC 220–238%, and Ca PIC 233–264% of the valuesin acute spinal rat motoneurons, both differences significant;Fig. 3C). These large PICs almost always produced NSRs in theI-V relation (n = 17/20), as in Fig. 2F, and as previously reported(Li and Bennett 2003). In chronic spinal rats, the onset voltage(V_START) of the Na and Ca PICs were, respectively, –65.3± 6.3 and –57.1 ± 7.1 mV, which were a fewmillivolts lower, although not significantly different, thanthe corresponding V_START values in acute spinal rats. The NaPIC onset (V_START) was significantly lower than the spike voltagethreshold (V_th), as in acute spinal rats. In summary, afterchronic spinal injury, the PICs were twice as large as thoseseen in acute spinal injury, but were still made up of Na andCa PICs in similar proportions (about 40% Na PIC and 60% CaPIC) and with similar onset voltages. Across all motoneuronsof chronic spinal rats, the Na PIC was weakly, but significantly,correlated with the input conductance (correlation coefficientr = 0.47, n = 19, P = 0.04).

PICs do not require fast synaptic transmission or spike-mediated transmission

With the exception of some motoneurons to which we initiallyadded TTX or Cd²⁺ (e.g., Fig. 3), all the results describedin this paper were recorded during a complete blockade of fastsynaptic transmission using CNQX, AP5, strychnine, and picrotoxinto block the AMPA/kainate, NMDA, glycine, and GABA_A receptors,respectively (see METHODS). Under this condition, the totalPIC was not significantly different to the total PIC previouslyreported without this synaptic blockade (Li and Bennett 2003).Thus the total PIC did not depend on fast synaptic transmission(such as NMDA receptor activation) or associated spinal circuitbehavior. Also, in fast synaptic blockade, large Ca and Na PICsexisted in motoneurons of chronic spinal rats (see Fig. 2F),as seen without this blockade (Li and Bennett 2003). However,there was a tendency (although not quite significant, P = 0.09)for there to be relatively smaller Na PICs in the fast synapticblockade compared with without (Na PIC was 29.6 ± 5.2%of total PIC in synaptic blockade compared with 39.5 ±12.0% without). Thus blockade of fast synaptic transmissionmay have indirectly eliminated a neuromodulator that somewhatfacilitated the Na PIC, and at the same time inhibited the CaPIC, so that there was no net effect on the total PIC. Interestingly,GABA_B receptor activation has this effect on motoneurons (Liet al. 2004c), and thus there may have been tonic GABAergicneuron activity that was blocked by the fast synaptic blockade.

In general, we found that the fast synaptic transmission blockaderendered the cord electrically completely silent, with no spontaneoussynaptic potentials or synaptic noise recorded on the motoneurons(data not shown). Thus if transmitters endogenous to the spinalcord (e.g., 5-HT in cut descending terminals or intrinsic 5-HTneurons) were in part responsible for enabling the large PICsthat we recorded with fast synaptic blockade (see DISCUSSIONand Harvey et al. 2005a), these neuromodulatory transmittersmust have been released from last-order neurons (not dependingon excitation) directly onto the motoneurons. This transmitter(e.g., 5-HT) may have been released from these last-order neuronsin a manner that does not depend on spiking (leak through spontaneousvesicle release) because the Ca PIC persisted for hours ( $≤$ 5 htested) when recorded in the presence of TTX (which blocks spiketransmission and Na PIC, n = 6).

