 |
||||
|
||||
|
||||
|
||||
Previous Article | Next Article
The Journal of Neuroscience, March 15, 2003, 23(6):2002
BRIEF COMMUNICATION
GABAergic Control of Action Potential Propagation along Axonal Branches of Mammalian Sensory NeuronsDorly Verdier1, James P. Lund1, 3, and Arlette Kolta1, 2, 3 1 Centre de Recherche en Sciences Neurologiques, and 2 Faculté de Médecine Dentaire, Université de Montréal, Montréal, Québec H3C 3J7, Canada, and 3 Faculty of Dentistry, McGill University, Montréal, Québec H3A 2B2, Canada
ABSTRACT
TOP
ABSTRACT
Introduction
The main axons of mammalian sensory neurons are usually viewed as passive transmitters of sensory information. However, the spindle afferents of jaw-closing muscles behave as if action potential traffic along their central axons is phasically regulated during rhythmic jaw movements. In this paper, we used brainstem slices containing the cell bodies, stem axons, and central axons of these sensory afferents to show that GABA applied to the descending central (caudal) axon often abolished antidromic action potentials that were elicited by electrical stimulation of the tract containing the caudal axons of the recorded cells. This effect of GABA was most often not associated with a change in membrane potential of the soma and was still present in a calcium-free medium. It was mimicked by local applications of muscimol on the axons and was blocked by bath applications of picrotoxin, suggesting activation of GABAA receptors located on the descending axon. Antidromic action potentials could also be blocked by electrical stimulation of local interneurons, and this effect was prevented by bath application of picrotoxin, suggesting that it results from the activation of GABAA receptors after the release of endogenous GABA. We suggest that blockage is caused mainly by shunting within the caudal axon and that motor command circuits use this mechanism to disconnect the rostral and caudal compartments of the central axon, which allows the two parts of the neuron to perform different functions during movement.
Key words: primary afferents; presynaptic inhibition; antidromic firing; mastication; central pattern generation; action potential block
Introduction
It is generally assumed that the axonal arbor of vertebrate neurons conducts action potentials without modulation over most of their length. In primary afferent neurons, spikes normally flow from the peripheral branch of the axon, in which they are generated toward the soma and central branch. However, in many of these neurons, modulation is known to take place at presynaptic terminals, in which GABA-induced depolarization inhibits local synaptic transmission (Cattaert et al., 1992
, 1994
Evidence of this comes from our recent work on primary afferents that innervate the spindles of jaw-closing muscles. In contrast to other primary afferents, their cell bodies are located in the trigeminal mesencephalic nucleus (NVmes) and not in a dorsal root ganglion. Furthermore, their somata receive synaptic inputs and are electrotonically coupled through gap junctions (Lazarov, 2002
View larger version (22K):[in this window]
[in a new window]
Figure 1. Functional compartmentalization of jaw-closing muscle spindle afferents (from Kolta et al., 1995
Here we test the hypothesis that the decoupling of the two parts of the axonal tree is controlled by GABAergic synapses on the axonal trunk.
Materials and Methods
We began by applying GABA to the axonal trunk to see whether this would prevent invasion of the cell body by action potentials generated in the caudal axon. We used an in vitro brainstem slice preparation that contains the somata and central axons of trigeminal muscle spindle afferents that were labeled by injections of DiIC18(3) into the masseter muscles of rats at birth.
