Characterization of the Circuits That Generate Spontaneous Episodes of Activity in the Early Embryonic Mouse Spinal Cord

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The Journal of Neuroscience, January 15, 2003, 23(2):587-600

Characterization of the Circuits That Generate Spontaneous Episodes of Activity in the Early Embryonic Mouse Spinal Cord
M. Gartz Hanson and Lynn T. Landmesser
Department of Neurosciences, Case Western Reserve University, School of Medicine, Cleveland, Ohio 44106-4975

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

In the developing nervous system, patterned spontaneous activity affects a variety of developmental processes. Thus, it isimportant to identify the earliest time that such activity occursand to characterize the underlying circuitry. In isolated mousespinal cord-limb preparations, highly rhythmic spontaneous activityoccurred as early as embryonic day 11 (E11)-E12, when many lumbosacralmotoneurons were still migrating and extending their peripheralprojections. This activity required both electrical and chemicaltransmission, and acetylcholine, rather than glutamate, providedthe main excitatory drive. Our data are consistent with motoneuronsthemselves playing a critical role in generating such activityby making excitatory connections on each other and on GABAergicinterneurons via dihydro- $beta$ -erythroidine hydrobromide (DH $beta$ E)-insensitivenicotinic receptors. This resulted in the generation of localbursts. Consistent with these observations, E12-E12.5 mouse motoneuronsretrogradely labeled by HRP were observed to have extensive axoncollaterals that projected locally within the lateral motor columnand to interneuron-containing regions dorsal and medial of thelateral motor column. Cholinergic axons, presumably from motoneurons,were also observed in the ventral and lateral funiculi. However,for local bursts to propagate throughout the cord, a second DH $beta$ E-sensitivecholinergic pathway that also involved glycinergic interneuronswas required. This circuit characterization should facilitatethe use of genetic mutations that alter specific subpopulationsof interneurons or cholinergic transmission to determine how modifyingdifferent aspects of this early activity affects subsequent developmentof the spinal motorcircuit.

Key words: motoneuron; interneuron; motor; cholinergic; glycinergic; GABAergic; gap junctions; development

  Introduction

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Rhythmic spontaneous episodes of activity are widespread in the developing vertebrate CNS, occurring in regions involved inthe generation of motor patterns, the processing of visual information,and learning and memory (Hamburger et al., 1965; Meister et al.,1991; Katz and Shatz, 1996; Chub and O'Donovan, 1998; Garaschuket al., 1998; Kandler and Katz, 1998; Milner and Landmesser, 1999)(for review, see Feller, 1999; O'Donovan, 1999). In the developingvisual system, spontaneous episodes of activity are importantin the formation and refinement of neuronal circuits, includingaxonal segregation into specific layers in the lateral geniculatenucleus (Shatz, 1996; Penn et al., 1998; Stellwagen and Shatz,2002) and in the organization of the visual cortex (Weliky andKatz, 1999). Within the ferret eye, spontaneous activity propagatesacross distinct domains of the retina as waves (Wong et al., 1993,1995; Feller et al., 1996, 1997). Early in retina development[postnatal day 0 (P0)-P9 ferret and embryonic day 8 (E8)-E11 chick],acetylcholine (ACh) provides the excitatory drive for these waves(Feller et al., 1996; Catsicas et al., 1998; Penn et al., 1998)through complex interactions between amacrine cells and retinalganglion cells (Zhou, 1998). As the retina develops (E13-E18 chick),this excitatory drive switches from ACh to glutamate (Wong, 1999;Sernagor et al., 2000).