Motoneurons that lack Na PICs show poor repetitive firing

The large variation in Na PICs in acute spinal rats providedan opportunity to examine the role of the Na PIC in recruitmentand firing of motoneurons. In the few motoneurons that entirelylacked Na PICs (Fig. 5B; n = 10/34), repetitive firing was difficultto initiate, as would be predicted given the importance of NaPICs in firing (see riluzole experiments described below; andLee and Heckman 2001; Li et al. 2004a). That is, during ourstandard slow current ramp, firing was not usually initiatedin these neurons (80% of these neurons had no firing, n = 8/10neurons); instead, the response was simply a linear depolarizationof the membrane potential, even when the potential increasedwell past the average spike threshold (–50.9 ±6.2 mV), up to –40 mV (Fig. 5A). In one-half of theseneurons, faster ramps could sometimes initiate high-frequencyfiring (50%; n = 4/8 neurons; data not shown), but the remainingneurons (n = 4/8) could not fire repetitively at all duringramps (Fig. 5A), even during fast current ramps $≤$ 4 nA/s (10 timesnormal slow ramp speed). The latter motoneurons, with no steadyrepetitive firing ability during fast ramps, were able to firetransiently but only during antidromic activation (Fig. 5A,inset) or fast current steps (Fig. 6, A and B). Usually, prolongedstep depolarizations would only generate a few spikes at theleading edge of the step (Fig. 6A). Occasionally, during verylarge current steps, these neurons could fire repetitively throughoutthe step, but only at high rates well above the usual minimumrate in acute motoneurons (>>6 Hz; Fig. 6B).

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FIG. 6. Na PIC amplitude controls firing ability near threshold. All traces recorded in current clamp, with depolarizing steps from rest in acute spinal rat motoneurons in nimodipine (Ca PIC blocked). A: example motoneuron with no Na PIC (as in Fig. 5B), where only transient firing occurred with depolarizing steps at threshold (left) or above threshold (right). B: different motoneuron with no Na PIC; repetitive firing occurred with large step pulses in this cell, but only at high rates (>>6 Hz), whereas firing was only transient with smaller current steps, like in A (data not shown). Inset in B is close-up on a few spikes. Note that interspike interval is shorter than AHP duration (indicated by box). C: motoneuron with a small Na PIC but no negative-slope region (as in Fig. 5D); in this cell repetitive firing occurred near threshold, and the maximum interspike interval was roughly equal to the AHP duration (inset). D: motoneuron with large Na PIC and NSR (as in Fig. 5F); in this cell, slow steady firing below 6 Hz (horizontal dashed line) was produced when the cell was held near threshold. Note interspike interval much longer than AHP duration (inset), and fast acceleration in membrane potential just prior to each spike (arrowheads). Horizontal mark in current scale bar in D indicates 0 nA. All figures and insets to same scale shown in D.

The neurons that lacked Na PICs (n = 10/34) were not damagedcells in that they exhibited a healthy resting potential (averageV_m = –72.6 ± 4.7 mV) and input resistance (averageR_m = 3.5 ± 1.2 M ${Omega}$ ). More importantly, they also had largehealthy fast sodium spikes (average spike height was 84.3 ±12.7 mV) that could be evoked by antidromic stimulation (Fig. 5A,inset) or current steps (Fig. 6A). Thus the poor spike initiationand repetitive firing in these cells was not caused by a directfailure of the fast sodium spike. Also, based on their inputresistance, antidromic stimulation response latency, spike shape(data not shown), and long afterhypolarization (AHP; Fig. 5A,inset), these recordings were definitely from motoneurons properand not from motor axons. When some firing was evoked in thesemotoneurons without a Na PIC (e.g., with a fast ramp), maximumrate of rise of potential during the first spike of repetitivefiring (dV/dt_max) was significantly less in these neurons (126.8± 41.4 V/s) than in motoneurons that had a Na PIC (163.6± 28.1 V/s). This might, in part, simply be the lackof a Na PIC that accelerates the membrane potential before thespike, but also may reflect greater fast transient sodium channelinactivation, as has previously been suggested in other motoneuronswith spike accommodation (Schlue et al. 1974

). Perhaps the amountof fast sodium channel inactivation and the size of the Na PICare linked, if a common sodium channel underlies both transientand persistent sodium currents (Crill 1996

