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Previous Article | Next Article
The Journal of Neuroscience, December 15, 1999, 19(24):10966-10976
Proprioceptive Control of Extensor Activity during Fictive Scratching and Weight Support Compared to Fictive Locomotion
Marie-Claude Perreault, Manuel Enriquez-Denton, and Hans Hultborn Department of Medical Physiology, The Panum Institute, University of Copenhagen, DK-2200 Copenhagen, Denmark
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
At rest, extensor group I afferents produce oligosynaptic inhibition of extensor motoneurons. During locomotor activity, however, such inhibition is replaced by oligosynaptic excitation. Oligosynaptic excitation from extensor group I afferents plays a crucial role in the regulation of extensor activity during walking. In this study we investigate the possibility that this mechanism also regulates extensor muscle activity during other motor tasks.
We show that the reflex pathways responsible for extensor group I oligosynaptic excitation during fictive locomotion can be activated during both fictive scratching and fictive weight support (tonic motor activity induced by contralateral scratching). These observations suggest that the excitatory group I oligosynaptic reflex pathways are open for transmission during several forms of motor activities. We also show that extensor group I input during fictive scratching can affect the amplitude and the timing of extensor activity in a pattern similar to that observed during locomotion. Most likely these effects involve the activation of the excitatory group I oligosynaptic reflex pathways. Accordingly, it is suggested that extensor group I oligosynaptic excitation during motor activities other than locomotion is also used to regulate extensor muscle activity. Furthermore, the similarity of effects from extensor group I input on the rhythmicity during scratching and locomotion supports the hypothesis that both rhythms are generated by a common network.
Key words: primary muscle spindles; Golgi tendon organs; spinal cord; sensory feedback; rhythm generating networks; motoneuron; motor control
INTRODUCTION
In the quiescent cat, activation of extensor group I afferents (which include afferents from both muscle spindle primaries and Golgi tendon organs) induces oligosynaptic reflexes in extensor motoneurons that are predominantly inhibitory [autogenic inhibition (Granit 1950
; Eccles et al., 1957
The disynaptic and the polysynaptic group I reflex pathways represent important sources of excitatory feedback during locomotion and provide a means by which extensor muscle activity can be generated, reinforced, and prolonged (Conway et al., 1987
In this study, we investigated the ability of ankle extensor group I afferents to evoke oligosynaptic EPSPs in hindlimb extensor motoneurons during fictive scratching (Deliagina et al., 1975
Some of the present results have been presented in abstract form (Perreault et al., 1997
MATERIALS AND METHODS
Preparation. Data were obtained from 19 cats (1.9-3.5 kg). After anesthesia with halothane-nitrous oxide (2-3% halothane, 70% N2O, and 30% O2), the animals were intubated, and cannulas were inserted in the jugular vein and carotid artery for administration of fluid and drugs and blood pressure monitoring. Atropine (0.1 mg/kg, s.c.) and dexamethasone (1 mg/kg, i.v.) were given at the beginning of the experiment while buffer solution (10% dextrose and 1.7% NaHCO3) was infused continuously (4.5 ml/hr). The following nerves from the left hindlimb were cut and dissected for recording or stimulation: the flexor nerves sartorius (Sart, with both medial and lateral branches) and tibialis anterior (TA), the extensor nerves semimembranosus and anterior biceps (SmAB), medial gastrocnemius (MG), and/or lateral gastrocnemius plus soleus (GS and/or LGS) and plantaris (Pl) and, the bifunctional nerves posterior biceps-semitendinosus (PBSt), quadriceps (Q with the rectus femoris portion), and flexor digitorum and hallucis longus (FDHL). The Q and Sart nerves were placed in cuff electrodes, and the other nerves were mounted on bipolar hook electrodes. From the right limb, GS or Pl and TA or DP (tibialis anterior plus extensor digitorum longus) nerves were mounted. In all experiments, the remaining femoral, sciatic, and obturator nerve branches, and the tendons around the hips, were cut bilaterally. After a laminectomy exposing L4-S1 spinal cord segments, animals were transferred to a rigid frame, and the head was positioned in a stereotaxic apparatus. Then, a second laminectomy exposing C1-C2 segments and a precollicular-postmammillary decerebration (with all brain tissue rostral to the transection removed) were performed. Decrease of the blood pressure to <80 mmHg was counteracted by injection of Dextran. Anesthesia was then discontinued, and the animal was paralyzed with pancuronium bromide (Pavulon; 4 mg · kg
1 · hr