Excitatory spontaneous activity may play similar roles in the development of the spinal motor circuit. For instance, in theearly chick spinal cord (E4-E5), at a stage of development whenaxons are still growing to their targets, cord circuits generatehighly rhythmic episodes of spontaneous activity, and cholinergicand GABAergic inputs have been shown to modulate the rhythm andpattern of these episodes (Milner and Landmesser, 1999). At laterstages (E9), well after target innervation and the formation ofthe neuromuscular junction (Chub and O'Donovan, 1998; Usiak andLandmesser, 1999), glutamatergic and GABAergic interneurons providemuch of the excitatory drive for spontaneous bursting (Sernagoret al., 1995; Chub and O'Donovan, 1998). However, the motoneuronsthemselves could also contribute to spontaneous episodes of activityby activating interneurons via their axon collaterals. In factin the E10-E12 chick, cholinergic collaterals have been shownto activate a Renshaw-like group of interneurons that may be responsiblefor subsequently activating cells throughout the circuit (Wennerand O'Donovan, 1999, 2001). Consistent with this idea, motoneuronsappeared to depolarize slightly before the interneurons in thisE10 circuit; however, pharmacological blockade of transmissionfrom the collaterals to the Renshaw-like interneurons did notblock spontaneous bursting (Ritter et al., 1999). Thus in theE10 chick, motoneurons may normally contribute to but are notrequired for the synaptic drive that generates spontaneousepisodes.

In the E12 mouse spinal motor circuit, a stage when motoneurons are still growing to their peripheral targets (Jones, 1979),we show that cholinergic, glycinergic, and GABAergic input, ratherthan glutamate, drive the circuit and that all are excitatory.We further show that motoneurons via nicotinic transmission playa critical role in generating spontaneous activity with participatingGABAergic interneurons by initiating localized bursting episodes.However, for such episodes to propagate throughout the cord, anadditional circuit that uses cholinergic and glycinergic as wellas electrical transmission isrequired.

  Materials and Methods

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

In vitro spinal cord-hindlimb preparation. This protocol is a modification of the chicken in vitro spinal cord-hindlimb preparationdescribed previously (Landmesser and O'Donovan, 1984). C57BL/J6mouse embryos between the ages of E11.5 and E13 or stage 25 chickembryos were decapitated, eviscerated, and placed in cool oxygenatedTyrode's solution. A ventral laminectomy was performed to exposethe spinal cord and allow oxygenation. Careful removal of theskin and surrounding limb connective tissue with fine tungstenneedles exposed motor nerve trunks. After dissection, the Tyrode'ssolution was warmed to 30°C for the duration of the experiment.Nerve recordings were performed using extra fine-tip suction electrodespulled from polyethylene tubing (PE-190; Clay Adams, Parsippany,NJ). A continuous negative pressure was used to draw the tipsof growing muscle nerves into the electrode, producing a tightseal (Fig. 1A). Activity was recorded continuously either on ananalog tape recorder (Vetter, Rebersburg, PA) with subsequentdigital conversion and storage on the computer or directly onthe computer with Axoscope 8 (Axon Instruments, Foster City, CA).It was simultaneously displayed on an oscilloscope (R5030; Tektronix,Beaverton, OR) and chart recorder (Gould Inc, Cleveland, OH).To produce an episode of activity, spinal cords were stimulatedwith suction electrodes at different sites (see Fig. 1A) witha Grass (Quincy, MA) S48 stimulator that was isolated from groundwith a stimulator isolation unit (GrassPSIU6B).

Drug treatments. Neurochemicals and receptor blockers were bath-applied to the in vitro spinal cord-hindlimb preparation usinga pump that circulated oxygenated Tyrode's solution over the preparation.Each drug was evaluated either alone or in combination with otherdrugs for its effect on spontaneous bursting activity. Drugs wereapplied for a minimum of 20 min before assessing their effectivenesson spontaneous activity by quantifying the change in episode frequency,number of bursts per episode, and burst structure; however, inmany cases, effects of the drugs were immediately evident. Asshown in Figure 1B, episodes of bursting activity, which consistedof one or more closely spaced bursts (within seconds of each other),occurred at regular intervals of $>=$ 1 min. This interepisode intervalwas used to quantify the frequency of episodes. The interepisodeinterval was defined as the time between the end of one episodeand the beginning of the next. When comparing different drug treatments, $>=$ 10 episodes were measured, and the data were displayed as mean± SE. Except where indicated, a given drug treatment was performedon two or more embryos with similar results, and, in most cases,drugs were washed out until burst parameters returned to controlvalues (several minutes to 1-2 hr depending on the drug). Significanceof data was evaluated by Student's t test, which determined thep value (SigmaPlot 2.0; Jandel Scientific, Corte Madera, CA);p < 0.05 was consideredsignificant.