Recruitment and firing occurs in acute spinal neurons with small Na PICs

In contrast to motoneurons without Na PICs, motoneurons thathad even small Na PICs were readily recruited and fired repetitivelyduring slow current ramps (Fig. 5C, in nimodipine). Typically,motoneurons in acute spinal rats had small Na PICs that werenot large enough to produce an NSR in the I-V relation, as describedabove (Fig. 5D; n = 20/34), and thus could not exhibit bistablebehavior (e.g., plateaus, self-sustained firing, or after-potentials).However, the Na PIC produced a downward (inward) inflectionin the I-V relation, and this always occurred subthreshold tothe firing level (V_START < V_th); thus the Na PIC was ableto assist in recruiting the neuron. That is, during slowly increasingcurrent ramps, the Na PIC activation caused an accelerationin the depolarization just subthreshold to firing. This subthresholdacceleration was caused by the Na PIC, because it was blockedby TTX (see Fig. 10D), and it did not occur in cells that didnot have a Na PIC, even when a fast ramp was used to inducefiring (data not shown). Furthermore, motoneurons without aNa PIC did not fire during slow ramps, as described above, andthus it is this Na PIC-mediated subthreshold acceleration thatis critical for initiating spiking with normal speed currentramps (see DISCUSSION). In some neurons with clear Na PICs,this subthreshold acceleration was accompanied by a small oscillationin the membrane potential (noise) just before recruitment (about2-mV oscillations at about 10 Hz; e.g., left of inset in Fig. 7B; also see Fig. 6A in Li et al. 2004a), and this oscillationwas also mediated by sodium currents (e.g., Na PIC, as in Geijo-Barrientosand Pastore 1995) because it was not seen in TTX. In these cells,the first spike at recruitment was triggered by one of thesenoisy oscillation cycles.

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FIG. 10. Selectively blocking the Na PIC eliminates repetitive firing but not the fast sodium spike. A: motoneuron from chronic spinal rat recorded in nimodipine showing typical repetitive firing during slow current ramps. B: current-voltage plot response to slow voltage ramp in nimodipine, for same cell as in A. Note the clear NSR and large Na PIC (downward arrow). C: overlay of the 1st spike from current ramp in nimodipine (thin line, from A) with the 1st spike from current step in nimodipine plus low-dose TTX (dots; from spike in F). D: application of low-dose TTX (0.5 µM) to the cell in A and B (with nimodipine present) eliminated all repetitive firing ability during slow current ramps, even though the fast sodium spike was not blocked (C and F). E: Na PIC was blocked by low-dose TTX, when lack of firing in D was recorded. F: in low-dose TTX, current steps still elicited 1–3 spikes, indicating transient sodium currents were not blocked. G: another motoneuron with riluzole (20 µM), rather than TTX, used to block the Na PIC (PIC not shown). Again, only transient firing was possible during current steps (G) and not ramps (not shown). H: with the Na PIC blocked in riluzole, motoneurons could still fire in response to repeated antidromic stimulation (1 spike for each stimulation at arrow; 10 Hz repetition); thus the spike was still capable of being activated repeatedly. I: Same as H, but at 20-Hz antidromic stimulation. Spike activation eventually failed (*) with repeated high-frequency stimulation.

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FIG. 7. Motoneurons of acute spinal rats, with large enough Na PICs to produce an NSR, exhibited steady very slow firing similar to that commonly seen in chronic spinal rats. A: top: current clamp recording of chronic spinal rat motoneuron held near threshold (in nimodipine). Brief depolarizing current pulse initiated a Na plateau and self-sustained firing at very low average frequency (2.6 ± 0.4 Hz), terminated by a hyperpolarizing current pulse (right). Bottom: amplification of top showing long interspike intervals (longer than AHP). Note that the Na PIC was activated before each spike (Na plateau above V_START, fast acceleration at arrowhead), but the AHP dropped the membrane potential below V_START, which deactivated the Na PIC/plateau. B: top: motoneuron from acute spinal rat (in nimodipine) that had Na PIC large enough to produce an NSR, also had steady slow firing mediated by Na plateaus as in A. Bottom: steady repetitive firing at frequencies below 6 Hz, with interspike intervals again greatly exceeding the AHP duration (determined from antidromic stimulation at rest). Again, note activation of Na plateau (vertical arrows) and fast acceleration (arrowhead) before spike. Scale bars in B also apply to A. Horizontal mark at bottom of frequency scale bars indicates 0 Hz.

In most motoneurons of acute spinal rats with typical smallNa PICs (not large enough to produce an NSR) after recruitment,the firing continued at currents above the recruitment threshold,but, as soon as the injected current dropped below recruitmentthreshold (during the downward current ramp), firing stoppedand the potential decreased symmetrically to the response onthe upward ramp (no after-potential; Fig. 5C, in nimodipine).These cells showed no self-sustained firing during slow currentramps ( ${Delta}$ I never more than 0; Fig. 5C) and at times exhibitedsome late spike frequency adaptation, with ${Delta}$ I < 0 (data notshown), unlike in chronic spinal rats (Li et al. 2004a

) or inacute spinal rats with NSRs induced by a large Na PIC (Fig. 5E).

