Downregulation of Tetrodotoxin-Resistant Sodium Currents and Upregulation of a Rapidly Repriming Tetrodotoxin-Sensitive Sodium Current in Small Spinal Sensory Neurons after Nerve Injury

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (265)

Citing Articles via Google Scholar

Google Scholar

Articles by Cummins, T. R.

Articles by Waxman, S. G.

Search for Related Content

PubMed

PubMed Citation

Articles by Cummins, T. R.

Articles by Waxman, S. G.

Previous Article  |  Next Article

Volume 17, Number 10, Issue of May 15, 1997 pp. 3503-3514
Copyright ©1997 Society for Neuroscience

Downregulation of Tetrodotoxin-Resistant Sodium Currents and Upregulation of a Rapidly Repriming Tetrodotoxin-Sensitive Sodium Current in Small Spinal Sensory Neurons after Nerve Injury

Theodore R. Cummins and Stephen G. Waxman
Department of Neurology, Yale University School of Medicine, New Haven, Connecticut 06510, and Neuroscience Research Center, Veterans Administration Medical Center, West Haven, Connecticut 06516

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Clinical and experimental studies have shown that spinal sensory neurons become hyperexcitable after axonal injury, and electrophysiologicalchanges have suggested that this may be attributable to changesin sodium current expression. We have demonstrated previouslythat sodium channel $alpha$ -III mRNA levels are elevated and sodiumchannel $alpha$ -SNS mRNA levels are reduced in rat spinal sensory neuronsafter axotomy. In this study we show that small (C-type) rat spinalsensory neurons express sodium currents with dramatically differentkinetics after axotomy produced by sciatic nerve ligation. UninjuredC-type neurons express both slowly inactivating tetrodotoxin-resistant(TTX-R) sodium current and a fast-inactivating tetrodotoxin-sensitive(TTX-S) current that reprimes (recovers from inactivation) slowly.After axotomy, the TTX-R current density was greatly reduced.No difference was observed in the density of TTX-S currents afteraxotomy, and their voltage dependence was not different from controls.However, TTX-S currents in axotomized neurons reprimed four timesfaster than control TTX-S currents. These data indicate that axotomyof spinal neurons is followed by downregulation of TTX-R currentand by the emergence of a rapidly repriming TTX-S current andsuggest that this may be attributable to the upregulation of asodium channel isoform that was unexpressed previously in thesecells. These axotomy-induced changes in sodium currents are expectedto alter excitability substantially and could underlie the molecularpathogenesis of some chronic pain syndromes associated with injuryto the axons of spinal sensory neurons.
Key words: sodium channel; sodium current; chronic pain; axotomy; dorsal root ganglion; excitability

INTRODUCTION

Although chronic pain affects >60% of spinal cord injury patients (Knutsdottir, 1993; Levi et al., 1995; Subbarao et al.,1995), its pathophysiology is not well understood. One possibilityis that nociceptive spinal sensory neurons generate inappropriateactivity after injury. Spinal sensory neurons become hyperexcitableand generate spontaneous impulses after injury in experimentalanimals (Wall and Gutnick, 1974; Lisney and Devor, 1987; Matznerand Devor, 1994) and humans (Nystrom and Hagbarth, 1981; Nordinet al., 1984). Interestingly, anticonvulsants and local anestheticshave been used at concentrations known to act on sodium channelsto manage chronic pain in humans (Boas et al., 1982; Chabal etal., 1989a; Chabal et al., 1992; Galer et al., 1993; Appelgrenet al., 1996). Matzner and Devor (1992, 1994) proposed that thehyperexcitability associated with chronic pain results from anincrease in sodium channel density at the site of injury. It alsohas been hypothesized that changes in the kinetics and voltage-dependentcharacteristics of sodium currents, possibly because of changesin the expression of sodium channel genes, contribute to the ectopicimpulse generation and hyperexcitability of spinal sensory (dorsalroot ganglion, DRG) neurons after nerve injury (Waxman et al.,1994; Rizzo et al., 1995, 1996).

DRG neurons possess a complicated mix of sodium currents (Caffrey et al., 1992; Black et al., 1996). Kostyuk et al. (1981)first reported that DRG neurons produced at least two types ofsodium currents, including a fast TTX-sensitive (TTX-S) currentand a slow TTX-resistant (TTX-R) current. Two groups recentlycloned a sodium channel isoform (SNS) that is resistant to TTXand is proposed to underlie the TTX-R current in small neurons(Akopian et al., 1996; Sangameswaran et al., 1996). It is notclear which sodium channel isoform or isoforms underlie the TTX-Scurrent. We have shown that normal DRG neurons can express asmany as seven different sodium channel $alpha$ -subunit mRNAs in situand in vitro (Black et al., 1996), and, therefore, more than onesodium channel isoform might contribute to the TTX-S or the TTX-Rcomponent. However, it is not known what the physiological importanceof the different isoforms is or if they have distinct kinetics.

Recently we demonstrated that axotomy induces an increase in the level of the type III and a decrease in SNS sodium channelmRNA in DRG C-type neurons (Waxman et al., 1994; Dib-Hajj et al.,1996), indicating that sodium current properties might be alteredby axotomy. We hypothesized that axotomy increases a TTX-S currentand decreases the TTX-R current in C-type DRG neurons, as previouslydemonstrated in large cutaneous afferent DRG neurons (Rizzo etal., 1995).

In this study we examined the effects of axonal injury on sodium current properties in small (18-25 µm) DRG C-type neurons(which include nociceptive and temperature-sensitive neurons)to determine whether the sodium currents of these neurons indeeddo change after axotomy. Surprisingly, we found that axotomy isfollowed by the expression of a TTX-S current with different kineticproperties, especially recovery from inactivation, as well asdownregulation of the TTX-R current in these cells. The axotomy-inducedemergence of a sodium channel characterized by rapid reprimingmay provide a basis for hyperexcitability in injured DRG neurons.

MATERIALS AND METHODS
Sciatic nerve injury. Axotomy of the sciatic nerve was performed as previously described (Waxman et al., 1994). Under anesthetic,the right sciatic nerve of adult Sprague Dawley female rats wasexposed, and a tight ligature was placed around the sciatic nervenear the sciatic notch proximal to the pyriform ligament. Thenerve was sectioned with fine surgical scissors immediately distalto the ligature site, and the proximal nerve stump was fit intoa silicone cuff. In some experiments the cuff contained 2 µl ofan 8% Fluoro-gold solution for retrograde labeling, which facilitateddefinitive identification of axotomized neurons (Schmued and Fallon,1986). The incision was closed, and the animals were allowed torecover.

Culture of spinal sensory neurons. DRG cells were studied after short-term culture (12-24 hr). The short-term culture (1)provided cells with truncated axonal processes that can be voltage-clampedreadily and reliably, (2) allowed the cells sufficient time toadhere to the glass coverslip, and (3) was short enough to minimizechanges in electrical properties that can occur in long-term cultures.The spontaneous electrical activity characteristic of DRG neuronsafter nerve injury can be observed in isolated injured neurons,but not in isolated control neurons (Study and Kral, 1996), demonstratingthat the isolation procedure does not drastically alter the electrophysiologicalproperties of the DRG neurons. Furthermore, adult rat DRG neuronsmaintained in vitro for 24 hr display a profile of sodium channelmRNA expression similar to that for DRG neurons in situ, indicatingthat short-term culture does not alter substantially the expressionof sodium channel mRNAs in these cells (Black et al., 1996). Itshould be noted, however, that changes in both sodium currentsand mRNA expression can be seen after 7 d in vitro. The culturewas performed as previously described (Caffrey et al., 1992).L4-L5 DRG neurons were cultured between 2 and 60 d postaxotomy(DPA). Only the right sciatic nerve was ligated, and the leftL4-L5 DRG neurons were used as controls.