Preparation of slices. Figure 2A shows a sagittal drawing of the brainstem with an outline of the cell body and the axonal branches of a trigeminal muscle spindle primary afferent neuron modified from Dessem and Taylor (1989)
View larger version (72K):[in this window]
[in a new window]
Figure 2. Illustration of the preparation used for recordings. A, Sagittal drawing of the brainstem showing a trigeminal muscle spindle primary afferent neuron modified from Dessem and Taylor (1989)
To visualize the cells from which to record, crystals of the carbocyanine dye DiI C18 ([1,1'-dioctadecyl-3,3,3',3'-tetra-methylindocarbo-cyanine perchlorate]; Molecular Probes, Eugene, OR) were inserted in the masseter muscles of cryoanesthetized rat pups (0-2 d) and allowed to diffuse for 1-3 weeks before slice preparation. Nine- to 28-d-old Sprague Dawley rats (Charles River, Montreal, Quebec, Canada) were anesthetized by methoxyflurane inhalation (Metofane; Janssen Pharmaceuticals, North York, Ontario, Canada) and decapitated. The brainstem was dissected, cooled in oxygenated ice-cold (4°C) modified artificial CSF (aCSF) (in mM: 225 sucrose, 5 KCl, 1.25 KH2PO4, 4 MgSO4, 0.2 CaCl2, 20 NaHCO3, and 10 D-glucose), and embedded in agar (Aghajanian and Rasmussen, 1989
Electrophysiology. The slices were viewed with an epifluorescence microscope (Nikon, Tokyo, Japan). Figure 2B shows the labeling of trigeminal afferents (NVmes) and motoneurons (NVmt), as well as facial motoneurons (NVII) obtained by the dye injections. DiI-labeled cell bodies of masseteric spindle afferents in NVmes were targeted for recording with glass microelectrodes (80-200 M
) filled with 2% Neurobiotin dissolved in potassium acetate (1 and 3 M). The recording (R) and stimulating (S) positions are indicated on the schematic drawing of the slice in Figure 2B. A diagrammatic neuron is drawn in red to help visualize how these relate to the axonal course. Data were recorded through a bridge circuit with an Axoclamp 2B amplifier (Axon Instruments, Foster City, CA) and sampled at 20 kHz, except when monitoring the effects of GABA over long periods. In these cases, the sampling rate varied from 1 to 10 kHz. Data were stored on disk and analyzed using pClamp 6-8 software (Axon Instruments). Antidromic action potentials were evoked by electrically stimulating the descending central axonal tract through bipolar twisted nichrome wire electrodes (25 µm diameter). The intensity and duration (0.05-0.3 msec) of pulses were gradually increased to establish the threshold of antidromic spikes, and stimulus intensity was set at twice threshold (50 µA to 10 mA). High-frequency following (100-250 Hz) was used to ensure that the elicited spikes resulted from direct activation of the neuron. Spike onset latencies and amplitudes were measured. All quantitative data are expressed as mean ± SE. Differences between measures were compared with Student's paired t test (SigmaStat software; SPSS, Chicago, IL) and were considered to be significant if the probability of
-type error was <0.05. Correlations between variables were established with Pearson's correlation test and linear regression.
Drug application. GABA (1, 10, and 50 mM) and muscimol (50 µM) were dissolved in Fast Green-containing normal aCSF or calcium-free aCSF. Small drops of 50-200 µm diameter (0.6-4 nl) were injected beneath the surface of the slice by pressure ejection (pulse duration, 20-50 msec) from a glass micropipette (tip diameter, ~5 µm) using a Picospritzer (General Valve, Fairfield, NJ). Figure 2C shows a photomicrograph of a brainstem slice showing the diameter of an effective drop of GABA (circle) in relation to R and S. Picrotoxin (50 µM) was applied to the bath with a syringe pump.
Labeling. Some somata of the recorded jaw-closing spindle afferents were filled with Neurobiotin. Depolarizing current pulses (1.0-1.5 nA, 1 Hz, 500 msec duration) were passed through the recording electrode for 20-30 min to eject Neurobiotin. At the end of the experiment, the slices were fixed in 4% paraformaldehyde in 0.1 M phosphate buffer (PB). Neurobiotin was revealed using standard procedures and the ABC kit (Vector Laboratories, Burlingame, CA).