In these neurons without a large enough Na PIC to produce anNSR, the average minimum firing rate was 8.3 ± 3.1 Hz,and the corresponding interspike interval was 120 ± 45ms, which was similar to the AHP duration (50–150 ms;Fig. 6, B and C; see also Li et al. 2004a). Importantly, theseneurons never produced steady very slow firing (<6 Hz) asdescribed below for neurons with an NSR. Thus a Na PIC–inducedNSR is critical for steady slow firing at <6 Hz.

Motoneurons with an NSR had enhanced firing

A few motoneurons of acute spinal rats (n = 4/34) exhibitedsuch large spontaneous Na PICs (measured in nimodipine; Fig. 5F)that they had a large NSR in the current-voltage relation, whichtheoretically indicated that these cells should exhibit all-or-nothingbistable behavior (sodium plateau potentials and self-sustainedfiring), as is common in motoneurons of chronic spinal rats(Li et al. 2004a). Indeed, these large Na PICs were associatedwith self-sustained firing during triangular current ramps ( ${Delta}$ I> 0; Fig. 5E) or after pulses (Fig. 7B). Also, these motoneuronswith large Na PICs had subthreshold sodium plateau potentialsthat led to a large acceleration in potential before recruitment(Fig. 5E, arrowhead), and an after-potential after derecruitment(double arrow). Ultimately, the response to the triangular currentramp was asymmetrical, with more firing on the downward rampand a prolonged depolarization (after potential), unlike inother acute spinal rat motoneurons. The subthreshold accelerationbefore recruitment was caused by the Na PIC, because it wasblocked by TTX (data not shown), as described above for cellswith smaller Na PICs, and clearly led to the initiation of thefirst spike during a current ramp.

Large Na PICs allow very slow steady firing

These few extreme motoneurons in acute spinal rats with largeenough Na PICs to produce an NSR all produced very slow firing(<6 Hz, corresponding to interspike intervals much longerthan the AHP duration) when the membrane potential was nearthreshold (Figs. 6D and 7B); this, too, relied on the bistable(plateau) behavior of the Na PIC. On average, the minimum firingrate in these four cells (5.0 ± 0.8 Hz) was significantlylower than the average minimum rate in motoneurons of acutespinal rats without NSRs (8.3 ± 3.1 Hz) and closer tothat in chronic spinal rats (4.6 ± 1.9 Hz, in nimodipine).

Previously, Li et al. (2004a) showed that chronic spinal ratmotoneurons with large Na PICs exhibit similar very low frequencysteady firing (very slow firing, much <6 Hz) with interspikeintervals $≤$ 1 s and much longer than the AHP duration (50–150ms). This very slow firing depends on the Na PIC (eliminatedby a Na PIC block) but not the Ca PIC (nimodipine-resistant,Li et al. 2004a). We also found that motoneurons of chronicspinal rats exhibited very slow firing (in nimodipine); furthermore,we found that this very slow firing persisted in the presenceof fast synaptic transmission blocking agents (including AP-5)and thus does not depend on persistent calcium currents or NMDAreceptors (Fig. 7A).

The detailed mechanism of how the Na PIC causes very slow firingis shown in Fig. 7 for both chronic and acute spinal rats (seealso Li et al. 2004a). When the membrane potential was justsubthreshold for the spike, the Na PIC came on slowly, causingan initially slowly increasing subthreshold sodium plateau (seeslow ramp-up in potential at vertical arrow in Fig. 7A). Furthermore,as the potential depolarized during this plateau, the Na PICcame on much more quickly (Na PIC is a fast current at moredepolarized levels; Li and Bennett 2003), and thus helped acceleratethe potential just before the spike (at arrowheads), and ultimatelyhelped initiate a spike (left of inset in Fig. 7, A and B).However, because the Na PIC deactivates quickly with hyperpolarization(Li and Bennett 2003), the spike's AHP deactivated the Na PICs/plateau(potential well below V_START of Na PIC, thin line) and leftthe membrane potential again just subthreshold for the spikeat the end of the 100-ms AHP (AHP estimated from antidromicpulse at rest, indicated with bar). The sodium plateau thenreactivated (bracketed by thick arrows) and produced a secondspike, but again this plateau was terminated by the AHP. Thisrepeated sodium plateau (Na PIC) activation and deactivationbehavior caused slow firing, because this slow firing was eliminatedwith a low dose of TTX (0.5 µM) or riluzole (20 µM)that reduced the Na PIC and eliminated the NSR before blockingspiking (data not shown, but see Li et al. 2004a).