Whole-cell patch-clamp recordings. Whole-cell patch-clamp recordings were conducted at room temperature (~21°C) with an EPC-9amplifier. Data were acquired on an Macintosh Quadra 950 computerwith the Pulse program (v 7.89, HEKA Electronic, Germany). Fire-polishedelectrodes (0.8-1.5 M $Omega$ ) were fabricated from 1.5 mm Drummond capillaryglass by using a Sutter P-97 puller (Sutter Instruments, Novato,CA). To minimize space clamp problems, we selected only isolatedcells with a soma size of 18-25 µm for recording. Cells were notconsidered for analysis if the initial seal resistance was <5G $Omega$ or if they had high leakage currents (holding current >1.0nA at $-$ 80 mV), membrane blebs, or an access resistance >4 M $Omega$ .Access resistance was monitored throughout the experiment, anddata were not used if resistance changes of >20% occurred. Theaverage access resistance was 2.1 ± 0.6 M $Omega$ (mean ± SD, n = 113)for control cells and 2.0 ± 0.7 M $Omega$ (n = 187) for axotomized cells.Voltage errors were minimized by using 70-80% series resistancecompensation, and the capacitance artifact was canceled by usingthe computer-controlled circuitry of the patch-clamp amplifier.Linear leak subtraction, based on resistance estimates from fourto five hyperpolarizing pulses applied before the depolarizingtest potential, was used for all voltage-clamp recordings. Membranecurrents usually were filtered at 5 kHz and sampled at 20 kHz.The pipette solution contained (in mM): 140 CsF, 1 EGTA, 10 NaCl,and 10 HEPES, pH 7.3. The standard bathing solution was (in mM):140 NaCl, 3 KCl, 1 MgCl₂, 1 CaCl₂, 0.1 CdCl₂, and 10 HEPES, pH7.3. The liquid junction potential for these solutions was <8mV; data were not corrected to account for this offset. The osmolarityof all solutions was adjusted to 310 mOsm (Wescor 5500 osmometer,Logan, UT). The offset potential was zeroed before patching thecells and checked after each recording for drift; if the driftwas >10 mV/hr, the recording was discarded.

In situ hybridization. To compare the patch-clamp results with the expression of SNS mRNA in DRG neurons, we used in situhybridization results from adult rat DRG neurons at DPA5 (Dib-Hajjet al., 1996); this time point was chosen to correspond to electrophysiologicalrecordings at DPA6, allowing for a 1 d lag between mRNA expressionand the appearance of functional channels. The hybridization signalin small (<30 µm in diameter) DRG neurons was scored from 0 to+++, as described by Dib-Hajj et al. (1996).

RESULTS
Sodium currents were recorded from small (18-25 µm) DRG neurons with whole-cell patch-clamp techniques. Control neurons werecultured from the uninjured left L4-L5 DRG of each rat (116 cellswere studied from 14 different cultures). To examine the effectsof injury on sodium currents, we cultured neurons from the axotomizedright L4-L5 DRGs of rats at 2, 6, 22, and 60 d postaxotomy (DPA2,DPA6, DPA22, DPA60). For each time point, 10-15 cells per culturewere recorded from at least three different cultures. Becausenot all of the L4-L5 axons are transected at the level of sciaticnerve ligation (because of branching of the nerve proximal tothe ligation site), it is estimated that only ~70% of the neuronscultured actually were axotomized (Yip et al., 1984; Devor etal., 1985). In most experiments we did not use retrograde labelingand recorded from randomly chosen small C-type neurons. This provideda comparison with the previous study on mRNA expression (Dib-Hajjet al., 1996) in which it was not possible to identify axotomizedneurons unequivocally. For some experiments (specified below),we studied fluorescently labeled axotomized neurons, which wecould identify positively as axotomized neurons. Because the labelingwas weak at DPA2 and DPA60, results on labeled cells are reportedonly for DPA6 and DPA22.

Sodium currents are altered after axotomy
Axotomy had a dramatic effect on the sodium currents of C-type neurons. Figure 1 shows recordings from a typical cell at eachtime point. The sodium currents in control neurons were similarto those previously described in small DRG neurons (Caffrey etal., 1992; Roy and Narahashi, 1992; Elliott and Elliott, 1993;Rizzo et al., 1994). Most control neurons expressed both fast-inactivatingand slow-inactivating sodium currents (Table 1), which we referto as "fast" and "slow," respectively. Axotomy decreased the numberof cells expressing predominantly (>70% of total) slow currentsand increased the number expressing predominantly (>70% of total)fast currents (Table 1) in which the relative contributions wereestimated by using the inflection point in the steady-state inactivationcurves (Fig. 1).
Fig. 1. Axotomy alters the inactivation kinetics and voltage dependence of inactivation of C-type DRG neurons. Left column, Familiesof traces from representative control and axotomized C-type neuronsare shown. Faster inactivation kinetics are observed for the totalsodium current in axotomized neurons. The currents were elicitedby 20 msec test pulses to $-$ 10 mV after 500 msec prepulses to potentialsover the range of $-$ 130 mV to $-$ 10 mV. Middle column, The correspondingsteady-state inactivation curves are shown for each cell. Currentis plotted as a fraction of peak current. In the control neuronthe midpoint for steady-state inactivation (V_h) is $-$ 38 mV. AtDPA2 V_h is $-$ 62 mV, and at DPA6 and DPA22 V_h is $-$ 65 mV. At DPA60V_h is $-$ 50 mV. However, two current components can be resolvedeasily in the control, DPA2, DPA22, and DPA60 cells: a slowlyinactivating component that has a relatively depolarized voltagedependence of inactivation and a fast-inactivating component thathas a more negative V_h. The steady-state inactivation curves forthese cells are bimodal because of the different inactivationproperties of the two components (arrow in B indicates point ofinflection). The DPA6 cell, on the other hand, appears to exhibitonly fast-inactivating currents, and the steady-state inactivationis not inflected. Right column, Repriming (recovery from inactivation)is shown for each cell. Changes in repriming are described indetail in the text and in Figure 8.
[View Larger Version of this Image (27K GIF file)]

Table 1. Effect of axotomy on sodium current kinetics

Cell type^a Current type (% of total)
Number of cells

Fast Mixed Slow

Control 15 39 46 113

Axotomized

    PDA2 32 48 20 40

    PDA6 71 29 0 31

    PDA22 73 21 6 33

    PDA60 50 35 15 54

^a Cells were categorized as displaying fast current if fast current constituted >70% of the total current and were categorizedas displaying slow current if slow current constituted >70% oftotal current. Numbers are percentages of DRG neurons.