Immunohistochemistry. In five experiments, animals that have been injected with crystals of DiI (see above) were perfused, first with saline PB (9% PBS) and then with a fixative solution containing 2% paraformaldehyde and 0.1% glutaraldehyde in 0.1 M PBS. Their brainstem was extracted and immersed in the fixative solution containing, in addition, 30% sucrose until it sank. It was then sectioned in 80- to 100-µm-thick slices on a sliding freezing microtome. In two other experiments, 300-µm-thick slices were prepared as described above (see section on preparation of slices) and immersed in a fixative solution containing 2% paraformaldehyde and 0.1% glutaraldehyde in 0.1 M PB for 24 hr. In all experiments, the sections were rinsed and incubated with a polyclonal rabbit anti-GABA antibody (1:200 and 1:500; Sigma, St. Louis, MO) or with a polyclonal rabbit anti-glutamate decarboxylase (GAD) antibody (1:1000; Chemicon, Temecula, CA) for 36 hr. The primary antibody was revealed with a goat-anti-rabbit secondary antibody conjugated to Alexa 633 or to Alexa 488 (1:100; Molecular Probes). After several rinses, the sections were mounted with GelMount (Biomeda, Foster City, CA) and examined using a multiphoton confocal microscope (excitation wavelengths of 488, 633, and 543 nm for Alexa Fluor 488, Alexa Fluor 633, and DiI respectively; emission filters: band pass 500-550 for Alexa 488, low pass 650 for Alexa 633, and low pass 560 for DiI when combined with Alexa 488 or band-pass 565-615 for DiI combined with Alexa 633).
Results
Close apposition of immunoreactive GABAergic fibers and central axons
We combined immunocytochemistry against GABA and GAD with confocal imaging in an attempt to localize contacts made by GABAergic fibers onto axons of DiI-labeled afferents. In four of four experiments with GABA and three of three experiments with GAD, immunoreactive boutons (Fig. 2D,E, green boutons) were seen in close apposition (white arrows) to large labeled afferent stem axons (Fig. 2D,E, red).
Axonal application of GABA impedes propagation of antidromic action potential
Recordings were made from 77 neurons in NVmes, and 17 cells filled with Neurobiotin were successfully recovered. All had the typical pseudo-unipolar morphology of primary afferent with a single process emerging from a round or ovoid cell body (Fig. 2C, inset). The cells had an average resting membrane potential of
57 ± 1 mV and an input resistance of 30 ± 2 M
Antidromic action potentials were elicited by electrical stimulation of the descending tract at the level of the SupV (n = 57), the IntV (n = 11), the ventral NVmes (n = 7), and the NVmt (n = 6). The responses obtained were considered as antidromic on the basis of four criteria. First, they were all-or-none responses that did not appear to arise from an underlying EPSP, and this was confirmed by hyperpolarizing the cell until the spike was abolished. Second, all occurred at very short and constant latencies (mean, 0.63 ± 0.02 msec; minimum, 0.4 and maximum, 1.1 msec). Neurons in which stimulation caused spikes with latencies above 1.2 msec or that were of variable latency were not included in the analysis. Third, all responses followed high-frequency (100-250 Hz) stimulation without alteration. Finally, they were not affected by removal of Ca2+ from the medium in 12 of 12 cases tested.
GABA was ejected along the axonal tract of 64 cells. In 22 cases (34%), GABA abruptly abolished the spikes, with no concomitant change in membrane potential in 20 of them (Fig. 3A). This occurred within seconds and lasted from 0.5 sec to 2 min. A block was also produced by pressure ejection of muscimol (50 µM), a GABAA agonist (n = 2; data not shown), and it was reversed by bath application of picrotoxin (50 µM), a GABAA receptor antagonist (n = 3) (Fig. 3A). GABA and muscimol were effective in Ca2+-free, high-magnesium aCSF (n = 2 for each), suggesting that they were acting directly on the axon of the recorded neuron.
View larger version (18K):[in this window]
[in a new window]
Figure 3. Block of conduction of antidromic action potentials. A, Antidromic potentials elicited by stimulation of the descending tract at the level of IntV (Control) were abolished by pressure application of GABA (1 mM) on the axon (GABA). After recovery (Recovery), bath application of picrotoxin (50 µM) prevented the effect of GABA (GABA+PTX). B, Application of GABA (10 mM; arrow) along the axon of another neuron elicited spikes, but this did not stop the propagation of antidromic potentials evoked by electrical stimulation (*). C, Stimulation of the SupV alone had no effect on the soma of a third neuron (Control), but it abolished antidromic spikes caused by stimulation of the NVmt (Control) when the conditioning-test (C-T) interval was 2 msec but not 5 msec. D, Blockage of antidromic spikes evoked by stimulation of the medial SupV (mSupV), after stimulation of the lateral SupV (latSupV), was prevented by bath application of picrotoxin (50 µM) (C-T 2 msec interval PTX). Stimulation of the lateral SupV by itself had no detectable effect. Calibration bars in A apply to C and D. All panels present five superposed traces in A and C and four in D.