Fictive motor programs. The motor programs studied include fictive scratching (Fig. 1A), fictive weight support (Fig. 1B), and fictive locomotion. Fictive weight support refers to the tonic activity of extensors seen in the hindlimb opposite to that performing scratching (Sherrington, 1910
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Figure 1. Motoneuronal activities during fictive scratching and weight support. Top to bottom, intracellular recording from an SmAB motoneuron (top trace), ENG recordings from the left hindlimb extensor (SmAB), flexor (Sart, TA), and hip extensor/knee flexor (PBSt) nerves (middle four traces) and ENG recordings from the right hindlimb extensor (Pl) and flexor (DP) nerves (bottom two traces). A, Fictive scratching was induced by manual stimulation of the left pinna and monitored with both intracellular recording from an extensor motoneuron in the left spinal cord (insert) and ENG recordings from left hindlimb nerves. Fictive scratching consisted of two periods: (1) an initial approach period during which extensor motoneurons (SmAB) were tonically hyperpolarized and hip, knee, and ankle flexor nerves (Sart, TA) fired tonically, and (2) a rhythmic period during which the bursts of activity in hip (SmAB, PBSt) and ankle extensors (MG, LGS; data not shown) alternated with bursts in hip (Sart) and ankle (TA) flexors. In the right hindlimb, sustained activity was seen in Pl extensor nerve (arrow). B, Fictive weight support was induced by stimulation of the right pinna so it could be monitored with the same intracellular and left hindlimb ENG recordings as in A. The tonic increase in extensor activity during fictive weight support was generally more pronounced in hip (SmAB and PBSt) than in ankle extensors (data not shown). The intracellular record during fictive weight support shows that sustained depolarization of the extensor motoneuron was accompanied by small, cyclic reductions in membrane potential as rhythmic scratching activity appeared in the right hindlimb extensors. In both panels, the vertical bars below the intracellular waveform indicate single shock stimulation to LGS nerve.
Experimental protocols. Independently of the fictive motor program induced, intracellular recordings were obtained from antidromically identified extensor motoneurons innervating the left hindlimb (Fig. 1). Glass micropipettes (tip diameter, 1.2-2 µm; resistance, 2-4 M
) filled with the lidocaine derivative QX-314 in potassium acetate (2 M) were used. QX-314 blocks sodium spikes and may, in addition, reduce calcium currents [Talbot and Sayer (1996)
Postsynaptic potentials were evoked by free-running (3-5 Hz) stimulation of ankle extensor nerves (1-3 pulses at 100-300 Hz). The strength of the peripheral nerve stimulation was expressed as multiple of the threshold (T) for the most excitable afferent fibers to evoke cord dorsum potential (CDP) at the L4 or L7 segment. The central latencies of the PSPs were measured from the arrival of the earliest component of the cord dorsum group I afferent volley (Fig. 2). The effects of group I input on the fictive scratching rhythm were investigated using short (relative to the duration of the extension or flexion phase) trains of stimuli (10-25 pulses at 100-300 Hz) to ankle extensor nerves. These trains were triggered from the onset of activity in one of the flexor (see Fig. 6) or extensor (see Fig. 7) nerves. In some experiments, the stimulation was delivered continuously throughout many cycles (see Fig. 5).
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Figure 2. Ankle extensor group I afferents evoke disynaptic EPSPs not only during fictive locomotion but also during fictive scratching and weight support. The top two traces in A-C are averaged intracellular recordings from an MG motoneuron, showing the group I disynaptic excitatory response (hatched areas) evoked by MG nerve stimulation during fictive locomotion, scratching, and weight support. During locomotion (A) and scratching (B), the superimposed traces are the averages during extension (solid trace) and flexion (dotted trace). In C, superimposed traces are from the averages during weight support (solid trace) and at rest (dotted trace). In all panels, the middle trace is the arithmetic difference between the top two traces. The bottom trace is the cord dorsum potential record of the arrival of the afferent volley (vertical dashed line). Number of trials used in the calculation of the averages and the value of the membrane potential are indicated.
Analysis. Integrated and rectified electroneurograms (ENGs), stimulus markers (from the MLR and the peripheral nerve stimulation), AC (cord dorsum potentials and intracellular records)-, and DC-coupled recordings (intracellular records) were digitized at a rate of 500 Hz, 2, 10, and 5 kHz, respectively. All data were collected and analyzed on a Concurrent 5450 or a personal computer (PC) with software developed by the Winnipeg Spinal Cord Research Center to run under real time Unix (Concurrent) or QNX (PC).