As has been shown by others, in control neurons the fast-inactivating current was sensitive to nanomolar concentrations ofTTX, but the slow-inactivating current was resistant (Fig. 2A,B).The relative TTX sensitivity of the fast and slow currents alsowas measured at DPA22 (n = 7) and DPA60 (n = 5) by using 100 nMTTX (Fig. 2C-F). For all cells in both groups the fast currentwas always sensitive and the slow current insensitive to TTX.As has been done in previous studies on DRG sodium currents (Royand Narahashi, 1992; Elliott and Elliott, 1993; Jeftinija, 1994),we will refer to the fast-inactivating TTX-sensitive currentsas the TTX-S component and the slow-inactivating TTX-resistantcurrents as the TTX-R component, although we did not always testthe TTX sensitivity.
Fig. 2. Tetrodotoxin (TTX) sensitivity of fast-inactivating and slowly inactivating currents in control neurons and neurons afteraxotomy. Representative current traces are shown for a controlneuron (A, B) and neurons at DPA22 (C, D) and DPA60 (E, F). C-typeneurons were held at $-$ 100 mV and stepped to 0 mV for 50 msec.Current traces are shown before (solid trace) and after (dashedtrace) 100 nM TTX (A, C, E). The TTX-S component, obtained byusing digital subtraction of the traces in A, C, and E, is shownin B, D, and F. The slow component is TTX-resistant, and the fastcomponent is TTX-sensitive in all three groups.
[View Larger Version of this Image (15K GIF file)]

For the majority of experiments, prepulse inactivation was used to separate the TTX-R and TTX-S current components (McLeanet al., 1988; Roy and Narahashi, 1992). Prepulse inactivationtakes advantage of the differences in the inactivation propertiesof the TTX-S and TTX-R currents and is simpler than TTX subtraction.TTX subtraction and prepulse inactivation give essentially thesame results (Fig. 3).
Fig. 3. Separation of TTX-S and TTX-R currents. Current traces were recorded from a control neuron before (A) and after (B) additionof 100 nM TTX to the bath solution. The currents were elicitedby 20 msec test pulses to $-$ 10 mV after 500 msec prepulses to potentialsover the range of $-$ 130 mV to $-$ 10 mV. C, The TTX-S component wasobtained by digitally subtracting the data in B from A. D, TheTTX-S currents were obtained by subtracting the data in A obtainedwith the $-$ 50 mV prepulse from the data in A obtained with morehyperpolarized prepulses. E, The steady-state inactivation (h $infinity$ )curve for the total current in A is shown ( $bullet$ ). The h $infinity$ curves forthe TTX-S and TTX-R components estimated with either TTX subtraction( $square$ , TTX-R; $triangle$ , TTX-S) or prepulse subtraction ( $black-square$ , TTX-R; $black-triangle$ , TTX-S)also are shown in E. Data were normalized to unity.
[View Larger Version of this Image (18K GIF file)]

Inactivation kinetics and steady-state inactivation
The rate of sodium current inactivation was measured in control neurons and after axotomy. The inactivating phase for boththe TTX-S and TTX-R component was well fit with a single decayingexponential. In control neurons the time constant for fast inactivation(test potential = 0 mV), using the prepulse inactivation protocol,was estimated to be 10-fold slower for the TTX-R current thanfor the TTX-S current (Table 2). Similar values were obtainedfor the TTX-S and TTX-R components, respectively, in DRG neuronsafter axotomy (Table 2). However, because DRG neurons expressedpredominantly the TTX-S current after axotomy, the total currentinactivated faster in these neurons than in control neurons (seeFig. 1).

Table 2. Inactivation of Na⁺ currents in C-type neurons

Inactivation

TTX-R
TTX-S

k (mV/efold) V_h (mV) $tau$ h (at 0 mV) (msec) k (mV/efold) V_h (mV) $tau$ h (at 0 mV) (msec)

Control (29) 7.5 ± 2.4 $-$ 30.9 ± 8.6 4.7 ± 1.9 6.4 ± 1.3 $-$ 69.3 ± 6.6 0.48 ± 0.14

Axotomized

    DPA2 (11) 8.7 ± 2.7 $-$ 32.7 ± 5.3 4.5 ± 1.4 6.7 ± 1.6 $-$ 68.4 ± 6.3 0.44 ± 0.13

    DPA6 (13) 7.9 ± 2.6 $-$ 30.3 ± 6.8 4.8 ± 0.9 6.1 ± 0.7 $-$ 67.2 ± 4.1 0.55 ± 0.23

    DPA22 (15) 6.4 ± 2.5 $-$ 31.3 ± 6.7 4.7 ± 1.3 6.9 ± 1.3 $-$ 66.6 ± 6.9 0.46 ± 0.12

    DPA60 (15) 8.7 ± 2.7 $-$ 32.7 ± 5.3 4.7 ± 1.5 6.5 ± 1.4 $-$ 67.7 ± 5.1 0.53 ± 0.17

Numbers in parentheses indicate number of cells. Data are expressed as mean ± SD.

Similarly, although a striking difference was observed between control neurons and neurons after axotomy in terms of the voltagedependence of steady-state inactivation (see Fig. 1), this differencewas attributable primarily to the downregulation of the TTX-Rcomponent after axotomy. In control neurons the midpoint of steady-stateinactivation (V_h; 500 msec inactivating prepulses) was significantlydifferent for TTX-S currents and TTX-R currents (Table 2, Fig.3). Similar values were observed for the TTX-S and TTX-R currents,respectively, after axotomy (Table 2). Thus the TTX-S and TTX-Rcomponents showed similar voltage dependencies of inactivationin control neurons and neurons after axotomy. It should be noted,however, that interneuronal variation, as previously describedfor small DRG neurons by Rizzo et al. (1994), was observed inthe midpoint of steady-state inactivation for all of the groups.

Sodium current activation
Prepulse inactivation/subtraction was used to separate the TTX-R and TTX-S components. In control neurons the TTX-S componentactivated at potentials ~10 mV more negative than the TTX-R component(Table 3). The midpoints of activation (V_m) estimated with TTX(100 nM) subtraction also showed that the TTX-S component in controlneurons activated ~13 mV more negative than the TTX-R component.

Table 3. Activation of Na⁺ currents in C-type neurons

Activation

TTX-R
TTX-S

k (mV/efold) V_m (mV) k (mV/efold) V_m (mV)

Control 6.4 ± 1.5 $-$ 15.7 ± 2.6 6.4 ± 1.5 $-$ 27.6 ± 4.9

Axotomized

    DPA6 (9) 7.9 ± 1.2 $-$ 16.9 ± 6.9 6.3 ± 1.7 $-$ 21.8 ± 6.6

    DPA22 (14) 6.8 ± 1.9 $-$ 16.2 ± 4.0 4.8 ± 1.8 $-$ 24.6 ± 5.5

Numbers in parentheses indicate number of cells. Data are expressed as mean ± SD.

We measured the voltage dependence of activation for the TTX-S current after axotomy at DPA6 and DPA22 (Table 3). The V_mfor the TTX-S currents from these neurons after axotomy was within6 mV of the V_m for the TTX-S currents from control neurons. Similarly,the V_m for the TTX-R currents after axotomy was very close tothe V_m for the TTX-R currents from control neurons. In all ofthe groups, cell-to-cell variability, as originally reported byRizzo et al. (1995), was observed for the voltage dependence ofactivation for TTX-R and TTX-S currents. It should be noted thatprecise measurements of activation in C-type DRG neurons are difficultbecause they have a high sodium current density. We used low-resistancepatch pipettes and 70-80% series resistance compensation to minimizevoltage errors. Our data on the voltage dependence of TTX-R andTTX-S current activation are similar to those reported by others(Roy and Narahashi, 1992; Elliott and Elliott, 1993; Ogata andTatebayashi, 1993).

The TTX-R current is downregulated after axotomy
To quantitate the amount of TTX-R and TTX-S currents expressed in each cell, we used prepulse inactivation (McLean et al.,1988; Roy and Narahashi, 1992) to separate the TTX-S and TTX-Rcurrent components (Fig. 3). The estimates of the TTX-S and TTX-Rcurrent amplitudes obtained with prepulse inactivation were nearlyidentical to estimates obtained by using TTX subtraction fromcontrol and axotomized neurons (Table 4).