It has been suggested that presynaptic depolarization of axonal terminals could cause conduction failure at axonal branch points (Henneman et al., 1984
In a second group of 16 neurons (25% of total), GABA applications to the axon did not block the spikes, but it did reduce their amplitude significantly (
View larger version (21K):[in this window]
[in a new window]
Figure 4. Differences between somatic and axonal applications of GABA that cause depolarization. A, GABA (10 mM) applied to the axon decreased spike amplitude and slightly depolarized the cell (4 mV) after 5 sec, but there was no significant correlation between depolarization and change in amplitude (n = 13 cells) (B). C, GABA (10 mM) applied to the soma depolarized another cell (12 mV) and gradually decreased spike amplitude and increased its duration. D, Depolarization and change in amplitude were strongly correlated (n = 12 cells). 1, Resting membrane potential; 2, peak of control spike. Antidromic spikes were evoked by stimulation of the SupV.
We tried to reproduce the effects of direct GABA application by activation of local circuits that might release GABA under physiological conditions. Conditioning pulses (0.1-0.3 msec duration) were delivered to areas that are active during fictive mastication and that are known to contain GABAergic neurons (the intertrigeminal area, the supratrigeminal area, the trigeminal principal sensory nucleus, the parvocellular reticular formation, and the nucleus pontis caudalis) (Li et al., 1996
Somatic applications of GABA produce different effects from axonal applications
GABA was applied to the soma of 21 neurons to ensure that the effects of axonal applications were not attributable to diffusion to the cell bodies. GABA depolarized the cells (2-17 mV in 19 of 21 cells) and decreased their input resistance by 9-58% (in five of five cells). In contrast, no significant changes of somatic input resistance were detected during axonal GABA application (n = 26). Unlike the axonal applications, somatic GABA rarely abolished antidromic spikes (2 of 21). Instead, it reduced their amplitude by 24 ± 4 mV (14 of 21; p < 0.001) (Fig. 4C) and increased their duration by 0.46 ± 0.08 msec; (14 of 21; p < 0.05). This also contrasts with axonal applications in which reduction in spike amplitude was not associated with changes in duration, latency, rise, or decay times. Furthermore, there was a strong relationship between changes in membrane potential and spike amplitude (r = 0.858; p < 0.001) (Fig. 4D) with somatic applications. These effects were present in Ca2+-free, high-Mg2+ aCSF (two of two cells tested; data not shown). In all cases, the recovery was gradual and was rarely complete until 1 min after the application.
Discussion
The transmission of action potentials along the caudal central axon of trigeminal muscle spindle afferents seems to be regulated during mastication (Kolta et al., 1995
This is the first description of a chemical mechanism powerful enough to completely block action potential propagation in large axons, although GABA has been shown to modify spikes in crayfish sensory afferents when it is applied near the first major branch point. The effect is a reduction in the amplitude of incoming action potentials through a combination of depolarization and shunting that depends on increased chloride conductance (Cattaert and el Manira, 1999
We suggest that modulation of conduction along trigeminal spindle afferent axons during mastication allows two regions of the axon and their respective collaterals to fire independently from each other and to transmit different messages to their postsynaptic targets during one phase of the movement (Fig 1). As a result, the central axon may become a premotoneuron, carrying signals from the CPG via a set of presynaptic terminals to motoneurons, whereas the rostral portion of the neuron provides feedback from its receptors, although even this is phasically gated by the CPG.