Considering the dependence of slow firing on the Na PIC, thelarger Na PICs in chronic spinal rat motoneurons should explainthe higher incidence of slow firing compared with that of acutespinal rats; furthermore, cells with larger Na PICs ought to,in general, have lower minimum rates. To examine this, we determinedthe relationship between the minimum firing rate and the NaPIC amplitude (Fig. 8A). For chronic spinal rat motoneurons,there was indeed a significant correlation between Na PIC amplitudeand the minimum firing rate ( $bullet$ , thick regression line; r = 0.538,n = 19, P = 0.02), and most of these motoneurons had an NSR(Fig. 8B, $bullet$ ). Furthermore, cells with Na PICs >1.3 nA (meanNa PIC amplitude) had a much lower minimum firing rate (3.3± 1.2 Hz, n = 7) compared with the minimum rate in cellswith Na PICs <1.3 nA (5.4 ± 1.8 Hz; n = 12; significantdifference). Acute spinal rat motoneurons exhibited a trendtoward this relationship, but the correlation was not quitesignificant ( ${circ}$ , thin regression line; r = 0.302, n = 25, P =0.1) because there were only a few neurons with a large Na PIC.However, the four cells that did have a large enough Na PICto produce a clear NSR ( ${circ}$ at right of Fig. 8B) exhibited someof the slowest firing among this group of cells (<6 Hz, significantlylower rate than cells without an NSR). Thus larger persistentsodium currents, especially those that induced NSRs, are associatedwith lower minimum firing rates.

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FIG. 8. Na PIC amplitude correlates with minimum firing rate. A: in chronic spinal rat motoneurons ( $bullet$ , thick regression line), large Na PICs correlated significantly with low minimum firing rates (r = 0.538). Acute spinal rat motoneurons ( ${circ}$ , thin regression line) also had a trend toward Na PICs correlating with minimum firing rates, but this was not significant. B: motoneurons with an NSR in current trace were more likely to exhibit steady slow firing (<6 Hz, below horizontal dashed line). The 4 acute spinal rat motoneurons with an NSR ( ${circ}$ at right) had minimum firing rates at the low end of range for normal motoneurons. With chronic spinal injury, many more motoneurons had an NSR in current trace and these had an average minimum firing rate below 6 Hz.

Frequency-current slope is not related to Na PIC amplitude

When only a Na PIC was present (with Ca PIC blocked with nimodipine),during increasing current ramps, the firing rate response increasedrelatively linearly (linear F-I relation; Fig. 5E). As previouslyreported (Li et al. 2004a), this is because the Ca PIC causesthe main nonlinearity in the F-I relation (acceleration in firing;Fig. 2E, top, double arrow), and this nonlinearity is blockedby nimodipine. On average, the slope of the F-I relation innimodipine was significantly smaller in chronic spinal rats(5.5 ± 1.6 Hz/nA; n = 16) compared with in acute spinalrats (7.4 ± 2.3 Hz/nA; n = 16; Fig. 9, right). Becausethe chronic spinal rats have larger Na PICs, this might suggestthat a shallower F-I slope is associated with larger Na PICs.However, the F-I slope was not significantly correlated to NaPIC amplitude in either acute or chronic spinal rat motoneurons(Fig. 9; acute: thin line, r = 0.157; chronic: thick line, r= 0.138). We also found that the F-I slope was not significantlycorrelated with the minimum slope-conductance of the I-V relation,G_min (where G_min is the slope of the I-V relation at the NSRin cells with a NSR, or just the minimum slope in other cells;r = 0.221, n = 18, P = 0.4). Thus the F-I slope is not relatedto the Na PIC, unlike with the Ca PIC (Li et al. 2004a). Consideringthat changes in the Na PIC are not associated with changes inthe F-I slope, whereas increases in the Na PIC lower the minimumfiring rate, the major action of the Na PIC on the F-I relationis to vertically shift the F-I relation to lower rates (cf.frequency plots in Fig. 5, C and E), allowing an overall broaderrange of firing (maximum rate in acute and chronic spinal ratsis similar, data not shown).