The PSPs evoked by peripheral nerve stimulation were averaged before (control) and during each of the fictive motor programs. During fictive scratching and locomotion, the responses occurring during the flexion or the extension phases were averaged separately. From these averages we excluded the responses evoked during the transition between the two phases. During the initial postural period of scratching (Fig. 1A, approach period), the responses were analyzed only if the duration of this period allowed a minimum of seven stimuli. During fictive weight support, the responses were analyzed after the initial membrane potential depolarization had reached a tonic plateau (Fig. 1B).
The oligosynaptic EPSPs were frequently preceded by monosynaptic group Ia EPSPs (Figs. 2, 3). To reduce the effect of such contamination on the latencies and amplitudes estimates, we isolated the oligosynaptic EPSPs from the monosynaptic EPSP. This was done by subtracting the "contaminating" monosynaptic EPSP. The traces used for subtraction contained monosynaptic but no oligosynaptic EPSPs (control traces for example). Before subtraction, this monosynaptic EPSP was scaled to the peak amplitude of the "contaminating" monosynaptic EPSPs. The latencies and amplitudes of the oligosynaptic EPSPs were usually measured from the trace remaining after subtracting the trace in the absence of motor activity (control) (Figs. 2C, 3A-C, "difference" trace). However, because disynaptic EPSPs appeared only during the extension phase of fictive locomotion and scratching, disynaptic EPSPs during extension phase were isolated by subtracting the trace during flexion (Fig. 2A,B). The statistics for the latencies and amplitudes are given as mean ± SEM, and statistical tests for differences between the means were done by one-way ANOVA using the Dunnett method for multiple comparisons against a single control group (
< 0.05; Glantz, 1981
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Figure 3. Modulation of group I polysynaptic EPSPs during fictive locomotion, scratching, and weight support. Averaged intracellular recordings from three different motoneurons (1 MG and 2 LGS) showing polysynaptic group I EPSPs (hatched areas) evoked by ankle extensor stimulation during fictive locomotion (A), scratching (B), and weight support (C). Note that when the stimulation was applied during the extension phase of either locomotion or scratching, or during weight support, disynaptic group I EPSPs were also evoked (arrows). For other details, see Figure 2.
To analyze the effects of train stimulation on the timing of nerve activity during scratching, we measured (1) the duration of each ENG burst and each cycle (time between the onset of two consecutive ENG bursts) and (2) plotted these values against time (see Figs. 5C-E, 6C, 7C,D). For the effects on the amplitude of the nerve activity, ENG bursts were averaged and aligned on the onset of the train of stimuli (see Figs. 6B, 7B) or, in the case of continuous stimulation (see Fig. 5B), on the onset of the SmAB activity.
RESULTS
Motor pattern characteristics of fictive scratching and weight support
Figure 1 shows the nerve activities induced in hindlimbs by manual stimulation of the left (A) and the right (B) pinna. Left pinna stimulation (diagram) induced fictive scratching in the left hindlimb. Fictive scratching was divided into two main periods (Deliagina et al., 1981
As described by Sherrington (1910)
2 mV) and never reached >20% of the amplitude of membrane potential oscillations seen during fictive scratching.
Database for intracellular recordings and observations on monosynaptic EPSPs and nonreciprocal IPSPs
The synaptic responses evoked by electrical stimulation (one to three shocks, 2 T) of ankle extensor nerves were examined in all 23 extensor motoneurons (12 experiments) recorded during fictive locomotion (n = 16), scratching (n = 18), and weight support (n = 12). In most cases (n = 16), the motoneurons were recorded during at least two different fictive programs (Table 1, Fig. 2). Seven motoneurons were recorded during locomotion, scratching, and weight support (L + S + W), four during locomotion and scratching (L + S), four during scratching and weight support (S + W), and one during locomotion and weight support (L + W).
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Table 1. Number and type of motoneurons recorded during fictive locomotion (L), scratching (S), and weight support (W) In the present experiments, the responses induced by ankle extensor nerve stimulation often included monosynaptic group Ia EPSPs (17 of 23 extensor motoneurons; Figs. 2, 3). During fictive locomotion and scratching, monosynaptic EPSPs were of smaller amplitude than at rest with mean amplitudes equal to 74 ± 8% (n = 12) and 73 ± 7% (n = 11) of control, respectively. Monosynaptic EPSPs showed little phasic modulation within the locomotor or the scratching cycle (the difference between the mean amplitudes during the flexion and extension phases was <10% during both conditions). During fictive weight support, monosynaptic EPSPs had a mean amplitude equal to 87 ± 10% of control (n = 6).