Although this is the first direct evidence of a new mechanism that controls action potential traffic in vertebrate neurons, it is probably not unique to the trigeminal sensory system, and its presence may explain the results of others. For instance, Wall and his colleagues showed that action potentials propagate easily along the large ascending branches of dorsal column afferents studied in vitro, but they often failed to penetrate the thin branches that travel caudally. This tonic blockade could be lifted by picrotoxin, a GABAA receptor antagonist (Wall, 1994
FOOTNOTES Received Sept. 9, 2002; revised Dec. 2, 2002; accepted Jan. 2, 2003.
This work was supported by the Canadian Institutes for Health Research.
Correspondence should be addressed to Dr. Arlette Kolta, Université de Montréal, Pavillon Paul Desmarais, C.P. 6128, Succursale Centre Ville, Montréal, Québec H3C 3J7, Canada. E-mail: arlette.kolta{at}umontreal.ca.
References
- Aghajanian GK, Rasmussen K (1989) Intracellular studies in the facial nucleus illustrating a simple new method for obtaining viable motoneurons in adult rat brain slices. Synapse 3:331-338[ISI][Medline].
- Bae YC, Nakagawa S, Yasuda K, Yabuta NH, Yoshida A, Pil PK, Moritani M, Chen K, Nagase Y, Takemura M, Shigenaga Y (1996) Electron microscopic observation of synaptic connections of jaw-muscle spindle and periodontal afferent terminals in the trigeminal motor and supratrigeminal nuclei in the cat. J Comp Neurol 374:421-435[ISI][Medline].
- Bevengut M, Clarac F, Cattaert D (1997) Antidromic modulation of a proprioceptor sensory discharge in crayfish. J Neurophysiol 78:1180-1183
[Abstract/Free Full Text] .- Bourque M-J, Kolta A (2001) Properties and interconnections of trigeminal interneurons of the lateral pontine reticular formation in the rat. J Neurophysiol 86:2583-2596
[Abstract/Free Full Text] .- Cattaert D, el Manira A (1999) Shunting versus inactivation: analysis of presynaptic inhibitory mechanisms in primary afferents of the crayfish. J Neurosci 19:6079-6089
[Abstract/Free Full Text] .- Cattaert D, el Manira A, Clarac F (1992) Direct evidence for presynaptic inhibitory mechanisms in crayfish sensory afferents. J Neurophysiol 67:610-624
[Abstract/Free Full Text] .- Cattaert D, el Manira A, Clarac F (1994) Chloride conductance produces both presynaptic inhibition and antidromic spikes in primary afferents. Brain Res 666:109-112[ISI][Medline].
- Cattaert D, Libersat F, el Manira A (2001) Presynaptic inhibition and antidromic spikes in primary afferents of the crayfish: a computational and experimental analysis. J Neurosci 21:1007-1021
[Abstract/Free Full Text] .- Dessem D, Taylor A (1989) Morphology of jaw-muscle spindle afferents in the rat. J Comp Neurol 282:389-403[ISI][Medline].
- Donga R, Lund JP (1991) Discharge patterns of trigeminal commissural last-order interneurons during fictive mastication in the rabbit. J Neurophysiol 66:1564-1578
[Abstract/Free Full Text] .- Dubuc R, Cabelguen J-M, Rossignol S (1985) Rhythmic antidromic discharges of single primary afferents recorded in cut dorsal root filaments during locomotion in the cat. Brain Res 359:375-378[ISI][Medline].
- Eguibar JR, Quevedo J, Jiménez I, Rudomin P (1994) Selective cortical control of information flow through different intraspinal collaterals of the same muscle afferent fiber. Brain Res 643:328-333[Medline].
- Eguibar JR, Quevedo J, Rudomin P (1997) Selective cortical and segmental control of primary afferent depolarisation of single muscle afferents in the cat spinal cord. Exp Brain Res 113:411-430[ISI][Medline].
- Gossard JP (1996) Control of transmission in muscle group 1A afferents during fictive locomotion in the cat. J Neurophysiol 76:4104-4112
[Abstract/Free Full Text] .- Gossard JP, Cabelguen J-M, Rossignol S (1991) An intracellular study of muscle primary afferents during fictive locomotion in the cat. J Neurophysiol 65:914-926
[Abstract/Free Full Text] .- Gossard JP, Bouyer L, Rossignol S (1999) The effects of antidromic discharges on orthodromic firing of primary afferents in the cat. Brain Res 825:132-145[ISI][Medline].