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FIG. 9. F-I slope is not related to the Na PIC amplitude. F-I slope measured from response to slow current ramps in the presence of nimodipine (Ca PIC blocked) in motoneurons from acute spinal ( ${circ}$ , thin regression line) and chronic spinal ( $bullet$ , thick regression line) rats, and plotted against Na PIC amplitude. No significant correlation was observed between F-I slope and Na PIC amplitude in either group. Average F-I slopes plotted at right show that motoneurons of acute spinal rats had significantly higher F-I slopes than motoneurons of chronic spinal rats.

Na PICs are essential in firing

To definitively prove that the Na PIC was essential for steadyrepetitive firing, we blocked the Na PIC without blocking thespike, using either a low dose of TTX (<1 µM, n = 6)or riluzole (20 µM, n = 9, combined data from acute andchronic spinal rats). When low-dose TTX was applied to a motoneuron,the Na PIC was blocked (Fig. 10, B and E) before affecting thefast sodium spike (Fig. 10C), because the Na PIC is more sensitiveto sodium channel blockers (Stafstrom et al. 1985). This lowdose of TTX (0.5 µM; as in Fig. 10, D–F) gave alonger period of time where the fast sodium spike was unaffectedwhile the Na PIC was blocked (minutes; Na PIC measured in nimodipine),compared with the normal 2-µM dose, which blocked bothalmost simultaneously. Riluzole (20 µM) had the same effectas low-dose TTX, but worked very slowly, taking 1 h to completelyblock the Na PIC (data not shown) and another hour to affectthe fast sodium spike. With either TTX or riluzole, during theperiod when the Na PIC was blocked and the spike was unaffected,the repetitive firing during a current ramp was always eliminated(cf. firing in Fig. 10A to lack of firing in Fig. 10D). Thusthe Na PIC was absolutely essential for spike initiation duringa ramp. During this period, a fast current step still initiateda few spikes (Fig. 10, C and G), and this was how we showedthat the fast spike was unaffected after the Na PIC block (overlappingspikes in Fig. 10C, before and after low-dose TTX). However,this step-evoked firing was never sustained (Fig. 10F in TTXand Fig. 10G in riluzole), and thus sustained repetitive firingalso required a Na PIC. Antidromic activation of the motoneuronsalso initiated normal full-height sodium spikes in riluzole(Fig. 10H).

Repeated short intracellular current pulses (data not shown)or antidromic stimulation at moderately low frequencies (10Hz; Fig. 10H) usually gave repeated full unattenuated spikes,showing that failure to fire repetitively during a ramp or stepinput was not simply caused by a failure of spikes with repetition.However, higher-frequency stimulation (20 Hz) at times led tospike inactivation, with a broadening of the spike over thecourse of many stimulations and ultimately complete failureof spiking (Fig. 10I, *). Such spike inactivation did not occurbefore riluzole or low-dose TTX (see repetitive firing in Fig. 10A),and thus subtle changes in the fast sodium channel inactivationoccurred in addition to the block of the Na PIC with these drugs.Thus spike initiation and repetitive firing depends primarilyon the Na PIC but also on a relative lack of spike inactivation.

The cells just described in Fig. 10 were recorded in the presenceof nimodipine to block the Ca PIC; in these cells, there wasrobust repetitive firing during a current ramp (Fig. 10A) andclear Na PICs (Fig. 10B) before the application of TTX or riluzole.In the absence of nimodipine, application of TTX or riluzoleto block the Na PIC also eliminated repetitive firing duringa current ramp (data not shown) before blocking the fast sodiumspike. Thus the Ca PIC itself is not sufficient for steady repetitivefiring. In low-dose TTX without nimodipine, there was stilla Ca PIC that produced a calcium plateau in chronic spinal rats(Li et al. 2004a), and this sometimes triggered a few spikesat its onset (data not shown). In this way, the Ca PIC onsetacted like a current step (as in Fig. 10, E and G), producinga rapid depolarization that initiated a spike.

