Spinal Cats on the Treadmill: Changes in Load Pathways

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The Journal of Neuroscience, April 1, 2003, 23(7):2789

Spinal Cats on the Treadmill: Changes in Load Pathways
Marie-Pascale Côté, Ariane Ménard, and Jean-Pierre Gossard
Centre de Recherche en Sciences Neurologiques, Département de Physiologie, Faculté de Médecine, Université de Montréal, Montréal, Québec, Canada H3C 3J7

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Treadmill training and clonidine, an $alpha$ -2 noradrenergic agonist, have been shown to improve locomotion after spinal cord injury.We speculate that transmission in load pathways, which are involvedin body support during stance, is specifically modified by training.This was evaluated by comparing two groups of spinal cats; onegroup (n = 11) was trained to walk until full-weight-bearing (3-4weeks), and the other (shams; n = 7) was not. During an acuteexperiment, changes in group I pathways, monosynaptic excitation,disynaptic inhibition, and polysynaptic excitation were investigatedby measuring the response amplitude in extensor motoneurons beforeand after clonidine injection. Monosynaptic excitation was notmodified by clonidine but was decreased significantly by training.Disynaptic inhibition was significantly decreased by clonidinein both groups, but more significantly in trained cats, and significantlyreduced by training after clonidine. Also, clonidine could reversegroup IB inhibition into polysynaptic excitation in both groupsbut more frequently in trained cats. We also investigated whetherfictive stepping revealed additional changes. In trained cats,the phase-dependent modulation of all three responses was similarto patterns reported previously, but in shams, modulation of monosynapticand polysynaptic responses was not. Overall, training appearsto decrease monosynaptic excitation and enhance the effects ofclonidine in the reduction of disynaptic inhibition and reversalto polysynaptic excitation. Because it is believed that polysynapticexcitatory group I pathways transmit locomotor drive to extensormotoneurons, we suggest that the latter changes would facilitatethe recruitment of extensor muscles for recovering weight-bearingduringstepping.

Key words: locomotion; weight-bearing; treadmill training; reflex pathways; spinalization; motor control

  Introduction

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Treadmill training has been shown to successfully enhance and maximize residual locomotor capacities of spinal cord injured(SCI) patients (Fung et al., 1990; Wernig et al., 1995; Harkemaet al., 1997; Harkema, 2001). Previous studies first demonstratedthis beneficial effect in adult spinal cats that have a remarkablecapacity to recover locomotion (Lovely et al., 1986; Barbeau andRossignol, 1987; Bélanger et al., 1996; De Leon et al., 1998).Moreover, clonidine, an $alpha$ -2 noradrenergic agonist, improves andaccelerates the recovery of stepping early after spinalizationin cats (Forssberg and Grillner, 1973; Barbeau and Rossignol,1991; Chau et al., 1998) and, when combined with treadmill training,improves walking patterns in SCI humans (Fung et al., 1990; Rémy-Nériset al., 1999).

The repeated sensory stimulation provided during treadmill training is the only source of input that the transected spinalcord can use to trigger recovery and underlying plastic changes(De Leon et al., 1999). But which sensory input is most importantfor recovery? It has been shown in many species, including humans(Prochazka, 1996; Duysens et al., 2000), that sensory feedbackfrom load receptors in the legs has a particularly powerful effecton the activity of the central pattern generator (CPG) for locomotion.Of particular interest is the reflex reversal occurring when IBinhibition (negative feedback) in extensors is replaced by excitation(positive feedback), reinforcing weight support during the stancephase of stepping (Gossard et al., 1994; Prochazka, 1996). Thisreversal is state dependent [i.e., it occurs only when the spinalcord is generating locomotion (Gossard and Hultborn, 1991; Stephensand Yang, 1996) or after injection of L-Dopa (Gossard et al.,1994) or clonidine (McCrea et al., 1995)]. Here, we hypothesizethat transmission of group I (IA plus IB) pathways is specificallymodified by training to assist extensors during stance. We testedthis by comparing two groups of cats transected at T13; one groupwas trained on a treadmill until "full-weight-bearing" (3-4 weeks),and the other was spinalized but not trained. Synaptic transmissionwas evaluated during an acute experiment using intracellular recordingsof motoneurons before and after clonidine injection. We foundthat treadmill training did induce plastic changes in the transmissionof group I pathways from extensors that could be helpful for recoveringweight-bearing duringstance.

  Materials and Methods

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

All procedures were conducted according to the Guide for Care and Use of Experimental Animals of Canada using protocols approvedby the Ethics Committee of Université de Montréal.

