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The Journal of Neuroscience, March 15, 2003, 23(6):2434
Bimodal Locomotion Elicited by Electrical Stimulation of the Midbrain in the Salamander Notophthalmus viridescens
Jean-Marie Cabelguen1, Céline Bourcier-Lucas2, and Réjean Dubuc2, 3 1 Institut National de la Santé et de la Recherche Medicale, Equipe 0358, Physiopathologie des Réseaux Neuronaux Médullaires, Institut François Magendie, 33077 Bordeaux Cedex, France, 2 Centre de Recherche en Sciences Neurologiques, Université de Montréal, Montréal, Québec, Canada H3C 3J7, and 3 Département de Kinanthropologie, Université du Québec à Montréal, Montréal, Québec, Canada H3C 3P8
ABSTRACT
TOP
ABSTRACT
Introduction
The present experiments were designed to identify the mesencephalic locomotor region (MLR) in the salamander. An in vitro semi-intact preparation from a decerebrate adult salamander (Notophthalmus viridescens) was developed in which the locomotor activities were monitored from electromyographic and video recordings. The results show that the two locomotor modes exhibited by salamanders (i.e., stepping and swimming) were evoked by electrical microstimulation (5-15 Hz; 0.1-10 µA; 2 msec pulses) of a circumscribed region in the caudal mesencephalon. At threshold current strength (0.5-3.5 µA at 15 Hz), rhythmic limb movements and intersegmental coordination, such as during stepping, were induced. As the stimulation strength was subsequently increased, the frequency of stepping became more rapid, and, at 2.0-5.5 µA, the limbs were held back against the body wall and swimming movements of the trunk were induced. An additional increase of the stimulation strength induced an increase of the frequency and amplitude of the swimming movements. Anatomical studies conducted in parallel revealed the presence of choline acetyltransferase immunoreactive cells in the functionally identified MLR region. Together, the present results indicate that the MLR is present in salamanders and that its level of activation determines the mode of locomotion. Walking is induced at low activation levels, and swimming, which constitutes a faster mode of locomotion, requires stronger stimulation of the MLR. Furthermore, as in other vertebrates, the MLR contains cholinergic cells.
Key words: salamander; mesencephalic locomotor region; locomotion; swimming; stepping; brainstem
Introduction
Adult salamanders are limbed lower vertebrates that spontaneously display two locomotor modes: swimming and terrestrial stepping. The two locomotor modes differ as to their patterns of activation of epaxial musculature (intersegmental coordination pattern) and limb muscles (Frolich and Biewener, 1992
; Delvolvé et al., 1997
One region located in the midbrain from which locomotion can be initiated is the mesencephalic locomotor region (MLR) (Shik et al., 1966
Materials and Methods
Experiments were performed on 28 adult salamanders (Notophthalmus viridescens) with snout vent length (SVL) ranging from 40 to 50 mm (44.9 ± 0.1 mm, mean ± SEM). The animals were obtained from the Connecticut Valley Biological Supply Company (Southampton, MA) and kept in an aquarium at room temperature. All experimental procedures conformed to the Canadian Medical Research Council guidelines and were approved by the University Animal Care Committee.
Semi-intact preparation. The animals were deeply anesthetized by immersion in a 0.1% aqueous solution of tricaine methanesulfonate (MS222; Sigma, Oakville, Ontario, Canada). Under general anesthesia, the low jaw and the forelimbs were removed, and the animal was eviscerated. The cranium and the remainder of the body, which included the hindlimbs and the tail, were placed in a Petri dish filled with cooled (6°C) and oxygenated amphibian Ringer's solution (Delvolvé et al., 1997
Brainstem stimulation. Glass-coated tungsten stimulating microelectrodes (~2.5 M
impedance; 10 µm tip exposed; Micro Probe, Gaithersburg, MD) were used for monopolar electrical stimulation. Electrodes were angled 30° anteroposteriorly, and penetrations, separated by 25 µm, were performed at different sites along the brainstem using a manually driven micromanipulator. At each site, the electrode was lowered into the brain tissue by 25 µm steps.
A stimulator with a constant-current isolation unit was used to deliver negative pulses of 2 msec duration at frequencies of 5-15 Hz. At each stimulated site, the current was increased by steps of 0.1 up to 10 µA. Typically, a few search trials were performed with continuous stimulation not exceeding 30 sec. A rest period of
1 min was allowed between successive trials. Once the MLR was localized, we did not stimulate for >30 sec in any one trial because of concerns about damaging the stimulation site. For later histological identification, an electrolytic lesion (n = 12) was made at the stimulation site using DC current (5 µA) applied for 10 sec at the end of experiments.