A list of the drugs used includes the following: cholinergic receptor blockers d-tubocurarine (dTC), atropine, dihydro- $beta$ -erythroidinehydrobromide (DH $beta$ E), mecamylamine, and methyllycoconitine (MLA);cholinergic agonist nicotine; GABA receptor blockers bicucullineand phaclofen; GABA agonist GABA; glutamate receptor blockersAPV and CNQX; glutamate agonists glutamate and kainate; Gly receptorantagonist strychnine; and gap junction blocker carbenoxolone.The effects of low-calcium (0.2 mM), high-magnesium (7 mM) Tyrode'ssolution or normal calcium (2 mM), high-magnesium (12 mM) Tyrode'ssolution were tested to determine the contribution of synapticinput on spontaneousactivity.

HRP back-labeling of motoneurons. E12.5 mouse spinal cords were prepared as described above for physiological recordings.Motor roots were injected with 10% horseradish peroxidase andincubated for 6 hr at 30°C in oxygenated Tyrode's solution toallow for retrograde transport to motoneurons. The embryos werefixed in 2% glutaraldehyde overnight and then washed with PBS.The tissue was embedded in agarose and sectioned at 50 µm usinga vibratome (OTS 3000; Electron Microscope Sciences). The sectionswere incubated with DAB (0.5 mg/ml) in Tris buffer containing0.03% hydrogen peroxide for 45 min, dehydrated using a seriesof ethanol washes (70, 90, and 100%), cleared in xylene, and thenmounted between two coverslips inPermount.

Immunohistochemistry. Embryonic day 12.5 mouse embryos were prepared as stated above. The embryos were then fixed in 3.7%formaldehyde for 1 hr at room temperature. The embryos were washedin 5% sucrose and PBS for 1 hr, placed in 30% sucrose and PBSovernight at 4°C, placed in a 1:1 mixture of 60% sucrose and tissue-freezingmedium (Triangle Biomedical Sciences, Durham, NC), and frozenin dry ice-cooled isopentane, before cryostat sectioning at 18µm at $-$ 30°C (Cryocut 1800; Leica, Nussloch, Germany). The sectionswere incubated with antibodies against the vesicular acetylcholinetransporter (anti-VCAT; V5387; Sigma, St. Louis, MO) and in somecases colabeled with antibodies against choline acetyltransferase(anti-ChAT; AB1448; Chemicon, Temecula, CA) to identify cholinergicneurons for 1 hr sequentially, incubated with Alexa-488 secondaryantibody (Molecular Probes, Eugene, OR) and biotin-conjugatedsecondary antibody plus avidin-rhodamine (Vector Laboratories,Burlingame, CA), respectively, and then rinsed and mounted usinga ProLong Antifade kit (MolecularProbes).

Image acquisition. Imaging was performed with a digital camera (Olympus MagnaFire) using the MagnaFire 2.0 software. For HRP-labeledmotoneurons, neurites from particular motoneurons were first identifiedusing a differential interference contrast condenser on an invertedmicroscope (Nikon Diaphot 300). Images were captured at severaldifferent focal planes (upright microscope, 63× oil, Nikon Microphot-FX).The images were then overlaid and merged in the z-axis using ImageProPlus software (MediaCybernetics, Silver Spring,MD).

  Results

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Before and during innervation of peripheral targets, rhythmic spontaneous activity in the mouse spinal cord is mediated by electrical and chemical transmission