Table 4. Current amplitude: comparison of prepulse inactivation and TTX subtraction

TTX-R
TTX-S
n

Prepulse inactivation TTX subtraction Prepulse inactivation TTX subtraction

Control 24.7 nA 22.1 nA 26.8 nA 28.7 nA 11

±3.5 ±3.0 ±4.7 ±4.8

DPA22 4.5 nA 4.0 nA 29.1 nA 29.8 nA 7

±1.8 ±1.4 ±3.4 ±3.9

DPA60 15.1 nA 15.1 nA 21.1 nA 22.7 nA

±4.8 ±5.0 ±2.8 ±3.3 5

Data are expressed as mean ± SEM.

The TTX-R current amplitude and current density (amplitude normalized to cell capacitance) were significantly lower than controlat all postaxotomy time points (Fig. 4A). The lowest TTX-R currentdensity (22% of control density) was observed at DPA6, with agradual increase at DPA22 and DPA60, when it reached 46% of controllevels. Surprisingly, axotomy had little effect on the currentdensity of the TTX-S component (Fig. 4B). Cell capacitance, whichprovides an electrical estimate of surface area, essentially wasunaffected by axotomy (Fig. 4C).
Fig. 4. Axotomy decreases TTX-R current density. The TTX-S and TTX-R current densities were estimated in control (n = 113), DPA2 (n= 40), DPA6 (n = 30), DPA22 (n = 33), and DPA60 (n = 47) C-typeneurons by using prepulse inactivation (500 msec prepulses) anda 0 mV test pulse. The TTX-R (A) and TTX-S (B) current densitieswere obtained by dividing the estimated peak current by the whole-cellcapacitance. The TTX-R current density was significantly lowerfor the axotomized neurons at each time point (A). The TTX-S currentdensity was not affected significantly by axotomy (B). Axotomyalso did not alter cell capacitance significantly (C). Error barsindicate mean ± SD.
[View Larger Version of this Image (14K GIF file)]

Under the conditions used in this study, both TTX-S and TTX-R currents were detected in most (95%) of the control neurons.Only 5 of 113 control cells expressed the TTX-S component alone,and only one expressed the TTX-R component in isolation. The ratioof the TTX-R amplitude to the TTX-S amplitude was 1.1 ± 0.8 (mean± SD, n = 113) in control neurons. By contrast, the ratio of theTTX-R amplitude to TTX-S amplitude fell to 0.65 ± 0.09 (n = 40),0.22 ± 0.05 (n = 31), 0.27 ± 0.06 (n = 33), and 0.45 ± 0.06 (n= 54) in neurons after axotomy at DPA2, DPA6, DPA22, and DPA60,respectively.

These patch-clamp data may be compared with the results of our previous study, which examined the expression of SNS and IIImRNAs in DRG neurons after axotomy (Dib-Hajj et al., 1996). Inthat study the level of SNS mRNA expression in small DRG neuronswas scored as undetectable, marginal/low, moderate, or high afternonisotopic in situ hybridization (ISH). The ISH data are shownin Figure 5A. To compare the ISH results with changes in TTX-Rcurrent expression, we classified small DRG neurons as havinga TTX-R/TTX-S current ratio of <0.1, 0.1-0.5, 0.5-1.0, or >1.0(Fig. 5B) or as having a TTX-R current density of <100, 100-200,200-500, or >500 pA/pF (Fig. 5C). The patterns for SNS mRNA expression(Fig. 5A) and TTX-R current levels (Fig. 5B,C) in control neuronsare similar; that is, a large percentage of the cells expressmoderate or high levels of SNS mRNA and also have >200 pA/pF TTX-Rcurrent. Conversely, at DPA5 a high percentage of the DRG neuronshave undetectable or low/moderate levels of SNS hybridizationsignal and at DPA6 a vast majority of DRG neurons show <200 pA/pFTTX-R current. At DPA60, on the other hand, approximately one-halfof the cells expressed moderate to high levels of TTX-R current,which is consistent with an observed partial recovery of SNS mRNAlevels at DPA58 (Dib-Hajj et al., 1996).
Fig. 5. Axotomy has a similar effect on SNS mRNA expression and on TTX-R current expression. A, The relative magnitude of SNS expressionwas measured in cultured control and DPA5 C-type neurons by insitu hybridization (Dib-Hajj et al., 1996). Expression was classifiedas either undetectable, marginal/low, moderate, or high. B, Theratio of the TTX-R current density to TTX-S current density isshown for control and axotomized neurons at DPA2, DPA6, DPA22,and DPA60. Cells were classified according to the ratio. C, Shownis the TTX-R current density for control and axotomized neuronsat DPA2, DPA6, DPA22, and DPA60. Cells were assigned to one offour groups for each time point on the basis of TTX-R currentdensity.
[View Larger Version of this Image (25K GIF file)]

The TTX-R current is downregulated in labeled axotomized cells
Although the majority of cells at DPA6 and DPA22 exhibited predominantly TTX-S current (Table 1), five cells at DPA6 andsix cells at DPA22 had a relatively high TTX-R current density(>500 pA/pF). It has been estimated that only 70% of L4-L5 neuronsare axotomized when the sciatic nerve is transected at the midthighlevel (Yip et al., 1984; Devor et al., 1985), and therefore thecells that expressed high densities of TTX-R current might beDRG neurons with axons that were not transected. To confirm thatthe TTX-R current was downregulated in axotomized cells, we didadditional experiments in which axotomized neurons were identifiedunequivocally by selectively labeling with a fluorescent indicator(see Materials and Methods). Neurons were cultured at days 6 and22 (DPA6 and DPA22). In these experiments all of the labeled cellsexpressed predominantly TTX-S currents. None of the labeled cellsexpressed >500 pA/pF of TTX-R current at either DPA6 (n = 16)or DPA22 (n = 14). The TTX-R to TTX-S ratio in labeled cells was0.17 ± 0.04 (n = 16) at DPA6 and 0.15 ± 0.06 (n = 14) at DPA22.This clearly demonstrates that the TTX-R current is downregulatedin axotomized C-type neurons.

Persistent currents are decreased after axotomy
Persistent currents (defined as the current remaining at the end of a 40 msec test depolarization) often were observed insmall C-type neurons. Figure 6 shows persistent current expressedas a fraction of the peak current for control neurons and Fluoro-gold-labeledDPA6 and DPA22 axotomized neurons. Persistent currents in controlneurons were large, often >10% of the peak current (Fig. 6A,B).Even when measured at the end of a 200 msec test pulse, the persistentcurrent still averaged almost 10% of the peak current in controlneurons (Fig. 6A). In contrast, persistent currents after axotomywere small, typically <2% of the peak current (Fig. 6B). We believethat the large persistent currents in control neurons were generatedby TTX-R channels because (1) the persistent currents in controlneurons were not sensitive to nanomolar concentrations of TTX,and large persistent currents were not observed in control neuronsthat expressed primarily TTX-S current (Fig. 6C); and (2) thepersistent currents occurred in a fairly narrow, negative voltageregion, where TTX-R window currents, resulting from overlap betweensteady-state activation and inactivation processes, might occur.On the other hand, the voltage dependence is also consistent withwhat has been reported for low-voltage-activated T-type calciumcurrents in newborn DRG neurons (Ogata and Tatebayashi, 1992).We do not believe that these persistent currents are calcium currentsbecause (1) our bath solution contains 100 µM Cd²⁺ and our pipette solution contained fluoride, which should blockcalcium currents; and (2) in a previous study we were unable todetect low-voltage-activated calcium currents in small adult DRGneurons (Caffrey et al., 1992).
Fig. 6. Axotomy decreases persistent currents in C-type neurons. A, Family of currents recorded from a control small DRG neuron. Currentwas elicited by test potentials from $-$ 75 to $-$ 25 in 10 mV steps.The peak current in this cell was 47 nA. B, Current-voltage relationshipfor the persistent current in small DRG neurons. Cells were heldat $-$ 100 mV and stepped to step voltages from $-$ 80 to 40 mV for40 msec. The average current measured from 38 to 40 msec was normalizedto the maximum peak current for each cell and is plotted againstthe test voltage. Data are shown for control ( $black-triangle$ , n = 12), DPA6( $bullet$ , n = 14), and DPA22 ( $black-square$ , n = 14). Axotomized cells in the DPA6and DPA22 groups were identified with a fluorescent label. Forthe control neurons the persistent current also was measured byusing 200 msec test depolarizations ( $triangle$ , n = 11). C, The persistentcurrent in control neurons (n = 4) that express both TTX-S andTTX-R currents is shown before ( $black-triangle$ ) and after ( $triangle$ ) 100 nM TTX. Incontrol neurons that express only TTX-S currents (n = 5), thepersistent currents were small ( $square$ ). Persistent currents were measuredat 38-40 msec, as in A.
[View Larger Version of this Image (16K GIF file)]