Nonreciprocal IPSPs in extensor motoneurons after extensor group I afferent stimulation are routinely replaced by group I oligosynaptic EPSPs during fictive locomotion (Gossard et al., 1994
Oligosynaptic group I EPSPs
Disynaptic EPSPs
Stimulation of group I afferents in ankle extensor nerves evoked disynaptic EPSPs in extensor motoneurons during fictive locomotion, scratching, and weight support. As described by others (Schomburg and Behrends, 1978
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Figure 4. Mean latency and amplitude of disynaptic and polysynaptic group I EPSPs during fictive locomotion, scratching, and weight support. The mean latency and amplitude during fictive locomotion, scratching, and weight support are shown both for the disynaptic (A1, A2) and the polysynaptic group I EPSPs (B1, B2). The values during the different phases of locomotion and scratching are indicated separately. The means (open circles) are shown with their corresponding SEs (rectangular boxes). SDs are also displayed (vertical bars). The asterisks indicate single observation.
Polysynaptic EPSPs
Extensor group I EPSPs of longer latency and slower rising phase than the disynaptic group I EPSPs were also induced in extensor motoneurons during fictive locomotion, scratching, and weight support. During fictive locomotion, such polysynaptic group I EPSPs have been studied mainly using train stimulation of three to seven shocks (Gossard et al., 1994Effects of extensor group I input on the scratching rhythm
To determine the effect of the group I reflex activation during fictive scratching, trains of stimuli were delivered to ankle extensor nerves at frequencies similar to the firing frequencies of muscle group Ia afferents during scratching (Feldman et al., 1977
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Figure 5. Continuous activation of ankle extensor group I afferents increases the frequency of the scratching rhythm. A, Pl nerve was stimulated continuously for ~3 sec during scratching. B, The averages during (n = 18; solid trace) and in the absence (n = 18; dashed trace) of stimulation showing that bursts in SmAB were increased both in amplitude and duration whereas the bursts in Sart were increased in amplitude but reduced in duration. After the stimulation, the bursts in SmAB and Sart returned to their original duration (C and D). Similar effects were seen when continuous stimulation was applied again (second stimulation). During stimulations, the majority of the individual scratching cycle durations were reduced (E). At cessation of stimulations, the rhythm frequency returned to a lower value.
Resetting of the rhythm
It is now well established that during locomotion, stimulation of extensor group I afferents during flexion can reset the rhythm to extension (for review, see Hultborn et al., 19981 SD (mean reduction of 65 msec). Similar reset of the scratching rhythm to extension was found in six additional experiments after stimulation of either Pl, MG, or LGS nerves. In two experiments, trains of stimuli were also given during fictive locomotion (data not shown). In both experiments, the locomotor rhythm was also reset to extension.
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Figure 6. Activation of ankle extensor group I afferents resets the scratching rhythm. Short trains to the Pl nerve were given during the flexion phase of scratching (1.8 T × 20; 300 Hz). A small bout of the recording session with integrated, rectified ENGs from Sart and SmAB nerves is displayed in A. The normalized averages (B) were from eight stimulated (solid trace) and 31 control (dashed trace) cycles. C, The effect of Pl nerve stimulation on the scratching cycle duration for the whole recording session is shown. Stimulated cycles are represented by solid circles (arrow).
Increase in amplitude and duration of extensor activity
Increases in the amplitude and/or duration of activity of extensors during fictive locomotion, [termed extension enhancement by Guertin et al. (1995)
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Figure 7. Ankle extensor group I input prolongs the activity of extensors. A, Pl nerve stimulation (trains of 10 stimuli, 200 Hz) was given during the extension phase of scratching. B, The corresponding normalized averages showing that Pl stimulation increased the duration of SmAB burst and prolonged the silent period in Sart. The effects of the stimulation on the duration of SmAB activity and the scratching cycle for the whole recording session (three bouts of scratching) are shown in C and D, respectively.
DISCUSSION
The present study shows that the ability of ankle extensor group I afferents to mediate oligosynaptic excitation of homonymous and synergist motoneurons is not restricted to locomotor activity. As during fictive locomotion, oligosynaptic excitation during fictive scratching and weight support is the result of two types of group I EPSPs (disynaptic and polysynaptic) that can be distinguished by their latency and pattern of modulation. For both EPSPs, the mean latency and the pattern of modulation during fictive scratching and weight support were similar to those during fictive locomotion. Thus, it is suggested that oligosynaptic group I EPSPs are mediated via the same reflex pathways during the three motor programs.