EMG recording. EMG recordings were made in 11 animals with pairs of insulated stainless steel wires (diameter of 50 µm; California Fine Wire, Grover Beach, CA) with bared ends (exposure <0.5 mm) inserted through the skin into myomeres of the musculus dorsalis trunci. The electrode tips were separated by <1 mm, and their rostrocaudal position was expressed as a fraction of the SVL. The voltage signals from electrodes were differentially amplified 10,000 times (bandpass of 30-300 Hz with a 60-Hz notch filter), displayed on an oscilloscope, and stored on magnetic tape.
Video recording. In two experiments, the motor responses of the animal were videotaped with a camera positioned 1 m above the bath. Each video frame was captured (Northern Exposure software; Empix Imaging, Mississauga, Ontario, Canada) to draw the body shape of the salamander. This method allowed us to characterize the induced motor behaviors.
Anatomical studies. The distribution of cholinergic neurons in the isthmic region of salamanders (n = 17; 12 animals with an electrolytic lesion in the MLR and five unlesioned) was studied using immunohistochemistry for choline acetyltransferase (ChAT). The fixed brains in 4% paraformaldehyde in 0.1 M phosphate buffer, pH 7.4, were frozen and cut at 20 µm thickness on a cryostat (American Optical, Buffalo, NY) or embedded in agarose and cut at 40 µm thickness on a vibratome (TPI, St. Louis, MO). The sections (mounted on gelatinized slides or free-floating sections, respectively) were then processed for immunohistochemistry using a procedure adapted from Marin et al. (1997)
Results
After a recovery period of 1-2 hr, all preparations were reactive to touching of the head or gentle squeezing of the tail or the hindlimbs. Most of them (n = 15) displayed some spontaneous rhythmic movements of the trunk and/or hindlimbs, but these movements were infrequent, and sequences were rarely longer than a few cycles. Therefore, they were not analyzed. Quantitative analyses were performed only on animals in which EMG recordings were made (n = 11).
For a typical experiment, repetitive (15 Hz) electrical stimulation of a mesencephalic region lying just rostral to the isthmus induced two distinct rhythmic motor patterns depending on the current intensity (Fig. 1). At low current intensity (2.8 µA), the motor pattern was characterized by an in-phase activation of the ipsilateral trunk myomeres and an alternated activation of left and right trunk myomeres (Fig. 1A1). The video recordings also showed that the electrical stimulation evoked small-amplitude rhythmic lateral displacements of the midtrunk and rhythmic alternated movements of the hindlimbs (Fig. 1A2). As the current intensity was subsequently increased to 3.8 µA, the induced EMG pattern changed dramatically, as did the movement pattern. The frequency and the amplitude of the EMG bursts increased markedly, and there was a rostrocaudal activation of trunk myomeres on the same side of the body, although left and right trunk myomeres were still activated in alternation (Fig. 1B1). The body and tail displayed rhythmic lateral displacements of large amplitude, whereas the hindlimbs were held back against the body wall (Fig. 1B2).
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Figure 1. Stepping (A1, A2) and swimming (B1, B2) elicited by electrical stimulation of the same midbrain site in an adult salamander. A1, EMG activity recorded at 0.53 SVL (i Rostral) and 0.76 SVL (i Mid) on the right side and at 0.46 SVL (co Rostral) on the left side during stepping evoked by midbrain microstimulation (2 msec pulses at 15 Hz, 2.8 µA). In-phase activation of ipsilateral myomeres is clearly visible (dashed line). A2, Drawings illustrating the body contours every 10th successive frame (video sampling at 60 Hz) during one step cycle taken from the same stepping episode. B1, EMG activity recorded at the same segmental levels during a swimming episode evoked by microstimulation of the same midbrain site (2 msec pulses at 15 Hz, 3.8 µA). A time delay between EMG bursts of ipsilateral myomeres is clearly visible (dashed line). B2, Body movements during one swimming cycle taken from the same swimming episode.
Similar EMG and movement patterns have been reported previously during overground stepping and swimming, respectively, in the intact salamander (Frolich and Biewener, 1992
The effective sites of stimulation were found on either side in the isthmic region, close to the midline, extending ~100 µm rostrocaudally. A good indication that the electrode was located in the effective zone was the observed stiffness of the trunk produced before locomotor movements. This postural change was related directly to the EMG pattern displayed by myomeres before the MLR-induced locomotor episode. Typically, a burst of EMG activity occurred in the rostral myomeres ipsilateral to the stimulation side, followed by a bilateral sustained EMG activity along the body (Fig. 2A1). Thereafter, the EMG pattern changed dramatically to a locomotor pattern characterized by vigorous EMG discharges during swimming (Fig. 2A2).