Axotomy upregulates a TTX-S current with rapid recovery from inactivation
Elliott and Elliott (1993) reported that in uninjured DRG neurons the TTX-R current recovered rapidly from inactivation andthe TTX-S current recovered very slowly. We studied reprimingin both control and axotomized small DRG neurons (Fig. 1, rightcolumn). We observed repriming kinetics similar to those reportedby Elliott and Elliott (1993) in control neurons. The reprimingkinetics in a typical control neuron are shown in Figure 7, Aand B. The time course was well fit with two exponentials. TTXwas used to confirm that the slowly inactivating, rapidly reprimingcomponent was TTX-insensitive and that the fast-inactivating,slowly repriming component was TTX-sensitive (n = 10; Fig. 7C).In control neurons that expressed both TTX-R and TTX-S currents,the TTX-R current recovered with a time constant of 1.0 ± 0.3msec, and the TTX-S current recovered with a time constant of60.5 ± 29.0 msec (mean ± SD, n = 45; recovery potential set at $-$ 100 mV). In some of the cells a small, ultraslow recovery componentalso was observed ( $tau$ ~150-250 msec).
Fig. 7. Recovery from inactivation has multiple components in control neurons. A, Data from a typical control C-type neuron are shown.The cell was held at $-$ 100 mV, stepped to 0 mV for 20 msec to inactivatechannels, and then brought back to $-$ 100 mV for increasing durationsbefore the test potential of 0 mV. Current traces shown in A correspondto specific time points in the recovery time course shown in B.The time course of recovery exhibited at least two components.The TTX-R component (traces 1 and 2) recovered rapidly, with atime constant of 0.7 msec. The TTX-S component recovered slowly(traces 5-7), with a time constant of 87 msec. C, Data from anothercontrol neuron are shown. The time course of recovery is shownfor the total current ( $bullet$ ) and for the separated TTX-R ( $square$ ) andTTX-S components ( $triangle$ ). The TTX-R time course was obtained in thepresence of 100 nM TTX. The TTX-S time course was obtained bysubtracting the currents recorded with TTX from the data obtainedwithout TTX.
[View Larger Version of this Image (13K GIF file)]

Figure 8A shows the averaged recovery time course for 45 control neurons that displayed both TTX-S and TTX-R currents, withthe rapid and the slow repriming components also shown separatelyfor clarity. For the five control neurons that only expressedTTX-S current, the time constant for recovery from inactivationwas intermediate (13.9 ± 9.9 msec, mean ± SD, n = 5) between therapid and slow time constants described above (data not shown).Only 3 of the 45 cells that expressed both TTX-S and TTX-R currentsexhibited a TTX-S component that recovered with a time coursethat might be considered as intermediate rather than slow.
Fig. 8. The kinetics of recovery from inactivation for TTX-S current, but not for TTX-R current, are different in axotomized neurons.A, The averaged time course of recovery from inactivation fortotal current from control C-type neurons that expressed bothTTX-S and TTX-R currents is shown ( $bullet$ , n = 45). At least two componentscan be distinguished. The time course of the rapid repriming componentfrom control neurons with predominantly TTX-R (>75%) current isplotted separately ( $square$ , n = 11). The time course for the slow component(obtained by digitally subtracting the current recovered after6 msec) in control cells expressing large TTX-S (>1nA/pF) currentsalso is shown ( $triangle$ , n = 12). B, The repriming time course of theTTX-R component in an axotomized neuron (DPA6) is shown ( $square$ ). Forcomparison, the averaged repriming time course of the TTX-R componentsfrom control neurons also is shown (dashed curve). Recovery frominactivation for the TTX-R current does not shift after axotomy.C, The time course of recovery from inactivation for injured DPA6( $open circle$ ) and DPA22 ( $square$ ) C-type neurons that expressed predominantlyTTX-S currents is shown. For comparison, the repriming time coursefor the TTX-S current of control neurons also is shown (dashedcurve). Note the leftward shift in the time course for recoveryfrom inactivation for the TTX-S current after axotomy. D, Theaveraged time course for recovery of the TTX-S current from inactivationin Fluoro-gold-identified axotomized DPA6 and DPA22 neurons (n= 30) is shown ( $open circle$ ). For comparison, the repriming time coursefor the TTX-S current of control neurons also is shown (dashedcurve).
[View Larger Version of this Image (29K GIF file)]

The repriming kinetics were measured in DRG neurons at all time points after axotomy. The TTX-R component recovered rapidlyin all of the cells from rats with ligated nerves. However, inonly 2 of the 30 Fluoro-gold-labeled axotomized neurons was theTTX-R component large enough to measure accurately the reprimingkinetics (Fig. 8B). In both of these cells, the TTX-R time constantfor recovery from inactivation was near 0.9 msec, i.e., it remainedclose to control values.

In contrast, axotomy was followed by the emergence of a distinct TTX-S current, which we term the "rapidly repriming TTX-S"current. The time constant for recovery from inactivation forthe rapidly repriming TTX-S current was shifted to dramaticallyshorter values. In all of the Fluoro-gold-labeled cells the TTX-Scurrent reprimed with an intermediate time course (Fig. 8C,D),with a time constant of 14.3 ± 6.3 msec (mean ± SD, n = 16) measuredat DPA6 and 15.8 ± 5.1 msec (n = 12) at DPA22. This time constantin axotomized neurons is much shorter than the slow recovery timeconstant measured for the TTX-S current in the majority of controlcells that expressed both TTX-R and TTX-S currents.

In recordings from randomly chosen DPA6 neurons from experiments in which Fluoro-gold labeling was not used, the TTX-S currentdominated in 21 of 30 cells, and again the repriming time coursewas well fit with a single intermediate exponential ( $tau$ = 14.9± 7.6 msec). Of the other nine DPA6 neurons in these experiments,six fit the pattern observed in control neurons with rapid ( $tau$ = 1.3 msec) and slow ( $tau$ = 72 msec) repriming kinetics correspondingto TTX-R and TTX-S components, and three had both fast ( $tau$ = 1msec) and intermediate ( $tau$ = 20 msec) kinetics corresponding toTTX-R and TTX-S components. In the DPA22 experiments in rats inwhich Fluoro-gold labeling was not used, the TTX-S component dominatedin 22 of 29 cells, and 21 of these had an intermediate time coursefor repriming (16.2 ± 6.8 msec). In the remaining predominantlyTTX-S cell, repriming had a slow time constant of 58 msec. Forthe seven DPA22 cells in these experiments with TTX-S and TTX-Rcurrents, five had both fast ( $tau$ = 1.0 msec) and slow ( $tau$ = 85 msec)recovery components, and two had fast ( $tau$ = 0.9 msec) and intermediate( $tau$ = 16 msec) recovery components.