Although rhythmic spontaneous activity has been characterized in the early embryonic chicken spinal motor circuit (E4-E5;Milner and Landmesser, 1999), less data are available for thecorresponding developmental stages in the mouse (Branchereau etal., 2002). To characterize the rhythmic episodes of activitybetween E11 and E14 in the mouse, during which time motoneuronsare growing to and innervating their targets (Jones, 1979), tight-fittingsuction electrodes were attached to motor nerves in an in vitrospinal cord-hindlimb preparation (Fig. 1A) (for additional methods,see Landmesser and O'Donovan 1984; O'Donovan and Landmesser, 1987).These episodes of activity were highly rhythmic, with little variationin the interepisode intervals at a given developmental stage (Fig.1B,C). However, both the duration of the bursting episode (datanot shown but previously described by Branchereau et al., 2000)and interepisode intervals increased as the circuit matured (Fig.1C). Two types of spontaneous episodes were observed. Major episodespropagated throughout the cord, with both right and left sciaticnerves (data not shown) and sciatic and crural trunks (Fig. 1D)bursting approximately in-phase and are therefore defined as propagatingepisodes. Although infrequent (19 of 378 intervals), other episodeswere confined to local regions of the spinal cord. For example,the episode from the crural trunk (Fig. 1D, top trace, bracket)was not observed in the ipsilateral sciatic recording (bottomtrace). Therefore, we defined these as episodes that were confinedto the recorded nerve as local. Finally, unitary spikes occurredat a low frequency throughout the intervals (Fig. 1D), althoughthey tended to increase (data not shown) as the time of a burstingepisode approached. This has also been observed in E10 chick cord(Chub and O'Donovan, 2001), where this has been attributed tothe recovery of the circuit from depression caused by the precedingepisode.

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Figure 1. Characterization of spontaneous episodes of activity in the early developing mouse spinal motor circuit. A, Suction electrodes were placed on embryonic mouse motor nerves in an isolated spinal cord-hindlimb preparation. B, Spontaneous activity consisted of high-amplitude bursting episodes separated by interepisode intervals of several minutes. Interepisode intervals were very constant for each age but increased with the developmental stage examined (C; mean ± SE). D, Recordings from different nerves demonstrated that episodes throughout the lumbar spinal cord were generally in-phase. Rhythmic activity could be abolished when chemical transmission was blocked by high Mg²⁺ and low Ca²⁺ (7.0 and 0.2 mM; E) or when electrical transmission was blocked by the gap junction inhibitor carbenoxolone (100 µM; F).

Both electrical coupling and chemical transmission could contribute to the depolarization of motoneurons that produces theseearly rhythmic episodes of activity. To evaluate the importanceof chemical transmission, which is dependent on extracellularCa²⁺, the preparation was perfused in the presence of low Ca²⁺ (0.2 mM) and high Mg²⁺ (7.0 mM). This abolished the rhythmic episodes of activity (Fig.1E), consistent with the requirement of chemical transmissionfor the propagation of spontaneous episodes in the early (E12)mouse spinal cord circuit. It is also possible that lowering thecalcium concentrations could affect other processes, such as Ca²⁺-induced calcium release. This result is similar to that observedin the immature chick spinal motor circuit (E5; Milner and Landmesser,1999).

Although chemical transmission appeared necessary for rhythmic episodes of activity, electrical coupling between neurons mightalso contribute to the generation of these episodes. Althoughgap junction coupling of neurons is found in many regions of theCNS, its function during development is currently not well understood(Roerig and Feller, 2000). Nevertheless, electrical coupling appearscapable of synchronizing the bursting activity in embryonic zebrafishspinal cord (Saint-Amant and Drapeau, 2001). To determine whetherelectrical transmission affected the rhythmic episodes of activityin E12 embryonic mouse cord, carbenoxolone (100 µM), a gap junctioninhibitor (Draguhn et al., 1998; Nolan et al., 1999), was bath-applied.This abolished the rhythmic episodes within 15 min (n = 3) (Fig.1F), similar to the observation made in the E5 chick spinal cord(Milner and Landmesser, 1999). Another gap junction blocker, octanol(3 mM), also abolished activity (data not shown). These observationsare consistent with electrical coupling being required to generatespontaneous activity. However, such compounds have also been shownto affect other processes, such as in the inactivation of sodiumchannels (Elliot and Elliot, 1989). In summary, both gap junction-mediatedcoupling and chemical transmission appear necessary for the propagationof rhythmic episodes of activity in the early (E12) mouse spinalcordcircuit.

