1Institut National de la Santé et de
la Recherche Médicale EP9914,
Delvolvé, Isabelle,
Pascal Branchereau,
Réjean Dubuc, and
Jean-Marie Cabelguen.
Fictive Rhythmic Motor Patterns Induced by NMDA in an In Vitro
Brain Stem-Spinal Cord Preparation From an Adult Urodele.
J. Neurophysiol. 82: 1074-1077, 1999.
An in
vitro brain stem-spinal cord preparation from an adult urodele
(Pleurodeles waltl) was developed in which two fictive rhythmic motor patterns were evoked by bath application of
N-methyl-D-aspartate (NMDA; 2.5-10 µM)
with D-serine (10 µM). Both motor patterns displayed left-right alternation. The first pattern was characterized by cycle
periods ranging between 2.4 and 9.0 s (4.9 ± 1.2 s,
mean ± SD) and a rostrocaudal propagation of the activity in
consecutive ventral roots. The second pattern displayed longer cycle
periods (8.1-28.3 s; 14.2 ± 3.6 s) with a caudorostral
propagation. The two patterns were inducible after a spinal transection
at the first segment. Preliminary experiments on small pieces of spinal cord further suggested that the ability for rhythm generation is
distributed along the spinal cord of this preparation. This study shows
that the in vitro brain stem-spinal cord preparation from
Pleurodeles waltl may be a useful model to study the
mechanisms underlying the different axial motor patterns and the
flexibility of the neural networks involved.
The neural networks generating axial muscle
activations during locomotion have been investigated extensively in the
lamprey (Grillner et al. 1995 Experiments were performed on 21 adult urodele amphibians
(Pleurodeles waltl) previously kept at 15°C for >1 wk.
The animals were deeply anesthetized by immersion in a 0.1% aqueous
solution of tricaine methanesulfonate (Sigma; MS 222). They were
perfused transcardially with cold oxygenated Ringer solution (in mM:
130 NaCl, 2.6 CaCl2, 2.1 KCl, 0.2 MgCl2, 1 NaHCO3, 5 glucose,
and 4 HEPES, pH 7.5) and transected at lumbar level. The rostral part was dissected in continuously perfused cold Ringer (3 ml/min). The
dorsal part of the skull and vertebrae was removed, and the preparation
was decerebrated by removing the brain tissue rostral to the
mesencephalon. The more caudal spinal cord (5th to 16th segments) was
completely isolated from the vertebrae, and special care was taken to
dissect the ventral roots (VRs) over a length of 1-2 mm (Fig.
1A). The dura mater and the
choroid plexus were removed to facilitate oxygen diffusion into the
preparation. The preparation was pinned down and stored overnight at
~5°C in oxygenated Ringer solution containing a neuromuscular
blocking agent (
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
) and Xenopus
embryo (Roberts et al. 1997
). In vitro preparations have
been developed more recently in higher vertebrates and provided
information on the overall structure of the spinal locomotor networks.
The complexity of the mammalian spinal cord has precluded, however, a
detailed understanding of the circuitry responsible for the generation
of stepping (Kiehn et al. 1997
). In this context, the
adult urodele appears as a useful model because it exhibits
spontaneously swimming and overground stepping. In a previous study we
have characterized the patterns of activation of epaxial myomeres
(intersegmental coordination patterns) during both swimming and
stepping in an intact adult urodele (Pleurodeles waltl)
(Delvolvé et al. 1997
). To study the neural
networks responsible, an in vitro brain stem-spinal cord preparation
from the adult urodele, P. waltl was used (see also
Wheatley et al. 1992
). The present paper reports on
results obtained with this in vitro preparation.
METHODS
TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
-bungarotoxin 1 µM, Sigma) to prevent the
remaining muscle fibers from contracting. All preparations remained
viable for >48 h.
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Fig. 1.
A: schematic representation of the preparation.
Extracellular recordings were made from 3 successive ventral roots
(VRs) on the ipsilateral side (iVR6, iVR9, and
iVR13) and from 1 VR on the contralateral side
(coVR8). Activity was induced by bath application of
N-methyl-D-aspartate (NMDA; 2.5-10 µM)
and D-serine (10 µM). B: 2 patterns of
rhythmic activity. B1: fast rhythmic activity with a
rostrocaudal intersegmental propagation. B2: slow
rhythmic activity with a caudorostral intersegmental propagation.
C: changes in the frequency of the rhythmic activity
(slow pattern) induced by different concentrations of NMDA. Vertical
bars indicate mean ± SE of cycle duration.
After a recovery of 12 h, motor activity was induced by bath application of a mixture of 2.5-10 µM N-methyl-D-aspartate (NMDA; Sigma) and 10 µM D-serine (Sigma). Ventral root activity was recorded by means of tight-fitting glass suction electrodes. The neurograms were amplified, filtered (70 Hz to 3 kHz), and stored on a computer for subsequent analyses using the Cambridge Electronic Design 1401 system. In each of five animals, one piece of two or three spinal segments was cut with small scissors, and ventral root activity was recorded after 1 h of recovery.
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RESULTS |
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One of the 21 preparations displayed spontaneous rhythmic activity alternating between the 2 sides in normal Ringer. This activity never lasted >1 min. After adding NMDA (2.5-10 µM) with D-serine (10 µM) to the bath, sustained rhythmic bursts of activity occurred within ~20 min in 20 of the 21 preparations. This activity persisted for up to 2 h and disappeared after wash out of the drugs. The threshold concentration of NMDA for evoking rhythmic activity was 2.5-5.0 µM. At concentrations above 15 µM, the activity in all VRs became tonic.