Spinalization and locomotor training. Eighteen adult female cats (2.5-4.1 kg) were used for this study. After administrationof preoperative medication, the cats were anesthetized (isoflurane,2%; Abbott Labs, Montreal, Canada) and spinalized at T13 underaseptic conditions. Protocols for spinalization procedures andsubsequent postoperative care were analogous to those describedpreviously (Chau et al., 1998). A patch of fentanyl (Duragesic,25 µg; Janssen-Ortho, Markham, Canada) was sutured on the backof the cat for continuous and stable delivery of analgesic overa 2 d period. The first group of cats (sham) was only spinalized,whereas the second group (trained) was also trained to walk untilthey could support the weight of their hindquarters (referredto as full-weight-bearing, as in previous reports), which took~1 month (mean, 28 d). Training on the treadmill (0.2-0.4 m/sec)started 2 d after surgery and consisted of one to four daily trainingsessions for periods of 10 min. In early training, hindquarterswere sustained by the experimenter to provide weight support,and perineal stimulation was used to induce and maintain locomotion.The animal gradually became able to support its hindquarters,and perineal stimulation was no longer needed. No drugs were usedto assist the locomotor training. The training was stopped whenthe cat was able to walk continuously on the treadmill for >5min while the experimenter assisted only for lateral stabilityby holding thetail.

Acute experiment. Cats were first anesthetized by inhalation of an oxygenated mixture (50%) of nitrous oxide (50%) and halothane(2-3%; MTC Pharmaceuticals, Cambridge, Canada). Cannulas wereinserted in the right common carotid artery to monitor blood pressureand in the jugular and cephalic veins for administration of pharmacologicalagents or fluids. Cats were then decerebrated and curarized (Pavulon,0.2 mg/kg, 45 min; Sabex, Boucherville, Canada) and artificiallyventilated as detailed previously (Ménard et al., 1999; Leblondet al., 2000).

The following muscle nerves from the left hindlimb were dissected free, cut, and mounted on bipolar silver chloride electrodesfor recording [electroneurogram (ENG)] and stimulation: posteriorbiceps-semitendinosus (PBSt), semimembranosus-anterior biceps(SmAB), lateral gastrocnemius-soleus (LGS), medial gastrocnemius(MG), plantaris (Pl), flexor hallucis longus (FHL) and flexordigitorum longus together, tibialis anterior, extensor digitorumlongus, and the sciatic nerve (uncut). Quadriceps nerves (Quad)were not cut and were inserted in a polymer-cuff electrode. SmABand PBSt nerves from the right hindlimb were also mounted forrecording andstimulation.

Stimulation, recordings, and analysis. The cord dorsum potential (CDP) was recorded with a silver chloride-ball electrodelocated near the dorsal root entrance at the L6-L7 border. Stimulationintensity required to just evoke a deflection in the CDP determinedthe threshold for the most excitable fibers for each nerve (1T). Stimulus intensity will be expressed as a multiple of thethreshold.

Intracellular potentials evoked by the stimulation of group I afferents of extensors [Pl, LGS, MG, sometimes together (gastrocnemii-soleus,GS), Quad; six pulses (p), 1.4-1.8 T, 200-300 Hz] were recordedin identified motoneurons (Leblond et al., 2000) with glass micropipettesfilled with K⁺-acetate (2 M) and N-(2,6-dimethylphenylcarbamoylmethyl) triethylammoniumbromide (100 mM; Alamone Laboratories, Jerusalem, Israel) to preventsodium spikes. The duration of the afterhyperpolarization (AHP)was measured in every cell, from the spike onset to the pointat which the AHP crosses the baseline (Gustafsson and Pinter,1984). Stimulation trains of peripheral nerves were given every0.3, 0.4, or 0.5 sec. The amplitude of EPSPs and IPSPs in motoneuronsevoked by monosynaptic, disynaptic, and/or polysynaptic pathwayswas measured (Fig. 1). A "trial" is the averaged response in onemotoneuron evoked by the stimulation of a given pathway (an afferent-motoneuronpair). Several trials could be studied from the responses of agiven motoneuron. The amplitude of monosynaptic EPSPs was measuredat a latency of 1.4 msec (i.e., just before the onset of possibledisynaptic components) (McCrea et al., 1995; Gosgnach et al.,2000). A train of stimuli evoked either disynaptic inhibitionor polysynaptic excitation depending on the conditions (Gossardet al., 1994). The amplitude of IPSP attributable to IB inhibitionwas measured at the maximal negative deflection in the intracellulartrace in response to the stimulation train, and the amplitudeof EPSP resulting from polysynaptic excitation was measured atthe maximal positive deflection, as illustrated by dotted linesin Figure 1. McCrea et al. (1995) have shown that polysynapticexcitation is not just masking the IB inhibition, but that thelatter completely disappears when there is a reversal. Thus, inour calculation, the finding of an excitation (reversal) was considereda 100% reduction of inhibitory transmission. Conversely, a cellshowing IB inhibition was considered to have zero transmissionin excitatory pathways. We also studied the long-lasting motorresponses to the stimulation of flexor reflex afferents (FRA)from each leg. For this, the PBSt and SmAB nerves of either legwere stimulated together with a train of 50 pulses at 50 T.