Rhythmic spontaneous activity requires cholinergic and glycinergic transmission but not glutamate

We next characterized the transmitters involved in the generation and propagation of the rhythmic episodes. In the maturespinal motor circuit, the main excitatory drive is from glutamatergicspinal interneurons, whereas inhibition is provided by glycinergicand GABAergic interneurons (Rekling et al., 2000). Therefore,endogenous glutamate, released by interneurons in the E12 mousemotor circuit, could drive circuit activity via NMDA or AMPA/kainatereceptors. However, the addition of CNQX, an AMPA/kainate receptorantagonist, APV, an NMDA receptor antagonist, or both had no affecton the rhythmic episodes of activity (Fig. 2A). Similar resultswere reported recently for the AMPA antagonist kynurenic acid(Branchereau et al., 2002) (for E15 rat, see Nishimaru et al.,1996). These data indicate that in contrast to the more maturecord circuit, glutamatergic transmission is not needed for spontaneousepisodes of activity at E12.

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Figure 2. Early embryonic spontaneous episodes of activity require glycinergic and cholinergic but not glutamatergic transmission. A, In the E12 spinal cord, glutamate receptor agonists and antagonists did not affect spontaneous activity. B, In contrast, many AChR antagonists (some considered general blockers and others directed against specific nicotinic subunit compositions; see Results for more detail) slowed the frequency of spontaneous episodes. However, bath application of DH $beta$ E (5 µM, a nicotinic antagonist with high sensitivity toward $alpha$ 3 $beta$ 2 and $alpha$ 4 $beta$ 4 receptors) abolished spontaneous episodes of activity (C). D, In the presence of GABA receptor antagonists, spontaneous activity persists; however, the GABA_A receptor antagonists bicuculline (50 µM) and picrotoxin (50 µM) decreased the frequency of the spontaneous episodes, whereas GABA_B receptor antagonists (Phaclofen, 100 µM; Hydrosaclofen, 50 µM) and GABA_C receptor antagonist (TPMPA, 100 µM) were without effect. The Gly receptor antagonist strychnine (Stryc, 5 µM) completely suppressed rhythmic episodes in the E12 mouse spinal cord (E) and greatly slowed the frequency of episodes in the stage 25 chicken spinal cord (F).

Cholinergic transmission plays a major role in the episodic activity in the maturing chick spinal motor circuit (Milner andLandmesser, 1999), and ACh could be released either from interneuronsor from motoneuron axon collaterals. It is generally acceptedthat motoneurons release ACh and that at later developmental stages,the rat cervical and lumbar cord contains cholinergic interneurons(Phelps et al., 1990). Endogenously released ACh from either sourcecould be acting via muscarinic receptors, a variety of nicotinicreceptors, or both. The latter, in which pharmacological and channelproperties are determined by their subunit composition, are widelyexpressed in the nervous system (Dwoskin and Crooks, 2001). However,a detailed characterization of the spatial expression patternsof the different receptor subtypes has not been performed duringearly mouse cord development. Therefore, we tested a variety ofcholinergic antagonists to see whether they affected rhythmicspontaneousactivity.

Most general as well as more specific (i.e., affecting specific subunit combinations) nicotinic ACh receptor (nAChR) antagonistsslowed the frequency of bursting activity, so that the interepisodeinterval (Fig. 2B) was significantly increased. The applicationof both low and high doses of general nAChR antagonists, suchas mecamylamine (1 and 20 µM) and dTC (5 and 10 µM), increasedthe time between episodes by approximately fourfold (Fig. 2B;p < 0.05). Similar effects were also seen with the addition ofthe neuromuscular nAChR antagonist decamethonium bromide, suggestingthe presence of $alpha$ 1 receptors (p < 0.05). However, the specific $alpha$ 7 nAChR antagonist MLA (1 µM) had no affect on spontaneous episodesof activity (p > 0.05). Interestingly, DH $beta$ E (5µM) rapidly andcompletely abolished the rhythmic episodes of activity (Fig. 2C).When propagating episodes were blocked with DH $beta$ E, local episodes(Fig. 1D) began to occur, although their amplitude and durationwere smaller, and they were less frequent compared with the controlepisodes (data not shown). These local episodes from sciatic andcrural nerves occurred randomly, were not synchronized throughoutthe cord (data not shown), and appear to represent the activationof local circuits. They will be discussed in more detail later.DH $beta$ E is a competitive antagonist of $beta$ 2 subunits in combinationwith $alpha$ 3 and $alpha$ 4 subunits. DH $beta$ E also has high affinity for $alpha$ 4 $beta$ 4nicotinic receptors (Dwoskin and Crooks, 2001). Muscarinic AChreceptors could also be playing a role in rhythmic spontaneousactivity. However, the muscarinic ACh receptor antagonist atropine(10 µM) had no affect on rhythmic spontaneous activity (p > 0.05).These data indicate that endogenously released ACh acting throughDH $beta$ E-sensitive nicotinic receptors plays a critical role in thegeneration of spontaneous bursting episodes in the early mousespinal motorcircuit.