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Figure 2. Initiation and termination of MLR-induced locomotion. A1, A period of postural adjustment began (arrow) a few seconds after the onset of MLR stimulation and lasted ~25 sec before the locomotion started (locomotor activity). The gray bar at bottom indicates the period during which the MLR was stimulated (2 msec pulses at 15 Hz, 2.5 µA). A2, Expansion of a part of the locomotor episode shown in A1. The rostrocaudal phase lag between EMG bursts of ipsilateral myomeres (dashed line) and the alternation between ipsilateral and contralateral EMG bursts are clearly visible. Same voltage amplification in A1 and A2. B1, Relationship between the onset delay and the stimulus intensity. B2, Relationship between the end ("offset") delay and the stimulation intensity. In B1 and B2, data are from the same four animals. The gray areas indicate the range of stimulus intensities that evoked stepping and/or swimming.
In four animals, the effective sites were not successfully identified, probably because of the very small size of the region and/or the damage that may have resulted from the multiple electrode penetrations in the region containing the effective sites. The extent of spread of the current injection was not tested, but moving the electrode away (25 µm) from an effective site led to disappearance of locomotion. Moreover, stimulation of slightly more rostral or lateral sites produced different motor responses (e.g., axial twisting and rhythmic movements of the tip of the tail or of only one hindlimb) or was not effective.
MLR-evoked locomotion (stepping or swimming) usually continued throughout the stimulation duration (up to 30 sec). However, signs of adaptation were sometimes observed (i.e., both the frequency and the amplitude of the evoked EMG bursts decreased and eventually locomotion stopped). The delay between the onset of stimulation and the onset of the MLR-evoked locomotion depended on the animal, but, for all individuals, it was always shorter for higher stimulation intensities. In four animals, we quantified the relationship between the onset delay and the current strength at a fixed frequency of stimulation (15 Hz). Figure 2B1 shows that there was a significant negative correlation (r = 0.63; p < 0.001) between the onset delay and the stimulus strength. Locomotion usually ceased on termination of the stimulation except at the highest current intensities (i.e., during fast swimming), at which it outlasted the stimulation period by a few seconds. A weak but significant positive correlation (r = 0.32; p < 0.05) was found between the offset delay and the current strength in data pooled from four individuals (Fig. 2B2).
In some cases, during constant electrical stimulation at intensity above the stepping threshold, a stepping pattern occurred first and then switched spontaneously in only one cycle to a swimming one (Fig. 3A). Swimming lasted a few cycles and switched back to a stepping pattern in one cycle.
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Figure 3. MLR stimulation induces two modes of locomotion in salamander. A, Traces are, from top to bottom, EMG activity recorded at 0.39 SVL (i Rostral) and 0.74 SVL (i Mid) on the right side and 0.41 SVL (co Rostral) on the left side. Electrical stimulation of the MLR (2 msec pulses at 15 Hz, 1.25 µA) started 2.2 sec before recordings and was maintained 30 sec. Note the abrupt switching from stepping to swimming and back to stepping. B1, Effect of increasing the stimulus intensity (2 msec pulses at 15 Hz) on the frequency of swimming. B2, Effect of increasing the stimulus frequency (2 msec at 6 µA) on the frequency of swimming. Bars are mean values, and error bars are SEM.
During evoked stepping, the frequency and the amplitude of the EMG bursts depended on the stimulation strength intensity. Increasing the current level from 2.8 to 3.5 µA (at 15 Hz) increased the intensity of the individual EMG bursts and also doubled the stepping rhythm (0.08-0.16 Hz). The amplitude and the frequency of the EMG bursts during swimming were also related to the intensity of stimulation. The frequency of bursting (Fig. 3B1) increased from 1.57 ± 0.07 to 2.01 ± 0.06 Hz when the current level was increased from 5.5 to 7 µA (at 15 Hz). Likewise, at a constant stimulating current (6 µA in this experiment), the swimming rhythm increased (1.12 ± 0.09 to 1.83 ± 0.04 Hz) (Fig. 3B2) as the stimulation frequency increased (8-15 Hz). In this example, swimming switched to stepping when the frequency of 6 µA amplitude pulses was lowered to 7 Hz, and, as the stimulating frequency was lowered more, the stepping pattern waned to a stop for stimulation frequency <5 Hz (data not illustrated).
Therefore, it could be concluded that the amplitude and frequency of the EMG bursts during evoked locomotion (stepping or swimming) could be controlled by the strength of the stimulation.
There is evidence that cholinergic cells are located in the physiologically identified MLR of several vertebrate species (Grillner et al., 1997
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Figure 4. ChAT-IR cells around the MLR-coagulated site. A, Transverse section (40 µm thick) at the isthmic level showing the coagulated site (right) and the intact side (left). Note the dense plexus of ChAT-IR fibers in the interpeduncular nucleus. B, Magnification of the boxed area in A showing ovoid ChAT-IR cells (arrows) and numerous ChAT-IR fibers around the coagulated site. C, Transverse section (20 µm thick) at approximately the same level as in A. The interpeduncular nucleus shows intense labeling. D, Magnification of the boxed area in C showing two distinct groups of ChAT-IR cells, the LDT and the NI. Note the axonal tract arising from the caudal LDT. Scale bars: A, C, 200 µm; B, D, 100 µm. IP, Interpeduncular nucleus; OT, optic tectum.