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Figure 1. Spinal proprioceptive pathways under study. A schematic representation of three sensory pathways transmitting inputs from muscle group I afferents to extensor motoneurons (Ext Mn) is shown to the left: the monosynaptic (stretch reflex) pathway (from group IA afferents originating in muscle spindles of extensors), the disynaptic inhibitory pathway (from group IB afferents of extensors originating in Golgi-tendon organs plus some group IA fibers), and the polysynaptic excitatory pathway (from group IB and IA afferents of extensors). In the acute spinal cat, this latter pathway shares interneurons with the network generating the excitatory locomotor drive in extensors (box E). Sample records of motoneuronal postsynaptic potentials used for measurements are on the right. a, The amplitude of monosynaptic EPSPs was measured at a latency of 1.4 msec (rising phase in this example; i.e., just before the onset of possible disynaptic components). b, The disynaptic IB inhibition was evoked by a short train of stimuli (6 pulses, 1.4-2.0 T, 200-300 Hz), and the IPSP amplitude was measured at the maximal negative deflection in the intracellular trace. Note that there were often monosynaptic EPSPs (six positive humps) overriding the inhibitory trough (dotted line). c, Polysynaptic excitation was evoked by a similar short train of stimuli, and the amplitude was measured at the maximal positive deflection (dotted line) underlying monosynaptic EPSPs.

All responses were also studied during a period of 2 hr after 500 µg/kg intravenous clonidine injection (Sigma, St. Louis,MO) and during fictive locomotion induced by perineal stimulation.Up to two doses of clonidine were injected in an experiment, anddata were recorded for the next 2 hr. Once clonidine was injected,there was no return to control conditions, and all subsequentrecordings were considered postclonidine data. Bursts of ENG activitieswere used to divide the step cycle into flexion (correspondingto swing) and extension (corresponding to stance) phases. Thelocomotor cycle, defined as the period between the onsets of twosuccessive bursts of ENG activity in extensors, was normalizedto the duration of the averaged cycle. Postsynaptic potentialsevoked during flexion and extension were separated and averagedto study phase-dependentmodulation.

Statistical analysis. Results in figures are expressed as means ± SEM. Statistical analysis was performed to disclose differencesbetween the sham and trained groups, between the averaged responsesin all motoneurons obtained before and after clonidine injection,between rest and fictive locomotion (state-dependent changes),and between flexion and extension phases (phase-dependent changes).The Kolmogorov-Smirnov-Liliefors (KSL) test was used to comparethe shape and location of the distribution of responses with anormal distribution. If KSL confirmed that the sample variablesdid fit a normal distribution, a one-way ANOVA was performed;if not, the Kruskal-Wallis one-way ANOVA on ranks was used. The $chi$ ² test with the Yates correction factor was used to compare theoccurrence of polysynaptic excitation between groups. Significantdifferences are indicated by asterisks (*p < 0.05; **p < 0.01;***p < 0.001).

  Results

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Changes in the transmission of group I pathways from extensors were monitored by measuring the peak amplitude of EPSPs andIPSPs at specific latencies in several extensor motoneurons of11 trained (22 LGSs, 18 MGs, 12 Pls, 14 FHLs, 19 SmAB) and sevennontrained (12 LGSs, 20 MGs, 10 Pls, 9 FHLs, 13 SmAB, 3 Quad)cats. Overall, we measured the responses evoked by 314 afferent-motoneuronpairs (134 in shams, 180 in trained cats) with a mean of 2, 29pairs (range, 1-5) per motoneuron. Although responses varied betweenmotoneurons, similar trends were observed among shams and trainedcats. Data pooled according to motor nuclei or stimulated nervesdid not show significant trends. For this reason, and becausethere is extensive convergence and divergence in the three pathwaysunder study (Jankowska, 1992), we grouped all extensor motoneuronsin the different conditions for additional analysis. In the firstpart, we compared the effects of clonidine in trained and nontrainedcats. In the second part, responses were studied during fictivelocomotion, which occurs in a curarized cat (i.e., without movement-relatedsensory feedback orreafference).