As demonstrated above, cholinergic transmission was required for rhythmic spontaneous activity; however, the classically inhibitorytransmitters GABA and Gly have been shown to modulate transmissionin the maturing embryonic spinal cord (Sernagor et al., 1995;Nishimaru et al., 1996, Branchereau et al., 2002). Furthermore,it is known that both GABA and Gly can be excitatory at earlydevelopmental stages in various regions of the nervous system(Wu et al., 1992; Reichling et al., 1994; Chen et al., 1996; Owenset al., 1996). When the GABA_A receptor antagonists bicuculline(50 µM) (Fig. 2D) and picrotoxin (5 µM) were applied to E12 mousespinal cords, both increased interepisode intervals (2.8-foldincrease compared with control; p < 0.05) (Fig. 2D). However,phaclofen and hydrosaclofen, GABA_B receptor antagonists (Fig.2D), and 1,2,5,6-tetrahydropyridin-4-yl)methyl phosphinic acid(TPMPA) (Fig. 2D), a GABA_C receptor antagonist, had no effecton the rhythmic spontaneous activity (p > 0.05). These data indicatethat endogenously released GABA acting via GABA_A receptors contributesto the excitatory drive in the early circuit, but that it is notrequired for the generation of spontaneous episodes of activity.Similar affects of GABA were also found in the early chick spinalmotor circuit (E5; Milner and Landmesser, 1999).

To assess the effect of Gly, which is inhibitory in more mature cord circuits, we bath applied the Gly receptor antagoniststrychnine (1-5 µM). This dramatically increased the interepisodeintervals and completely abolished spontaneous bursting activitywithin 60 min (Fig. 2E; n = 5), indicating that at this developmentalstage, Gly is excitatory. Interestingly, during bath applicationof strychnine, multiple local episodes of smaller amplitude andduration occurred between episodes. Although propagating episodeswithin the left crural nerve and left sciatic nerve were foundto be in-phase with each other, local episodes were not in-phasewith each other (data not shown). However, they persisted afterpropagating episodes of activity were abolished. The effect ofinhibiting glycinergic transmission with strychnine was also testedin the E5 chick spinal cord. Although the intervals between episodesincreased considerably, they were never completely abolished (Fig.2F). Strychnine has also been shown to block nicotinic $alpha$ 7 receptors(Matsubayashi et al., 1998). However, because the $alpha$ 7 receptorantagonist MLA had no effect on spontaneous episodic activityin either the E5 chicken (Milner and Landmesser, 1999) or theE12 mouse (this study) (Fig. 2B), it is unlikely that the actionsof strychnine are via nicotinic $alpha$ 7receptors.

In summary, ACh and Gly were the two transmitter systems required for the generation of spontaneous propagating activity inE12 mouse cord. Furthermore, the fact that DH $beta$ E was able to rapidlyblock spontaneous bursting, whereas spontaneous episodes couldpersist for up to 1 hr in the presence of the glycinergic antagoniststrychnine, points to a central role of cholinergic transmissionin this system. It is presently unclear why strychnine took solong to block spontaneous bursting. Although strychnine may behaveas a slow-acting alkaloid in several systems in culture (Boehmet al., 1997; Levi et al., 1999), in E15.5 rat spinal cord slices(Kulik et al., 2000), the antagonistic affects of strychnine onGly receptor activation were immediate. Consistent with this observation,we found that Gly, when applied alone, elicited a series of bursts,and these could be blocked by strychnine as early as 15 min. Thissuggests that strychnine is blocking glycinergic receptors. Howeverat this time point, spontaneous propagating episodes were stilloccurring. One explanation for why strychnine took so long toblock the propagating episodes could be that in the absence ofglycinergic transmission, other inputs such as cholinergic areable to sustain bursting for some length of time. However, littleis known about glycinergic circuitry in the spinal cord at thisstage in development of either the mouse or thechicken.