- Graham B, Redman S (1994) A simulation of action potentials in synaptic boutons during presynaptic inhibition. J Neurophysiol 71:538-549
[Abstract/Free Full Text] .- Henneman E, Luscher HR, Mathis J (1984) Simultaneously active and inactive synapses of single Ia fibres on cat spinal motoneurones. J Physiol (Lond) 352:147-161
[Abstract/Free Full Text] .- Inoue T, Masuda Y, Nagashima T, Yoshikawa K, Morimoto T (1992) Properties of rhythmically active reticular neurons around the trigeminal motor nucleus during fictive mastication in the rat. Neurosci Res 14:275-294[ISI][Medline].
- Kolta A, Lund JP, Westberg KG, Clavelou P (1995) Do muscle spindle afferents act like interneurons during mastication? Trends Neurosci 18:441[ISI][Medline].
- Kolta A, Westberg KG, Lund JP (2000) Identification of brainstem interneurons projecting to the trigeminal motor nucleus and adjacent structures in the rabbit. J Chem Neuroanat 19:175-195[ISI][Medline].
- Lamotte dB, Meunier C, Monnet ML, Jami L, Zytnicki D (1998) Reduction of presynaptic action potentials by PAD: model and experimental study. J Comput Neurosci 5:141-156[ISI][Medline].
- Lazarov NE (2002) Comparative analysis of the chemical neuroanatomy of the mammalian trigeminal ganglion and mesencephalic trigeminal nucleus. Prog Neurobiol 66:19-59[ISI][Medline].
- Li YQ, Takada M, Kaneko T, Mizuno N (1996) Gabaergic and glycinergic neurons projecting to the trigeminal motor nucleus: a double labeling study in the rat. J Comp Neurol 373:498-510[ISI][Medline].
- Lomeli J, Quevedo J, Linares P, Rudomin P (1998) Local control of information flow in segmental and ascending collaterals of single afferents. Nature 395:600-604[Medline].
- Lomeli J, Castillo L, Linares P, Rudomin P (2000) Effects of PAD on conduction of action potentials within segmental and ascending branches of single muscle afferents in the cat spinal cord. Exp Brain Res 135:204-214[Medline].
- Luo P, Li J (1991) Monosynaptic connections between neurons of trigeminal mesencephalic nucleus and jaw-closing motoneurons in the rat: an intracellular horseradish peroxidase labeling study. Brain Res 559:267-275[ISI][Medline].
- Pinault D (1995) Backpropagation of action potentials generated at ectopic axonal loci: hypothesis that axon terminals integrate local environmental signals. Brain Res Rev 21:42-92[Medline].
- Segev I (1990) Computer study of presynaptic inhibition controlling the spread of action potentials into axonal terminals. J Neurophysiol 63:987-998
[Abstract/Free Full Text] .- Turman Jr JE, Chandler SH (1994) Immunohistochemical evidence for GABA and glycine-containing trigeminal premotoneurons in the guinea pig. Synapse 18:7-20[ISI][Medline].
- Wall PD (1994) Control of impulse conduction in long range branches of afferents by increases and decreases of primary afferent depolarisation in the rat. Eur J Neurosci 6:1136-1142[ISI][Medline].
- Wall PD (1995) Do nerve impulses penetrate terminal arborizations? A pre-presynaptic control mechanism. Trends Neurosci 18:99-103[ISI][Medline].
- Wall PD, Bennett DLH (1994) Postsynaptic effects of long-range afferents in distant segments caudal to their entry point in rat spinal cord under the influence of picrotoxin or strychnine. J Neurophysiol 72:2703-2713
[Abstract/Free Full Text] .- Wall PD, McMahon SB (1994) Long range afferents in rat spinal cord. III. Failure of impulse transmission in axons and relief of the failure after rhizotomy of dorsal roots. Philos Trans R Soc Lond B Biol Sci 343:211-223[ISI][Medline].