Training and clonidine

The monosynaptic stretch reflex is thought to make a major contribution to the level of EMG activities during stepping (Steinet al., 2000), although this role in humans was questioned previously(Sinkjaer et al., 2000). Clonidine did not affect the amplitudeof monosynaptic EPSP significantly (Fig. 2). When preclonidineand postclonidine values were grouped together, it was found thatthe amplitude of monosynaptic excitation was significantly decreased(by 36%) by training (Fig. 2). Motoneurons, divided in two groupsaccording to their AHP duration, corresponding approximately toslow (>50 msec) and fast (20-50 msec) motor units, were also comparedbefore and after clonidine and between shams and trained cats,but no significant changes were observed.

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Figure 2. Clonidine did not modify monosynaptic excitation. The mean amplitude of monosynaptic EPSPs (109 trials in 73 cells) evoked by the stimulation of knee and ankle extensor group I afferents (Quad, Pl, LGS, MG) was not changed significantly by clonidine injection. If we grouped all values together (preclonidine and postclonidine), there is a significant decrease in the amplitude monosynaptic EPSPs (*p < 0.05) caused by training. Filled bars, Clonidine; gray bars, no drug; open bars, preclonidine and postclonidine.

To evaluate transmission in the IB inhibitory pathways, we measured and compared disynaptic IPSPs in response to a short trainof stimuli (appropriate to recruit interneurons) in group I (IAplus IB) (Jankowska and McCrea, 1983; Jankowska, 1992) afferentsfrom extensors in sham and trained cats. In Figure 3, the troughof IB inhibition was reduced in the extensor motoneurons afterclonidine in both groups of cats (Fig. 3a,b). Overall (Fig. 3c),IB inhibition was decreased by clonidine injection in sham cats(by 30.5%; p < 0.05) and, even more so, in trained cats (by 61.0%;p < 0.001). Training was able to enhance the reduction of IB inhibitionfor responses evoked after clonidine (p < 0.01).

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Figure 3. Training plus clonidine injection decreased disynaptic IB inhibition. a, b, IPSPs evoked by stimulation of GS group I afferents [6 p 1.8 T] in a Pl motoneuron in a sham (a) and Pl group I afferents (6 p 1.8 T) in an LGS motoneuron (similar AHP as the Pl cell) in a trained cat (b) before (gray trace) and after (black trace) clonidine. Clonidine decreased IB inhibition in both groups of cats. Mn, Motoneuron. c, Afferent volley was monitored by the CDP. Overall, disynaptic IPSPs (314 trials in 143 cells) evoked by stimulation of knee and ankle extensor group I afferents (Quad, Pl, LGS, MG, GS) were significantly decreased by clonidine in shams (30.5%; *p < 0.05) and even more significantly in trained cats (61.0%; ***p < 0.001). Training enhanced significantly the reduction of IB inhibition after clonidine (**p < 0.01). d, Plot of EPSP amplitude versus IPSP amplitude measured from the same cell in shams (filled circles) and trained cats (open circles).

Decreases in both monosynaptic excitation and disynaptic inhibition could result from a similar modification in motoneuronalproperties (e.g., a decrease in membrane resistance). In Figure3d, we plotted the amplitude of monosynaptic EPSP against theamplitude of disynaptic IPSP measured from the same cell in shams(filled circles) and trained cats (open circles). If both responseswere to change together, because of the same motoneuronal modification,one would expect the values from shams to be grouped in the topright corner (i.e., large EPSP and large IPSP together) and thevalues from trained cats, which are both significantly reduced,to be grouped in the bottom left corner. The considerable scatteringof points in this graph suggests on the contrary that these twopathways were modifiedindependently.

The reversal of IB inhibition into excitation was first described in acute spinal cats (Gossard and Hultborn, 1991; Gossardet al., 1994; McCrea et al., 1995). In this system, group I afferentsfrom knee and ankle extensors converge on pathways to producethe excitatory drive to extensor muscles during stance. Here,we investigated the occurrence and amplitude of polysynaptic excitationof extensors in chronic spinal cats after clonidine and training.Surprisingly, there were instances of reversals without drugsor locomotion in both sham (8 of 94 trials) and trained (9 of103 trials) cats. This indicates that after 3-4 weeks of spinalization,interneurons in the polysynaptic excitatory pathways recoveredsome level of excitability. As expected, clonidine injection succeededin reversing IB inhibition into excitation in motoneurons fromboth groups of cats, as shown in Figure 4. In shams, the occurrenceof reversals was more frequent (21.5%; p < 0.01) and its amplitudewas greatly increased (from 0.09 to 0.60 mV; 535.6%; p < 0.001)with clonidine. In trained cats, there was a significant increasein amplitude of polysynaptic excitation (from 0.17 to 0.68 mV;307.8%; p < 0.001) and a highly significant increase in occurrence(30.2%; p < 0.001) attributable to clonidine.