Antidromic activation of motoneurons can elicit an episode that propagates throughout the lumbar cord

The ACh that was shown to play a critical role in generating spontaneous propagating episodes may arise from motoneurons orfrom interneurons. Because cholinergic interneurons have not beenobserved in the E12 mouse spinal cord, we tested the possiblerole of motoneurons in generating propagating activity. Characterizationof the E9-E12 chick spinal cord circuit (Chub and O'Donovan, 1998;O'Donovan et al., 1998; Fedirchuk et al., 1999) has shown thatspontaneous episodes result when recurrent excitatory connectionsbetween motoneurons and interneurons reach a threshold that elicitsan episode that propagates throughout the cord. This then resultsin a network depression so that episodes cannot be elicited fora period after a spontaneous episode. However, stimulation ofdescending input (stimulation of the cervical or thoracic regionof the cord) after this period will elicit an episode of the sameamplitude and duration as spontaneous propagating episodes. Similarly,in E12 mouse cord, after sufficient recovery from network depression,we found that activation of descending inputs, either at thoracic(Fig. 3B, 1) or more rostral lumbar (Fig. 3B, 2) levels, eliciteda burst of activity that propagated throughout the circuit andthat could be recorded with a delay from the right sciatic nerve.Such circuit activation could also be elicited by direct activationof motoneurons by stimulation of the segments containing the recordedmotoneurons and interneurons (Fig. 3B, 3). As expected, such directactivation of the motoneurons elicited a compound action potentialin the sciatic nerve (Fig. 3C, 3). Note that the latency of thismode of activation was considerably decreased compared with morerostral stimuli.

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Figure 3. Triggering of episodes by different sources of stimulation. A, Diagram of lumbar and thoracic regions of spinal cord. Stimulation electrodes (black) were placed at low thoracic (1), at lumbar segment 2 (2), directly over the recorded motoneurons (3), or directly onto the nerve from which the recording was made (4). B, The responses to each of these modes of stimulation are shown as bursts on a slow time base. C, The faster time base shows that only direct activation of large numbers of motoneurons by stimulating them directly in the cord or in the nerve proximal to the recording electrode resulted in a compound action potential. The stimulus artifact is noted by asterisks in the slow time base traces (left) and by SA in the faster time base traces (right). Antidromic activation of the motoneurons in the right sciatic nerve (B, 4) elicited a bursting episode that propagated throughout the cord, including left sciatic motoneurons.

To determine whether activation of motoneurons alone was capable of eliciting a burst that propagated throughout the circuit,the right sciatic nerve was stimulated proximal to the recordingsite (Fig. 3B, 4, top trace). This stimulation also produced aburst of similar amplitude and duration as those elicited by descendinginput, presumably via retrograde activation of the circuit viamotoneuron axon collaterals. Such antidromic activation of theright sciatic motoneurons was capable of activating the entirelumbar circuit, including the left sciatic motoneurons (Fig. 3B,4, bottom trace). Motor nerve stimulation also produced a compoundaction potential distally, because of the synchronous activationof many motoneurons, as seen in the expanded time base recording(Fig. 3C, 4, top trace). No compound action potential accompaniedthe burst in the left sciatic motoneurons, because these neuronswere not directly activated (Fig. 3C, 4, bottom trace). In addition,the burst recorded from this nerve occurred with some delay, asmight be expected if activation were occurring via propagationof activity through thecircuit.