At DPA60, repriming kinetics was examined in 48 randomly chosen cells from experiments in which Fluoro-gold labeling was notattempted. Almost one-half of the cells exhibited predominantlyTTX-S current. For these 21 TTX-S cells the time course showedintermediate kinetics ( $tau$ = 17.9 ± 6.6 msec). The other 27 DPA60cells possessed both TTX-S and TTX-R currents. Sixteen of thesecells displayed fast ( $tau$ = 1.3 msec) and slow ( $tau$ = 69 msec) componentsof repriming, six displayed fast ( $tau$ = 1.0 msec) and intermediate( $tau$ = 19 msec) components, and five had multiple components. Therepriming data indicate that axotomy results in the expressionof TTX-S current with different properties, as well as downregulatingthe TTX-R current, and show that these changes persist for atleast 60 d after axotomy.

TTX-S currents in normal and axotomized neurons display lidocaine sensitivity
Previous studies have indicated that lidocaine and other sodium channel inhibitors can block ectopic impulses in injured neuronsat concentrations that are not sufficient to block normal nociception(Yaari and Devor, 1985; Chabal et al., 1989b; Devor et al., 1992).Roy and Narahashi (1992) reported that TTX-R currents were lesssensitive to lidocaine than TTX-S currents (K_D values of 200 µMand 50 µM, respectively). Therefore, we wanted to test the relativesensitivity of TTX-S currents in axotomized neurons. We applied50 µM lidocaine to control and axotomized (labeled DPA8) neurons.Use-dependent lidocaine inhibition was measured by comparing theamplitude of the first and 20th pulse in a 10 Hz pulse train (10msec, 0 mV depolarizations). Although the TTX-S component wasinhibited by 62 ± 22%, the TTX-R component in control neuronswas inhibited by only 11 ± 6% (n = 4). In the labeled DPA8 neuronsthe TTX-S current was inhibited by 53 ± 16% (n = 4). Thus theTTX-S components in both control and injured neurons were significantlymore sensitive to therapeutic concentrations of lidocaine thanthe TTX-R component in control neurons. The sensitivity of theTTX-R current was not measured in DPA8 cells, because they exhibitedonly small TTX-R currents. Because the TTX-S current dominatesin axotomized neurons, the total sodium current in axotomizedneurons is relatively more sensitive to lidocaine than the currentin uninjured neurons (Fig. 9).
Fig. 9. Axotomy increases the relative sensitivity of C-type neurons to frequency-dependent inhibition by lidocaine. Representativetraces from a control (A) and DPA8 (B) neuron are shown. Cellswere exposed to 50 µM lidocaine. After 5 min, the cells were stimulatedwith a 10 Hz train of 20 depolarizations (to 0 mV for 10 msec).The currents elicited by the first (solid trace) and 20th (dashedtrace) depolarizations are shown.
[View Larger Version of this Image (10K GIF file)]

DISCUSSION
We have studied the effects of axotomy on sodium currents in small C-type DRG neurons. Axotomy results in dramatic and complexchanges in the sodium currents expressed in these neurons. Axotomydecreased the amount of slowly inactivating TTX-R current andresulted in increased expression of a distinct fast-inactivating/rapidlyrepriming TTX-S current. These changes were still evident 60 dafter axotomy. The results presented here, in conjunction withour previous studies that examined sodium channel mRNA expressionin axotomized DRG neurons, provide new insights into the molecularpathophysiology of peripheral nerve injury and may have implicationsfor understanding chronic pain syndromes.

Axotomy downregulates TTX-R current and SNS mRNA levels
One striking effect of axotomy was the downregulation of TTX-R current density. It has been proposed that the TTX-R currentis encoded by the SNS transcript (Akopian et al., 1996; Sangameswaranet al., 1996). Our data support this proposal. ISH demonstratedthat ~90% of small neurons express SNS $alpha$ -subunit mRNA (Black etal., 1996). This closely correlates with the observation presentedhere that 101 of 113 control neurons expressed significant levels(>50 pA/pF) of TTX-R current. Furthermore, the effect of axotomyon SNS mRNA levels at DPA5 is similar to the effect on TTX-R currentdensity at DPA6 (Fig. 5). With the use of RT-PCR of the wholeganglion, it has been demonstrated that SNS mRNA partially recoverstoward control levels by 58 d after axotomy (Dib-hajj et al.,1996). In agreement with the recovery of SNS levels at later timespostaxotomy, we observed an increase in TTX-R current densitybetween DPA6 and DPA60.

It has been suggested that axotomy might cause a reversion to an embryonic mode of sodium channel expression (Iwahashi etal., 1994; Waxman et al., 1994). The loss of TTX-R current isconsistent with an embryonic mode of sodium channel expression.Fedulova et al. (1994) reported that only 24% of embryonic (E17)DRG neurons express TTX-R currents and observed a TTX-R currentdensity in E17 cells that was comparable to our results from DPA6and DPA22 axotomized neurons.

Axotomy upregulates rapidly repriming TTX-S current and type III mRNA levels
In contrast to the effect on SNS mRNA levels, axotomy induces expression of type III mRNA in DRG neurons (Waxman et al., 1994).Surprisingly, we did not see a significant change in the TTX-Scurrent density after axotomy. However, the TTX-S current componentsin control and injured neurons displayed significantly differentrates of recovery from inactivation. Axotomized neurons expressa TTX-S current that recovers much faster than in control neurons(Fig. 8). The emergence of a TTX-S current with different reprimingkinetics could result from upregulation of type III channels anddownregulation of a TTX-S channel that is expressed in uninjuredneurons. This axotomy-induced change in repriming kinetics isalso consistent with a reversion to an earlier developmental modeof sodium channel expression (Ogata and Tatebayashi, 1992).

Our data raise the intriguing possibility that different channel isoforms may show important differences in terms of reprimingkinetics. Surprisingly little electrophysiological differencehas been observed to date among the different brain sodium channelisoforms, leading some to ask why so many channel isoforms exist.Differences in repriming kinetics could have important implicationsfor excitability and repetitive firing properties. Changes inrepriming kinetics also could have pathophysiological importance.Indeed, some of the skeletal muscle sodium channel mutations associatedwith hereditary forms of paramyotonia congenita increase the rateof recovery from inactivation (Yang et al., 1994), which can contributeto hyperexcitability of affected skeletal muscle by reducing therefractory period (Chahine et al., 1994).

If the slow- and fast-recovering TTX-S currents are encoded by distinct isoforms, then our results predict that other mRNAsbesides SNS are downregulated by axotomy. If so, what $alpha$ -subunitproduces the TTX-S current in control neurons? We found that allbut 1 of 113 control neurons expressed >50 pA/pF of TTX-S current.Using ISH, Black et al. (1996) found that virtually all smallneurons express an mRNA that hybridized to the hNE-Na probe. Exceptfor the SNS probe, no other transcript was nearly so abundantin uninjured small neurons. Recombinant hNE-Na channels expressedin HEK-293 cells seem to have fast inactivation decay kineticsand are TTX-sensitive (Klugbauer et al., 1995), but the reprimingkinetics have not yet been characterized. Thus, the hNE-Na isotypeis a candidate for encoding the TTX-S current with slow recoveryfrom inactivation.