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Figure 4. Clonidine increased polysynaptic group I excitation in both groups of cats. a, b, EPSPs evoked by stimulation of LGS afferents [6 p 1.8 T] recorded in MG motoneurons (with similar AHPs) in a sham cat (a) and a trained cat (b) before and after clonidine. Here, clonidine reversed IB inhibition (gray trace) to polysynaptic excitation (black trace) both in sham and trained cats. Mn, Motoneuron. c, Overall, the amplitude of polysynaptic EPSPs (313 trials in 143 cells) evoked by stimulation of knee and ankle extensor group I afferents (Quad, Pl, LGS, MG, GS) was increased by clonidine in sham (535.6%; ***p < 0.001) and in trained (307.8%; ***p < 0.001) cats.

We succeeded in keeping intracellular recordings of four motoneurons while injecting clonidine and had the opportunity toobserve changes in responses. In a sham, a Pl cell showed a decreasein IB inhibition (from $-$ 7.2 to $-$ 4.1 mV), and in another sham,an FHL cell showed a reversal from inhibition to excitation (from $-$ 2.2 to 1.4 mV). In a trained cat, an LGS cell showed a decreasein IB inhibition (from $-$ 1.6 to $-$ 0.8 mV) and, in another trainedcat, an MG cell showed a reversal (from $-$ 2.7 to 1.6 mV). Similarresults were found in the overall population, as reported above.Table 1 gives the mean amplitude of monosynaptic excitation,disynaptic inhibition, and polysynaptic excitation in shams andtrained cats before and after clonidine injection.


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Table 1. The effects of clonidine and training on the mean amplitude of responses in the specified pathway and on occurrence of reversals

The long-lasting reflexes evoked by stimulating FRA after administration of L-Dopa in spinal cats are believed to be partof the locomotor circuitry (Jankowska et al., 1967a,b; Schomburget al., 1998). Moreover, it was shown that group I afferents fromextensors and contralateral FRA (coFRA) converge on common interneuronsto excite extensors after L-Dopa injection (Gossard et al., 1994).The involvement of the FRA pathways in chronic spinal cats hasbeen questioned (Grillner, 1973; Barbeau et al., 1987). In thisstudy, we found that primarily flexors (16 of 18 cats) and notextensors were excited by coFRA stimulation, with or without clonidine.Similar patterns were observed both in sham cats (18 of 24 trials)and trained cats (30 of 38 trials). This strongly suggests thatpathways mediating flexion reflexes are deeply reorganized afterchronicspinalization.

Training and fictive locomotion

Before clonidine injection, rhythmic bursts of ENG activity were scarcely evoked by perineal stimulation (Barbeau and Rossignol,1987; Bélanger et al., 1996) in shams (two of seven cats) (Fig.5a). Surprisingly, training did not increase significantly theoccurrence of fictive locomotor activities (7 of 11 cats) (Fig.5b). After clonidine, perineal stimulation induced robust andwell organized episodes of fictive locomotion in both groups ofcats (Fig. 5c,d). As exemplified by reflex reversals, it is nowwell established that transmission in several sensory pathwaysis deeply modified during locomotion (Rossignol, 1996). We thusinvestigated whether fictive stepping disclosed additional effectsof training on the transmission of group I pathways (state-dependentchanges). We also studied whether training modified the CPG-dependentmodulation in reflex transmission (phase-dependent changes).

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Figure 5. Fictive locomotion can be induced in shams and trained cats. a, b, Motoneuronal intracellular potential and ENG activity in flexor and extensor muscle nerves in a sham (a) and a trained (b) cat. Rhythmic bursts of activity evoked by perineal stimulation before clonidine injection were observed in trained cats (7 of 11) and in shams (2 of 7). c, d, After clonidine, perineal stimulation induced robust locomotor episodes in both groups of cats. Ext Mn, Extensor motoneuron.