- Westberg KG, Kolta A, Clavelou P, Sandstrom G, Lund JP (2000) Evidence for functional compartmentalization of trigeminal muscle spindle afferents during fictive mastication in the rabbit. Eur J Neurosci 12:1145-1154[ISI][Medline].
Copyright © 2003 Society for Neuroscience 0270-6474/03/2362002-06$05.00/0
This article has been cited by other articles:
R. Khanbabaie, A. S. Mahani, and R. Wessel
Contextual Interaction of GABAergic Circuitry With Dynamic Synapses
J Neurophysiol, April 1, 2007; 97(4): 2802 - 2811.
[Abstract] [Full Text] [PDF]
P. M. Lang, G. Moalem-Taylor, D. J. Tracey, H. Bostock, and P. Grafe
Activity-Dependent Modulation of Axonal Excitability in Unmyelinated Peripheral Rat Nerve Fibers by the 5-HT(3) Serotonin Receptor
J Neurophysiol, December 1, 2006; 96(6): 2963 - 2971.
[Abstract] [Full Text] [PDF]
M. Saito, Y. Murai, H. Sato, Y.-C. Bae, T. Akaike, M. Takada, and Y. Kang
Two Opposing Roles of 4-AP-Sensitive K+ Current in Initiation and Invasion of Spikes in Rat Mesencephalic Trigeminal Neurons
J Neurophysiol, October 1, 2006; 96(4): 1887 - 1901.
[Abstract] [Full Text] [PDF]
S. Mejia-Gervacio and A. Marty
Control of interneurone firing pattern by axonal autoreceptors in the juvenile rat cerebellum
J. Physiol., February 15, 2006; 571(1): 43 - 55.
[Abstract] [Full Text] [PDF]
S. Rossignol, R. Dubuc, and J.-P. Gossard
Dynamic Sensorimotor Interactions in Locomotion
Physiol Rev, January 1, 2006; 86(1): 89 - 154.
[Abstract] [Full Text] [PDF]
C. G. Evans, A. Romero, and E. C. Cropper
Inhibition of Afferent Transmission in the Feeding Circuitry of Aplysia: Persistence Can Be as Important as Size
J Neurophysiol, May 1, 2005; 93(5): 2940 - 2949.
[Abstract] [Full Text] [PDF]
I. Skaliora, T. P. Doubell, N. P. Holmes, F. R. Nodal, and A. J. King
Functional Topography of Converging Visual and Auditory Inputs to Neurons in the Rat Superior Colliculus
J Neurophysiol, November 1, 2004; 92(5): 2933 - 2946.
[Abstract] [Full Text] [PDF]
D. Verdier, J. P. Lund, and A. Kolta
Synaptic Inputs to Trigeminal Primary Afferent Neurons Cause Firing and Modulate Intrinsic Oscillatory Activity
J Neurophysiol, October 1, 2004; 92(4): 2444 - 2455.
[Abstract] [Full Text] [PDF]
J.-M. Goaillard, D. J. Schulz, V. L. Kilman, and E. Marder
Octopamine Modulates the Axons of Modulatory Projection Neurons
J. Neurosci., August 11, 2004; 24(32): 7063 - 7073.
[Abstract] [Full Text] [PDF]
D. Bucher, V. Thirumalai, and E. Marder
Axonal Dopamine Receptors Activate Peripheral Spike Initiation in a Stomatogastric Motor Neuron
J. Neurosci., July 30, 2003; 23(17): 6866 - 6875.
[Abstract] [Full Text] [PDF]
This Article Abstract 
Full Text (PDF) Submit an eLetter Alert me when this article is cited Alert me when eLetters are posted Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in ISI Web of Science Similar articles in PubMed Alert me to new issues of the journal Download to citation manager 
Citing Articles Citing Articles via HighWire Citing Articles via ISI Web of Science (21) Citing Articles via Google Scholar Google Scholar Articles by Verdier, D. Articles by Kolta, A. Search for Related Content PubMed PubMed Citation Articles by Verdier, D. Articles by Kolta, A.
|
|
|
|
 |
|