Physiological implications
We show in Figure 3 that control neurons express approximately the same amount of TTX-S and TTX-R current when held at $-$ 100mV for prolonged periods. However, the resting potential of DRGneurons is reported to be approximately $-$ 60 mV (Caffrey et al.,1992; Jeftinija, 1994). At this potential much of the TTX-S currentin C-type neurons (V_h approximately equal to $-$ 69 mV; see Table2) might be inactivated. Indeed, Rizzo et al. (1994) studiedC-type DRG neurons, using $-$ 60 mV as the holding potential, andobserved virtually no TTX-S currents. This seems to indicate thatcontrol neurons produce high densities of TTX-S channels thatare not available for activation. An alternative explanation isthat small DRG neurons have a bistable resting potential, as hasbeen reported for other types of excitable cells (Gola and Niel,1993; O'Donnell and Grace, 1995). TTX-R persistent currents mightplay a role in setting the resting potential, as demonstratedin optic nerve axons (Stys et al., 1993). Under some circumstancesthe C-type neurons may reside at more negative potentials fromwhich the TTX-S currents are available for activation. However,because the TTX-S current reprimes very slowly in control neurons,the TTX-S currents probably would be involved only in the initialresponse to a given stimulus. After the initial response the TTX-Rcurrents probably dictate the repetitive firing properties.

Our results suggest that the situation in injured neurons is significantly different. In the labeled neurons at DPA6 and DPA22,the predominant sodium current was a TTX-S current with intermediaterepriming kinetics. Downregulation of the TTX-R current shouldresult in relatively rapid inactivation during spike electrogenesis,which would produce narrow action potentials. Axotomy also greatlyreduces the TTX-R persistent currents, which could affect restingpotential and thus might increase the relative amount of TTX-Scurrent that is available for activation. Because the TTX-S currentafter axotomy reprimes relatively rapidly, the injured neuronswould be expected to sustain higher firing frequencies.

Chronic pain
This study, in conjunction with our previous studies on mRNA expression (Dib-Hajj et al., 1996), shows that axotomy causesa decrease in expression of the SNS channel and the TTX-R sodiumcurrent in small spinal sensory neurons. Thus the hyperexcitabilityobserved in these cells after axotomy, which is believed to underliesome chronic pain syndromes, is not attributable to an increasein SNS/TTX-R current expression. On the other hand, our data showthe emergence of a TTX-S current with rapid recovery from inactivationafter axotomy (Fig. 8) and suggest that rapidly repriming TTX-Scurrents contribute to inappropriate firing in C-type neurons.Our results also show that type III mRNA expression is upregulatedafter axotomy (Waxman et al., 1994; Dib-Hajj et al., 1996).

Lidocaine and other sodium channel blockers have been used in the treatment of chronic pain (Boas et al., 1982; Chabal etal., 1989a). An expanding body of evidence suggests that it ispossible pharmacologically to block some types of sodium channelswhile leaving other types unblocked; for example, it is possiblepharmacologically to block the persistent sodium current thatmediates damaging sodium influx in the anoxic optic nerve whileleaving the fast sodium current, which underlies action potentialelectrogenesis, unblocked (Stys et al., 1992). Similarly, somesodium channel blockers inhibit ectopic activity in peripheralnerves at concentrations that do not block nociception (Yaariand Devor, 1985; Burchiel, 1988; Chabal et al., 1989b; Devor etal., 1992). Matzner and Devor (1994) found that high concentrations(3-300 µM) of TTX blocked ectopic impulses in chronically injuredDRG neurons, providing additional evidence that sodium channelsunderlie hyperexcitability after nerve injury, although theirresults did not identify the channel subtype or subtypes involved.Interestingly, the recombinant SNS channel expressed in Xenopusoocytes is only weakly sensitive to lidocaine and phenytoin (Akopianet al., 1996). Consistent with this, Roy and Narahashi (1992)reported that the TTX-R channel is relatively insensitive to lidocaine(K_D ~0.2 mM), and we have confirmed that result. Our data (Fig.9), on the other hand, show that the predominant TTX-S currentin axotomized neurons is sensitive to lidocaine.

Our data on sodium current (this study) and mRNA expression levels (Waxman et al., 1994; Dib-Hajj et al., 1996) indicate thataltered expression of TTX-S sodium channel isoforms, in additionto or rather than an alteration in SNS and TTX-R currents, playsa predominant role in generating hyperexcitability, which underliespain after injury to DRG neurons. Moreover, our results demonstratethat the TTX-S sodium channel that is expressed in spinal sensoryneurons after axotomy exhibits rapid recovery from inactivationand suggest that this rapid repriming predisposes these cellsto abnormal firing, which underlies chronic pain. Drugs targetedat the sodium channel isoforms producing rapidly repriming currents(possibly type III isoform) therefore may be appropriate for thetreatment of some types of chronic pain.

FOOTNOTES

Received Dec. 11, 1996; revised March 3, 1997; accepted March 5, 1997.

This work was supported in part by the Medical Research Service, Department of Veterans Affairs. T.R.C. was supported in partby a fellowship from the Eastern Paralyzed Veterans Associationand by a grant from the Paralyzed Veterans of America Spinal CordResearch Foundation. We thank Drs. Joel Black, Sulayman Dib-Hajj,and Marco Rizzo for helpful discussions.

Correspondence should be addressed to Dr. Stephen G. Waxman, Department of Neurology, LCI 707, Yale University School of Medicine,333 Cedar Street, P.O. Box 3333, New Haven, CT 06510.