The amplitude of monosynaptic EPSPs in motoneurons was reported to be decreased during fictive locomotion (by 34%) inducedby mesencephalic stimulation in decerebrate cats because of atonic level of presynaptic inhibition (Gosgnach et al., 2000).In this study with chronic spinal cats, fictive stepping did notinduce a significant decrease in monosynaptic EPSP amplitude comparedwith rest in both sham (by 31.2%) and trained (by 29.2%) cats.During walking, transmission in the monosynaptic reflex pathwayis phasically modulated in the cat (Forssberg and Grillner, 1973;Akazawa et al., 1982; Gossard, 1996; Ménard et al., 1999) andin humans (Capaday and Stein, 1986; Simonsen and Dyhre-Poulsen,1999), being maximal during stance in extensors when motoneuronalpools are depolarized. Figure 6 illustrates that the phases formaximal amplitude of monosynaptic EPSPs are opposite in a shamand a trained cat. Phase-dependent modulation was found to besignificant only in a few trials (5 of 29 in 4 of 22 cells) (Gosgnachet al., 2000). Among those, it was found that training significantlymodified the pattern of modulation (p < 0.01), the maximum amplitudeoccurring during the depolarized active phase (Fig. 6c). Thisvery limited sample suggests that training may modify the monosynapticIA-transmission pathway to extensor motoneurons so that it ismaximally transmitting during the extensor (stance) phase.

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Figure 6. Training could change the pattern of CPG-related modulation of monosynaptic excitation. a, The amplitude of monosynaptic EPSPs evoked by Pl stimulation [1 p 1.8 T] was larger during the hyperpolarized (Hyp) phase in an LGS motoneuron from a sham cat. b, The amplitude of monosynaptic EPSPs evoked by LGS stimulation (1 p, 1.8 T) was larger during the depolarized (Dep) phase in an MG motoneuron from a trained cat. Mn, Motoneuron. c, Training modified significantly the pattern of phase-dependent modulation of monosynaptic EPSPs (5 trials in 4 cells; **p < 0.01) evoked by group I afferents of ankle extensors (Pl, MG, LGS), with the maximum amplitude occurring during the hyperpolarized phase in sham cats and during the depolarized phase in trained cats.

We also investigated whether fictive stepping disclosed additional effects of training on the transmission of IB inhibitorypathways. It was found that fictive locomotion did not changesignificantly the amplitude of disynaptic IPSPs compared withrest in both sham (48 trials in 27 cells) and trained (35 trialsin 26 cells) cats. We also assessed the phase-dependent modulationin IPSP amplitude. Figure 7 illustrates that the amplitude ofIPSPs was larger during the depolarized phase in motoneurons inboth sham (Fig. 7a) and trained (Fig. 7b) cats. From motoneuronspresenting a significant phasic modulation (40 of 59 trials in33 of 41 cells) between depolarized (active) and hyperpolarizedphases, it was found that the average depth of modulation wasnot significantly changed by training (sham, 28.8%; trained, 29.3%).Analysis also showed that the IPSP reduction was not related tothe amplitude of locomotor depolarization in motoneurons. Thissuggests that the CPG-related modulation that was similar in bothgroups probably occurred in IB interneurons.

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Figure 7. Training did not change the pattern of CPG-related modulation of IB inhibition. a, b, IPSPs evoked by Quad (6 p, 1.8 T) in MG motoneurons during fictive locomotion in a sham (a) and a trained (b) cat. The amplitude of IPSPs (trough) was increased during the depolarized (dep) phase in the sham (black trace) and the trained (gray trace) cat. Mn, Motoneuron. c, The depth of modulation in IPSPs (40 trials in 33 cells) was not significantly changed by training. Hyp, hyperpolarized.

Compared with rest, the occurrence of reversals from IB inhibition to excitation was more frequent during fictive locomotionin shams (25.1%; p < 0.001) but not in trained cats (11.7%; notsignificant). Also, the amplitude of responses was much increasedduring fictive stepping in shams (48 trials, by 225.5%; p < 0.05),whereas it was unchanged in trained cats (36 trials). We alsoassessed its phase-dependent modulation. For example, in Figure8, the amplitude of polysynaptic EPSPs was increased during thedepolarized phase in the motoneuron from a sham (Fig. 8a), whereasit was decreased during that same phase in a motoneuron from atrained cat (Fig. 8b). From motoneurons presenting a significantphasic modulation (19 of 29 trials in 15 of 21 cells), it wasfound that the average depth of modulation was not significantlychanged by training. However, the polysynaptic excitation waslarger (by 8.1%) during the depolarized phase in sham cats, whereasit was decreased (by 19.3%) during that same phase in trainedcats (Fig. 8c). The fact that, in trained cats, the amplitudeof polysynaptic excitation is smaller during fictive steppingcompared with rest and smaller during the depolarized phase maybe attributable to the occlusion of this pathway caused by itsrecruitment by the CPG to produce extensor activities (Gossardand Hultborn, 1991; Gossard et al., 1994). This was evaluatedby comparing in both groups of cats the linear regressions relatingthe amplitude of polysynaptic excitation and the amplitude oflocomotor bursts of activity of the parent extensor nerve. Inshams, the amplitude of polysynaptic excitation was growing withincreasing ENG-burst amplitude (upward slope), whereas in trainedcats, it decreased with increasing ENG bursts (downward slope),and this difference was significant (p < 0.03).

