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The Journal of Neurophysiology Vol. 87 No. 6 June 2002, pp. 2676-2683
Copyright ©2002 by the American Physiological Society
1Shanghai Institute of Materia Medica, Shanghai Institutes of Biological Sciences, Chinese Academy of Sciences, Shanghai 200031, China; and 2The Nobel Institute for Neurophysiology, Department of Neuroscience, Karolinska Institutet, SE-171 77 Stockholm, Sweden
Hu, Guo-Yuan,
Zoltán Biró,
Russell H. Hill, and
Sten Grillner.
Intracellular QX-314 Causes Depression of Membrane Potential
Oscillations in Lamprey Spinal Neurons During Fictive
Locomotion. J. Neurophysiol. 87: 2676-2683, 2002. Spinal neurons undergo large cyclic membrane potential
oscillations during fictive locomotion in lamprey. It was investigated whether these oscillations were due only to synaptically driven excitatory and inhibitory potentials or if voltage-dependent inward conductances also contribute to the depolarizing phase by using N-(2,6-dimethylphenyl carbamoylmethyl)triethylammonium
bromide (QX-314) administered intracellularly during
fictive locomotion. QX-314 intracellularly blocks inactivating and
persistent Na+ channels, and in some neurons,
effects on certain other types of channels have been reported. To
detail the effects of QX-314 on Na+ and
Ca2+ channels, we used dissociated lamprey
neurons recorded under whole cell voltage clamp. At low intracellular
concentrations of QX-314 (0.2 mM), inactivating
Na+ channels were blocked and no effects were
exerted on Ca2+ channels (also at 0.5 mM). At 10 mM QX-314, there was, however a marked reduction of
ICa. In the isolated spinal cord of
the lamprey, fictive locomotion was induced by superfusing the spinal cord with Ringer's solution containing
N-methyl-D-aspartate (NMDA), while recording the
locomotor activity from the ventral roots. Simultaneously, identified
spinal neurons were recorded intracellularly, while infusing QX-314
from the microelectrode. Patch electrodes cannot be used in the intact
spinal cord, and therefore "sharp" electrodes were used. The
amplitude of the oscillations was consistently reduced by 20-25% in
motoneurons (P < 0.05) and unidentified spinal neurons
(P < 0.005). The onset of the effect started a few
minutes after impalement and reached a stable level within 30 min.
These effects thus show that QX-314 causes a reduction in the amplitude of membrane potential oscillations during fictive locomotion. We also
investigated whether QX-314 could affect glutamate currents by applying
short pulses of glutamate from an extracellular pipette. No changes
were observed. We also found no evidence for a persistent Na+ current in dissociated neurons, but these
cells have a much-reduced dendritic tree. The results indicate that
there is an inward conductance, which is sensitive to QX-314, during
membrane potential oscillations that "boosts" the synaptic drive
during fictive locomotion. Taken together, the results suggest that
inactivating Na+ channels contribute to this
inward conductance although persistent Na+
channels, if present on dendrites, could possibly also contribute to
shaping the membrane potential oscillations.
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