REFERENCES

Akopian AN, Sivilotti L, Wood JN (1996) A tetrodotoxin-resistant voltage-gated sodium channel expressed by sensory neurons. Science 379:257-262.
Appelgren L, Janson M, Nitescu P, Curelaru I (1996) Continuous intracisternal and high cervical intrathecal bupivacaine analgesia in refractory head and neck pain. Anesthesiology 84:256-272[ISI][Medline].
Black JA, Dib-Hajj S, McNabola K, Jeste S, Rizzo MA, Kocsis JD, Waxman SG (1996) Spinal sensory neurons express multiple sodium channel $alpha$ -subunit mRNAs. Mol Brain Res 43:117-132[Medline].
Boas RA, Covino BG, Shahnarian A (1982) Analgesic responses to i.v. lignocaine. Br J Anaesth 54:501-505[Abstract/Free Full Text].
Burchiel KJ (1988) Carbamazepine inhibits spontaneous activity in experimental neuromas. Exp Neurol 102:249-253[ISI][Medline].
Caffrey JM, Eng DL, Black JA, Waxman SG, Kocsis JD (1992) Three types of sodium channels in adult rat dorsal root ganglion neurons. Brain Res 592:283-297[ISI][Medline].
Chabal C, Jacobson L, Russell LC, Burchiel KJ (1989a) Pain responses to perineuronal injection of normal saline, gallamine, and lidocaine in humans. Pain 36:321-325[ISI][Medline].
Chabal C, Russell LC, Burchiel KJ (1989b) The effect of intravenous lidocaine, tocainide, and mexiletine on spontaneously active fibers originating in rat sciatic neuromas. Pain 38:333-338[ISI][Medline].
Chabal C, Jacobson L, Mariano A, Chaney E, Britell CW (1992) The use of oral mexiletine for the treatment of pain after peripheral nerve injury. Anesthesiology 76:513-517[ISI][Medline].
Chahine M, George AL, Zhou M, Ji S, Sun W, Barchi RL, Horn R (1994) Sodium channel mutations in paramyotonia congenita uncouple inactivation from activation. Neuron 12:281-294[ISI][Medline].
Devor M, Govrin-Lippmann R, Frank H, Raber P (1985) Proliferation of primary sensory neurons in adult rat dorsal root ganglion and the kinetics of retrograde cell loss after sciatic nerve section. Somatosens Res 3:139-167[ISI][Medline].
Devor M, Wall PD, Catalan N (1992) Systemic lidocaine silences ectopic neuroma and DRG discharge without blocking nerve conduction. Pain 48:261-268[ISI][Medline].
Dib-Hajj SD, Black JA, Felts P, Waxman SG (1996) Down-regulation of transcripts for Na channel $alpha$ -SNS in spinal sensory neurons following axotomy. Proc Natl Acad Sci USA 93:14950-14954[Abstract/Free Full Text].
Elliott AA, Elliott JR (1993) Characterization of TTX-sensitive and TTX-resistant sodium currents in small cells from adult rat dorsal root ganglia. J Physiol (Lond) 463:39-56[Abstract/Free Full Text].
Fedulova SA, Kostyuk PG, Veselovsky NS (1994) Comparative analysis of ionic currents in the somatic membrane of embryonic and newborn rat sensory neurons. Neuroscience 58:341-346[ISI][Medline].
Galer BS, Miller KV, Rowbatham MC (1993) Response to intravenous lidocaine infusion differs based on clinical diagnosis and site of nervous system injury. Neurology 43:1233-1235[Abstract/Free Full Text].
Gola M, Niel JP (1993) Electrical and integrative properties of rabbit sympathetic neurones re-evaluated by patch clamping non-dissociated cells. J Physiol (Lond) 460:327-349[Abstract/Free Full Text].
Iwahashi Y, Furuyama T, Inagaki S, Morita Y, Takagi H (1994) Distinct regulation of sodium channel types I, II, and III following nerve transection. Mol Brain Res 22:341-345[Medline].
Jeftinija S (1994) The role of tetrodotoxin-resistant sodium channels of small primary afferent fibers. Brain Res 639:125-134[ISI][Medline].
Klugbauer N, Lacinova L, Flockerzi V, Hofmann F (1995) Structure and functional expression of a new member of the tetrodotoxin-sensitive voltage-activated sodium channel family from human neuroendocrine cells. EMBO J 14:1084-1090[ISI][Medline].
Knutsdottir S (1993) Spinal cord injuries in Iceland, 1973-1989. A follow-up study. Paraplegia 31:68-72[ISI][Medline].
Kostyuk PG, Veselovsky NS, Tsyndrenko AY (1981) Ionic currents in the somatic membrane of rat dorsal root ganglion neurons. I. Sodium currents. Neuroscience 6:2423-2430[ISI][Medline].
Levi R, Hultling C, Nash MS, Seiger A (1995) The Stockholm spinal cord injury study. I. Medical problems in a regional SCI population. Paraplegia 33:308-315[ISI][Medline].
Lisney SJW, Devor M (1987) Afterdischarge and interactions among fibers in damaged peripheral nerve in the rat. Brain Res 415:122-136[ISI][Medline].
Matzner O, Devor M (1992) Na⁺ conductance and the threshold for repetitive neuronal firing. Brain Res 597:92-98[ISI][Medline].
Matzner O, Devor M (1994) Hyperexcitability at sites of nerve injury depends on voltage-sensitive Na⁺ channels. J Neurophysiol 72:349-359[Abstract/Free Full Text].
McLean MJ, Bennett PB, Thomas RM (1988) Subtypes of dorsal root ganglion neurons based on different inward currents as measured by whole-cell voltage clamp. Mol Cell Biochem 80:95-107[ISI][Medline].
Nordin M, Nystrom B, Wallin U, Hagbarth KE (1984) Ectopic sensory discharges and paresthesiae in patients with disorders of peripheral nerves, dorsal roots, and dorsal columns. Pain 20:231-245[ISI][Medline].
Nystrom B, Hagbarth KE (1981) Microelectrode recordings from transected nerves in amputees with phantom limb pain. Neurosci Lett 27:211-216[ISI][Medline].
O'Donnell P, Grace AA (1995) Synaptic interactions among excitatory afferents to nucleus accumbens neurons: hippocampal gating of prefrontal cortical input. J Neurosci 15:3622-3639[Abstract].
Ogata N, Tatebayashi H (1992) Comparison of two types of Na⁺ currents with low-voltage-activated T-type Ca²⁺ current in newborn rat dorsal root ganglia. Pflügers Arch 420:590-594[ISI][Medline].
Ogata N, Tatebayashi H (1993) Kinetic analysis of two types of Na⁺ channels in rat dorsal root ganglia. J Physiol (Lond) 466:9-37[Abstract/Free Full Text].
Rizzo MA, Kocsis JD, Waxman SG (1994) Slow sodium conductances of dorsal root ganglion neurons: intraneuronal homogeneity and interneuronal heterogeneity. J Neurophysiol 72:2796-2815[Abstract/Free Full Text].
Rizzo MA, Kocsis JD, Waxman SG (1995) Selective loss of slow and enhancement of fast Na⁺ currents in cutaneous afferent dorsal root ganglion neurons following axotomy. Neurobiol Dis 2:87-96.[ISI][Medline]
Rizzo MA, Kocsis JD, Waxman SG (1996) Mechanisms of paraesthesiae, dysaethesiae, and hyperaesthesiae: role of Na channel heterogeneity. Eur Neurol 36:3-12[ISI][Medline].
Roy ML, Narahashi T (1992) Differential properties of tetrodotoxin-sensitive and tetrodotoxin-resistant sodium channels in rat dorsal root ganglion neurons. J Neurosci 12:2104-2111[Abstract].
Sangameswaran L, Delgado SG, Fish LM, Koch BD, Jakeman LB, Stewart GR, Sze P, Hunter JC, Eglen RM, Herman RC (1996) Structure and function of a novel voltage-gated tetrodotoxin-resistant sodium channel specific to sensory neurons. J Biol Chem 271:5953-5956[Abstract/Free Full Text].
Schmued LC, Fallon JH (1986) Fluoro-gold: a new fluorescent retrograde axonal tracer with numerous unique properties. Brain Res 377:147-154[ISI][Medline].
Study RE, Kral MG (1996) Spontaneous action potential activity in isolated dorsal root ganglion neurons from rats with a painful neuropathy. Pain 65:235-249[ISI][Medline].
Stys PK, Ransom BR, Waxman SG (1992) Tertiary and quaternary local anesthetics protect CNS white matter from anoxic injury at concentrations that do not block excitability. J Neurophysiol 67:236-240[Abstract/Free Full Text].
Stys PK, Sontheimer H, Ransom BR, Waxman SG (1993) Noninactivating, tetrodotoxin-sensitive Na⁺ conductance in rat optic nerve axons. Proc Natl Acad Sci USA 90:6976-6980[Abstract/Free Full Text].
Subbarao JV, Klopfstein J, Turpin R (1995) Prevalence and impact of wrist and shoulder pain in patients w

Volume 17, Number 10, Issue of May 15, 1997 pp. 3503-3514 Copyright ©1997 Society for Neuroscience

Downregulation of Tetrodotoxin-Resistant Sodium Currents and Upregulation of a Rapidly Repriming Tetrodotoxin-Sensitive Sodium Current in Small Spinal Sensory Neurons after Nerve Injury

Volume 17, Number 10, Issue of May 15, 1997 pp. 3503-3514
Copyright ©1997 Society for Neuroscience