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Figure 8. Different patterns of CPG-related modulation of polysynaptic excitation. a, EPSPs recorded in an MG motoneuron (tilted 90°) in a sham were evoked by Quad stimuli [6 p 1.8 T] at different moments in the step cycle illustrated by the rectified and filtered ENG activity of the LGS nerve. The amplitude of polysynaptic EPSPs was maximal (gray trace) when occurring during the active period of LGS (i.e., during the extension phase). b, The amplitude of polysynaptic EPSPs evoked by Pl stimulation and recorded in an FHL motoneuron (tilted 90°) from a trained cat (6 p, 1.8 T) was minimal (black trace) during the extension phase when LGS was maximally active. Mn, Motoneuron. c, Overall, the pattern of phase-dependent modulation of polysynaptic EPSPs (19 trials in 15 cells) tended to be opposite in shams and trained cats, but this difference was not statistically significant.

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Acute experimentation in curarized animals is advantageous to investigate transmission of sensory pathways because it allowsstable intracellular recordings, and responses can be solely attributedto the operation of central networks. The effects of trainingor clonidine observed in this study can then be attributed tochanges occurring in spinal pathways and not to an alterationin peripheral sensory events or muscle fibers. There is now growingevidence that reflex pathways are not "hard-wired" (Forssbergand Svartengren, 1983), and that they can display a certain levelof plasticity in response to central or peripheral lesions oroperant conditioning (Mendell, 1984; Durkovic, 1996; Wolpaw, 1997;Wolpaw and Tennissen, 2001). The recovery of stepping with treadmilltraining has been attributed solely to plasticity of the CPG (Lovelyet al., 1986; Rossignol, 1996; Harkema, 2001). This study is thefirst to report that recovery of locomotion may also involve changesin several reflex pathways. Plastic changes in a reflex arc canoccur in motoneurons, interneurons, or primary afferents. Ourresults showed that stimulation of the same group I afferentscould elicit opposite response patterns in two different pathways(monosynaptic and polysynaptic), one being increased and the otherdecreased in amplitude, in the same motoneuron. Also, decreasesin monosynaptic and disynaptic responses did not appear to covaryin the same motoneuron. Additionally, clonidine injection significantlymodified transmission in disynaptic pathways without affectingmonosynaptic transmission. Moreover, AHP duration, which variessystematically with input resistance and membrane time constant(Gustafsson and Pinter, 1984), was found not to be modified by1 month of training (data not shown). Therefore, premotoneuronalmechanisms can most easily explain our response patterns. Finally,there is an unknown contribution and plastic modification of recurrentinhibition in our recordings. However, IB inhibition and its reductioncaused by training were observed between motoneurons (e.g., Quad)and group I fibers from muscle nerves (e.g., Pl) known to lackrecurrent inhibitory connections (Baldissera et al., 1981). Wethus believe that plasticity induced by training in load pathwayswas occurring primarily in interneurons of the group I pathwaysto extensors and interneurons of presynapticinhibition.

The first finding of this work is that training decreases monosynaptic excitation by 36%. This was apparent when we pooledall amplitude values because of the lack of significant effectof clonidine on this transmission. In the few cells in which itwas possible to test, the phase-dependent modulation showed amaximum monosynaptic transmission occurring during the extensorphase in trained cats in which it could help the excitation ofmotoneurons. Intrathecal injection of clonidine also failed tochange the H-reflex in incomplete paraplegic subjects (Rémy-Nériset al., 1999). Also, treadmill training decreased and improvedthe gating of IA reflexes in spinal-cord-injured humans comparedwith normal subjects (Trimble et al., 1998). Transmission in thispathway can be changed by presynaptic inhibition and/or motoneuronalproperties. As explained above, postsynaptic changes alone cannoteasily explain all of the response patterns observed in this work.We thus believe that training may have increased the level ofpresynaptic inhibition in IA terminals ending in the ventral horn.Such an increase was inferred to explain a general (non-muscle-specific)tonic decrease in IA-EPSPs (by 34%) in a majority of hindlimbmotoneurons during fictive locomotion evoked by mesencephalicstimulation in the cat (Gosgnach et al., 2000). We thus suggestthat training could help reduce spasticity by decreasing IA transmissionand improve phase-dependent modulation of the stretch reflexesduringstepping.