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Figure 5. Schematic representation of the distribution of ChAT-IR cells at the isthmic level. Each schematic represents three consecutive 20-µm-thick sections. Total distance, 240 µm. Scale bars: whole brain representation, 1 mm; brainstem transverse sections, 200 µm. IP, Interpeduncular nucleus; OT, optic tectum.
Discussion
Two main conclusions can be drawn from the present study: (1) the MLR is present in salamanders, and (2) depending on its strength, the MLR activation induces two distinct locomotor patterns (stepping and swimming). It is noteworthy that walking occurs at low intensity, whereas swimming requires higher intensities. This is consistent with swimming being the fastest mode of locomotion in these animals, which are mechanically better adapted for swimming than walking because of their sprawling posture and their short limbs (Ashley-Ross, 1994
For both walking and swimming, the locomotor rhythm was always slower than the locomotor rhythms in intact salamanders (Frolich and Biewener, 1992
Previous behavioral observations in decerebrated Necturus have shown that electrical stimulation of the lateral mesencephalic tegmentum can induce rhythmic movements of the body, the tail, and the limbs in different combinations (Shik, 1997
The present study also shows that the effective sites of stimulation were located within a specific and relatively small region at the mesopontine border. The MLR is a structure that was defined functionally rather than anatomically. Physiological and pharmacological observations made in mammals indicate that cell bodies and not passing axons constitute the MLR. Our data did not allow us to determine whether the neural elements activated were passing axons and/or neurons. However, stimulation of the rostral midbrain did not evoke locomotion, suggesting that there is not a more rostral nucleus projecting through the region that we now define as the MLR of salamanders and that is responsible for the locomotor movements observed. Therefore, a subset of this area must contain the cell bodies of origin for descending pathways responsible for initiating locomotion. In higher vertebrates, local electrical stimulation in different parts of the MLR generates various locomotor behaviors, suggesting that this region is heterogeneous (Sinnamon, 1993
There is anatomical and electrophysiological evidence in several species that the MLR activates the spinal pattern generators for locomotion through an activation of RS neurons (for review, see Orlovsky et al., 1999
It is unknown whether or not the activated target RS cells involved are different during MLR-induced stepping and swimming. One possibility is that stepping and swimming involve specific populations of RS cells and that the switch to swimming results simply from an additional recruitment of groups of RS neurons. However, because at a specific stimulation strength, locomotion could sometimes spontaneously switch from stepping to swimming and back to stepping, this hypothesis seems less likely. Another possibility is that the transition between the two locomotor modes may result from a reconfiguration of the same spinal network by RS modulatory influences. Hence, the abrupt switch from stepping to swimming would be explained by modifications of cellular properties and/or intercellular connections within that spinal network. Interestingly, it has been proposed previously that the axial motor patterns during swimming and stepping are both generated by the same, essentially lamprey-like, network that receives different input drives from the limb locomotor networks, depending on the locomotor mode (Delvolvé et al., 1997
In conclusion, we showed that salamanders, like other vertebrates, do have a specific mesencephalic locomotor region that controls the initiation of locomotion and that the level of activation of that region determines the mode of locomotion. The presence of such a region with characteristics similar to that found in other vertebrates provides additional evidence that the mechanisms of brainstem control of locomotion are well preserved throughout the vertebrate phylum. Moreover, a cholinergic component from the MLR is most likely involved in the initiation of locomotion, as in mammals and lampreys.
FOOTNOTES Received Oct. 30, 2002; revised Dec. 13, 2002; accepted Dec. 19, 2002.
This work was supported by a group grant (Neurological Sciences) from the Canadian Institutes for Health Research (CIHR) and the Institut National de la Santé et de la Recherche Medicale INSERM-CIHR exchange program. C.B.L. received a studentship from a group grant from Le Fonds pour La Formation de Chercheurs et l'Aide à la Recherche (Québec, Canada). We thank D. Veilleux for her technical assistance.
Correspondence should be addressed to Prof. Jean-Marie Cabelguen, Institut National de la Santé et de la Recherche Médicale, Equipe 0358, Physiopathologie des Réseaux Neuronaux Médullaires, Institut François Magendie, 1 rue Camille Saint-Saëns, 33077 Bordeaux Cedex, France. E-mail: cabelguen{at}bordeaux.inserm.fr.
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Copyright © 2003 Society for Neuroscience 0270-6474/03/2362434-06$05.00/0
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