Sources of modulation of the oligosynaptic group I EPSPs during fictive scratching and weight support
The modulation of the oligosynaptic group I EPSPs in extensor motoneurons during fictive locomotion has been discussed extensively in previous studies (Brownstone et al., 1994
In the present study, disynaptic group I EPSPs were detected only when the motoneurons were relatively depolarized, i.e., during the extension phase of scratching and during fictive weight support. On the other hand, polysynaptic group I EPSPs, which were also detected during motoneuron depolarization, were evoked most often when the motoneurons were most hyperpolarized, i.e., during the flexion phase of scratching. Because both EPSPs can be evoked in the same motoneurons, the mechanisms responsible for the modulation are probably selective for each type of EPSP, and mechanisms such as a widespread change in motoneuronal conductance are unlikely to be involved. Selective mechanisms that may account for the modulation of the group I oligosynaptic EPSPs include (1) depolarization of the group I afferent fiber terminals, (2) activation of voltage-dependent conductances in extensor motoneurons, and (3) changes of excitability of the interneurons interposed between the group I afferents and the motoneurons. These possibilities are considered in turn.
Depolarization of primary afferent terminals (PAD) may decrease the transmission from primary afferents and, in theory, contribute to the modulation of reflex pathways. However, the PAD pattern produced in group I afferents during the induction and throughout fictive scratching (Baev and Kostyuk,1981
An activation of voltage-dependent conductances by input to motoneurons from the interneurons responsible for the generation of the locomotor and scratching drive potentials may contribute to the modulation of the group I oligosynaptic EPSPs (Brownstone et al., 1994
A change in the excitability of the interneurons may be the most plausible mechanism for the modulation of the group I oligosynaptic EPSPs. This would be consistent with the finding that candidate interneurons for the mediation of the disynaptic group I EPSPs responded to extensor group I afferent stimulation during the extension phase of locomotion but not during the flexion phase and neither at rest (McCrea, 1998
A common rhythm-generating network for locomotion and scratching?
Locomotion and scratching are clearly different motor behaviors involving different movement trajectories and underlying patterns of muscle activity. Therefore, one can hardly expect that all the interneurons activated during locomotion will also be activated during scratching and vice and versa. Consistent with this idea is the recent demonstration that the interneurons that mediate cutaneous disynaptic EPSPs in extensor motoneurons can be activated during fictive locomotion but not during scratching (Degtyarenko et al., 1998
The idea of a common network for the generation of both the locomotion and the scratching rhythms has been proposed earlier by Orlovsky and collaborators (for review, see Gelfand et al., 1988
Functional relevance
The present experiments show that the excitatory group I reflex pathways are open for transmission during fictive scratching and weight support, providing us with a neuronal substrate for excitatory feedback from extensor group I afferents during these activities. The importance of the excitatory group I reflexes during real scratching and weight support will depend, however, on the amount of activity in the primary afferents. Unfortunately, there is little information on this, particularly for group Ib afferents, which are believed to represent the main input to these reflex pathways (see introductory remarks). We know that during real locomotion, group Ib afferents monitor the changes in muscle force (Prochazka and Gorassini, 1998a
Excitatory feedback from extensor group I afferents during real scratching may be used to adjust the onset and duration of hindlimb extensors (Kuhta and Smith, 1990
FOOTNOTES Received June 28, 1999; revised Sept. 27, 1999; accepted Sept. 28, 1999.
This work was supported by grants from the Danish Medical Research Council, the Lundbeck Foundation, the NOVO Nordisk Foundation, and the Human Frontier Science Program Organization. We thank the following people for their assistance: Mrs. Lillian Grøndahl and Conni Temdrup for their help during the experiments, Allan Djørup with computers, Kurt Helmer with mechanics, and Egil Gudbrandsen and the late Jan Nielsen with electronics. We would also like to thank Drs. Morten Raastad and Matthew Tresch for their useful comments.
Correspondence should be addressed to M.-C. Perreault, Department of Physiology, University of Oslo, P.O. Box 1103, Blindern, N-0317 Oslo, Norway. E-mail: m.c.perreault{at}basalmed.uio.no.
Dr. Denton's present address: Institute of Biomedical and Life Sciences, Division of Neuroscience and Biomedical Systems, West Medical Building, University of Glasgow, Glasgow G12 8QQ, Scotland.
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