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

The results show that normal motoneurons have Na and Ca PICsimmediately after spinal transection (acute spinal condition),but these are small and only increase substantially with long-terminjury (chronic spinal). Interestingly, the PICs occur immediatelyafter spinal transection despite the massive loss of brain stem–derivedmonoamines (5-HT and NE) that normally regulate PICs (Hounsgaardet al. 1988a; Hultborn and Kiehn 1992; Lee and Heckman 1998a).The small PICs in acute spinal rats generally do not lead topronounced bistable behavior (plateau potentials and self-sustainedfiring), consistent with previous studies of acute spinal animals(cat: Conway et al. 1988; turtle: Hounsgaard et al. 1988b; guineapig: Nishimura et al. 1989; rat: Powers and Binder 2003). However,these PICs are usually sufficient to at least produce an inflection(flattening) in the I-V relation, which has previously beenargued to underlie graded amplification of motoneuron responsesnear threshold (as in Fig. 5, see also Li and Bennett 2003;Prather et al. 2001; Schwindt and Crill 1982) and participatein recruitment and repetitive firing.

The results also show that all motoneurons that lack the abilityto produce steady repetitive firing during slow current rampsalso lack a Na PIC, suggesting that Na PICs are necessary forsteady repetitive firing. Conversely, most neurons that didnot have any detectable Na PIC could not fire repetitively duringa slow current ramp. A few of these neurons could fire repetitivelyduring slow ramps (2/10), but this may have been caused by smallNa PICs that were not detectable. That is, even when an I-Vrelation is relatively linear, suggesting no detectable Na PIC(see METHODS), TTX application can at times still reveal a smallTTX-sensitive Na PIC (unpublished data). Taken together, theseresults suggest that repetitive firing is highly correlatedwith the presence of a Na PIC.

To directly prove that the Na PIC is essential for repetitivefiring, the Na PIC must be blocked without blocking the sodiumspike, and this has been done by blocking the Na PIC with riluzoleor low-dose TTX (see RESULTS), or using a depolarization block(Lee and Heckman 2001). In riluzole or low-dose TTX, repetitivefiring is eliminated as expected when the Na PIC is blocked,even though transient firing is possible with a fast currentstep. Thus riluzole creates a situation like in neurons thatnaturally lack Na PICs (cf. Figs. 10D and 5A). This verifiesthe essential role of the Na PIC in repetitive firing, supportingthe conclusions of Lee and Heckman (2001) in cat motoneuronsand Stafstrom et al. (1985) in cat neocortical cells. Furtherevidence for the role of the Na PIC in firing comes from ourcompanion papers, where we show that motoneurons that lack repetitivefiring and Na PICs can be rescued by application of 5-HT₂ receptoragonists, which increase the Na PIC amplitude and thus enablerepetitive firing (Harvey et al. 2005b). Conversely, 5-HT andNE antagonists eliminate the Na PIC and repetitive firing, likeriluzole, although these antagonists do so by indirectly modulatingthe Na PIC through receptors linked to Gq-protein–coupledintracellular pathways (Harvey et al. 2005a).

Variation in Na PIC amplitude with state of animal preparation

In acute spinal rats, the Na PIC is usually large enough toassist in spike initiation and enable repetitive firing, butnot so large as to produce bistable plateau behavior. In a fewextreme acute spinal rat motoneurons (11.8%), the Na PIC isso large that it does produce a substantial NSR in the I-V relationthat enables Na plateaus and slow subthreshold oscillations,resulting in the characteristic very slow firing seen with largeNa PICs (Li et al. 2004a). On the other extreme, in the motoneuronswithout clear Na PICs (29.4%), repetitive firing is poor orabsent, consistent with the fundamental role of the Na PIC inenabling repetitive firing. From the wide variation in Na PICsin acute spinal rats, it is clear that any motoneuron that canproduce steady repetitive firing is likely to have at leasta small Na PIC, and larger Na PICs are associated with slowerfiring (lower minimum rates).

For comparison, it is noteworthy that motoneurons from deeplypentobarbitol-anesthetized animals have no