Two distinct patterns of rhythmic activity were observed. The first one was characterized by a rostrocaudal propagation of the rhythmic activity along the spinal cord (Fig. 1B1). The second one consisted of a slower rhythm with a caudorostral propagation (Fig. 1B2). Increasing the concentration of NMDA from 5.0 to 7.5 µM increased progressively the slow rhythm frequency in five experiments (Fig. 1C; t-test: P <0.0001) while it elicited a switch to a fast rhythm in two experiments.
The cycle periods, defined as the time intervals between the onset of
two successive bursts in a given VR, were distributed in two distinct
ranges (measured in 4 animals): 2.4-9.0 s (4.9 ±1.2 s, mean ± SD; n = 86; Fig.
2A; ; "fast
rhythm") and 8.1-28.3 s (14.2 ± 3.6; n = 290; Fig. 2A;
; "slow rhythm"). The delay between
motor burst onsets in the 9th and 11th VRs was measured during both
rhythmic motor activities in three animals. The phase lag (delay/cycle
duration in the 9th VR) had a positive value (0.13 ± 0.10) during
the fast rhythmic activity (Fig. 2B; empty bars) and a
negative value (
0.16 ± 0.09) during the slow rhythmic activity
(Fig. 2B; filled bars). The phase lag values for the two
rhythmic patterns were significantly different from zero
(t-test: P < 0.001) and each other
(t-test: P < 0.0001).
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At 5 µM NMDA, 17 preparations displayed a slow rhythmic motor pattern, whereas one showed the fast rhythmic pattern. Interestingly in two preparations, both patterns of rhythmic activity were observed as the rhythmic activity spontaneously switched from one pattern to the other without any changes in the concentration of NMDA. This is exemplified in Fig. 3A, where the rhythmic activity first switched from a slow rhythm to a fast one, and then again to a slow rhythm, with a short recurrence of the slow rhythm in the middle of the fast activity (arrow). The transition from one pattern to the other occurred within 1-2 cycles. In preparations displaying both patterns, the slow rhythm predominated with longer and more numerous episodes. In seven experiments it was also possible to selectively induce a switch from slow to fast activity by increasing the NMDA concentration from 5 to 10 µM (Fig. 3B). A spinal transection was performed at the first spinal segment in five experiments; three preparations displayed a slow rhythm, one a fast rhythm, and one both rhythms, indicating that both patterns were present in the isolated spinal cord.
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Preliminary experiments were carried out to determine how distributed the neural network-generating rhythmic axial motor activity was. Figure 3C shows a bilaterally alternating rhythmic motor activity (slow rhythm) in a piece a of three spinal segments (11th to 13th) during coapplication of NMDA (5 µM) and D-serine (10 µM) in the bath. Ventral root discharges on one side were nearly synchronous in this short piece of spinal cord. A similar rhythmic activity was observed in the other pieces of the three spinal segments (2nd to 4th; 8th to 10th; 14th to 16th) and in one piece of two segments (14th to 15th).
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DISCUSSION |
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Our results show that the in vitro brain stem-spinal cord preparation from the adult P. waltl superfused with a mixture of NMDA and D-serine displays a sustained rhythmic motor activity in the absence of rhythmic sensory inputs (fictive activity). Two distinct patterns were observed with different intersegmental coordination.
The fast rhythm displayed a rostrocaudal propagation as seen during
swimming in intact urodeles (Delvolvé et al. 1997;
Frolich and Biewener 1992
). It remains to be determined
whether this pattern of coordination reverses at two specific sites of
the trunk, as reported for myomere activations during forward swimming
in intact animals (Delvolvé et al. 1997
).
During the slow pattern, the intersegmental coordination was reversed
with a caudorostral propagation. This feature is similar to that
reported for the axial motor pattern recorded during real or fictive
struggling in Xenopus embryos (Green and Soffe
1996; Kahn and Roberts 1982
). However, further
experiments are needed to establish whether the adult Pleurodeles
waltl can exhibit a behavior similar to struggling seen in
Xenopus tadpoles.
The NMDA-evoked rhythms observed in the present study were slower than
the locomotor rhythms in intact animals (Devolvé et al.
1997). The activation of non-NMDA receptors might speed up the
fictive rhythm as reported in lamprey (Brodin et al.
1985
).
Our preliminary experiments further suggest that the rhythm-generating
capability is distributed along the spinal cord. Hence the axial
locomotor network in P. waltl might have a similar
longitudinal organization (chain of coupled segmental oscillators) to
the lamprey or Xenopus embryo locomotor networks
(Cohen and Wallén 1980; Roberts and Alford
1986
). Although in lampreys, every isolated spinal segment
shows equal rhythm-generating capability (Grillner et al.
1983
), in the Xenopus embryos, caudal spinal
segments show progressively less ability to sustain a rhythm
(Roberts and Alford 1986
). Further experiments are in
progress to investigate whether the frequency and pattern of motor
activity are similar in every piece of the spinal cord of P. waltl.
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ACKNOWLEDGMENTS |
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We thank Dr. T. Bem for valuable comments on the manuscript.
This study was supported by grants from Université Bordeaux I, the Conseil Régional d'Aquitaine, a France-Québec exchange program, and a Group grant from the Canadian Medical Research Council to R. Dubuc.
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FOOTNOTES |
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Address for reprint requests: J.-M. Cabelguen, Institut National de la Santé et de la Recherche Médicale EP9914, rue Camille Saint-Saëns, F-33077 Bordeaux Cedex, France.
The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
Received 24 December 1998; accepted in final form 22 April 1999.
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