Another main finding from this work is that the decrease in IB inhibition after clonidine is enhanced by training. A normalizationof inhibitory systems in the spinal cord may be of prime importancein recovering stepping (Robinson and Goldberger, 1986; De Leonet al., 1999). For example, it was recently described that thenumber of cells stained for GAD67 mRNA was specifically decreasedby step training in laminas V and VI (in which IB interneuronsare located) in spinal cats (Tillakaratne et al., 2002). Notethat during reflex reversal, the disappearance of disynaptic inhibitionprecedes the appearance of polysynaptic excitation (Gossard etal., 1994; McCrea et al., 1995). We thus interpret the observedreduction of IB inhibition as a first step toward reversals. Theresults also showed that clonidine increased more significantlythe occurrence of polysynaptic excitation in trained cats thanin shams. However, it was surprising not to see more effects oftraining on the amplitude of polysynaptic excitation. Perhapssmaller doses of clonidine would have revealed more differences.Indeed, the dose used (500 µg/kg) was determined from previousreports on acute spinal cats and is possibly more than sufficientto evoke reflex reversals in all spinalcats.

Fictive locomotion did not reveal additional training-related changes in IB inhibition amplitude or phase-dependent modulationpatterns. However, it showed that the minimal amplitude in polysynapticexcitation occurred during the extensor phase when the locomotorexcitation is maximal in trained cats. We interpret this patternas being attributable to the occlusion of the pathways by theaction of the CPG during the extensor phase as it was proposedin the acute spinal cat (Gossard et al., 1994). We interpret thisas being another step toward the establishment of locomotor-relatedpolysynaptic excitatory pathways to extensors caused by training.The same reasoning may help explain why the occurrence and amplitudeof polysynaptic excitation in shams were increased during fictivestepping. If locomotor circuitry is not as well established inshams as in trained cats, there is less occlusion in these pathwaysand the segmental responses become moreapparent.

In the decerebrate cat walking on a treadmill, it was estimated that up to 50% of the force generated during the stance phasewas caused by muscle reflexes (Hiebert and Pearson, 1999; Steinet al., 2000). We may presume that the isolated spinal cord woulddepend even more on sensory feedback to generate force duringstepping. Although modest, the reported plastic changes indicatethat after spinal cord injury, load pathways would have a largercontribution in the control of stance if trained regularly andtogether with pharmacological intervention. Our results supportprevious reports that load receptors may contribute to the activationof leg extensors during walking in humans (Ghori and Luckwill,1985; Dietz et al., 1992; Stephens and Yang, 1999; Sinkjaer etal., 2000; Stein et al., 2000). For example, it was proposed thatafferent inputs from receptors signaling contact forces duringthe stance phase are essential for the activation of spinal locomotorcenters in SCI subjects (Harkema et al., 1997). Moreover, theimprovement in treadmill and overground locomotor patterns wasattributed to the repetitive alternating-limb loading using body-weightsupport (Wernig et al., 1998). Whether treadmill training or repetitiveloading revived the previous (prespinalization) CPG or whetherit set up a new locomotor circuitry is still debatable. Our resultsindicate clearly that some pathways involved in locomotion inthe acute spinal cat, namely the FRA networks (Jankowska et al.,1967a,b), are reorganized after chronic spinalization (Barbeauet al., 1987). Moreover, fictive stepping sometimes occurred withoutconcomitant appearance of group I polysynaptic excitation in someextensor motoneurons, which was not seen in the acute cat injectedwith L-Dopa (Gossard et al., 1994). Thus, as proposed previously(Hodgson et al., 1994; De Leon et al., 1999), our results supportthe idea that the isolated spinal cord "learned" how to walk byestablishing new locomotorpathways.

  FOOTNOTES

Received May 1, 2002; revised Jan. 15, 2003; accepted Jan. 21, 2003.

This work was supported by the Canadian Institutes of Health Research and the Christopher Reeve Paralysis Foundation. M.-P.C.was supported by the joint Fonds pour la Formation de Chercheurset l'Aide à la Recherche du Québec and Fonds de la Rechercheen Santé du Québec (FCAR-FRSQ). A. M. was supported by the NaturalSciences and Engineering Council of Canada and FCAR-FRSQ. We thankF.-J. Lapointe for assistance in statistical analysis and F. Lebelfor technicalsupport.

Correspondence should be addressed to Dr. Jean-Pierre Gossard, Centre de Recherche en Sciences Neurologiques, Départementde Physiologie, Faculté de Médecine, Université de Montréal,C.P. 6128, Succ. Centre-ville, Montréal, Québec, Canada H3C3J7. E-mail: jean-pierre.gossard{at}umontreal.ca.

  References

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

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