Within the spinal motor circuit, motoneuron activation might simply reflect the output imposed by networks of interneurons.Alternatively, motoneurons might also play an active role in generatingor contributing to the activation of the cord circuit via cholinergictransmission from axon collaterals. The data presented above indicatethat motoneuron activation alone can elicit an episode of activitythat propagates throughout the cord. Furthermore, this mode ofcircuit activation occurred even when the dorsal roots were cutto prevent activation via sensory input (data not shown). In fact,at E12, dorsal root ganglion neurons are just beginning to projectaxons centrally (Ozaki and Snider, 1997). Afferents that projectout ventral roots have been described in postnatal animals, andventral root stimulation in P12-P20 rats (Jiang et al., 1991)produced glutamatergic EPSPs onto motoneurons. However, we havenot seen any anatomical evidence for such afferents in the E12mouse cord. Furthermore, the bursts that were elicited by stimulationof peripheral nerves were not blocked by glutamatergic antagonists.Taken together, our data indicate that the pattern of motoneuronactivation during spontaneous episodes may not simply reflectthe output of a circuit comprising interneurons, but also thatmotoneurons may activate the circuit presumably through axon collaterals(Cullheim et al., 1977; Lagerbäck et al., 1981).

We confirmed, by retrograde HRP labeling after direct injection of HRP into spinal nerves, that E12.5 mouse motoneurons hadnumerous axon collaterals that branched extensively (Fig. 4A,B).These axon collaterals appeared to terminate both within the motorcolumns and nearby regions of the cord as well as in the lateraland ventral white matter tracts (Fig. 4A; data not shown) (forembryonic cat and chick, see Ramon y Cajal, 1952a,b). To labelall of the cholinergic processes including axon collaterals, thesections were labeled with antibodies directed against the VCAT.At E12, this labeled the motoneuron somas in the lateral motorcolumn as well as their neurites (Fig. 4C). Similar to the HRPlabeling, large numbers of VCAT-positive neurites were found inthe lateral and ventral white matter tracts (Fig. 4C-E, LF, VF).VCAT-positive neurites also emerged from the lateral motor columnto terminate in the ventral spinal cord dorsal and medial to themotoneuron containing lateral motor column (Fig. 4C, asterisks).These data suggest that by E12.5, motoneurons have axon collateralsthat not only project locally but also project rostrally or caudallywithin the ventral and lateral funiculi. Although we cannot excludethe possibility that some of these VCAT-stained processes aredendrites, their overall distribution and morphology differedmarkedly from those of the dendritic processes of motoneuronsthat we observed with HRP back-labeling. Thus, we believe thatmost VCAT-positive neurites are axon collaterals of motoneurons.By using a combination of ChAT and VCAT labeling, we observedthat most cholinergic neurons at E12.5 reside within the lateralmotor column and are thus likely motoneurons (data not shown).However, by E15 in the rat, a cholinergic population of interneuronsthat resides medial to the motoneurons has been observed (Phelpset al., 1990; Barber et al., 1991). Although we occasionally observedChAT-positive neurons in this region in E12.5 mouse cord, retrogradeHRP labeling showed that at this time, some motoneuron somas hadnot yet migrated into the lateral motor column and might accountfor these cholinergic neurons. Unambiguous identification of thispopulation as interneurons as opposed to migrating motoneuronswill require assessing their expression of transcription factors(Saueressig et al., 1999; Pieriani et al., 2001). In summary,although we cannot exclude the presence of a small number of cholinergicinterneurons in the E12-E12.5 mouse cord, most cholinergic axonsappear to arise from motoneurons.

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Figure 4. Activation of a minimal number of motoneurons is required to elicit an episode that propagates throughout the cord. A, An E12.5 motoneuron retrogradely labeled with injection of HRP into spinal nerve reveals the cell soma, its axon projecting out the ventral root (VR, arrowhead) and axon collaterals (some denoted by asterisks) within the ventral horn. B, Inset showing location of labeled motoneuron in A. C, Immunohistochemistry of VCAT labeling also at E12.5 displays VCAT-positive neurites projecting from the lateral motor column into the ventral funiculus (VF), lateral funiculus (LF), and interneuron-containing regions dorsal and medial to the lateral motor column (asterisks). Scale bars, 25 µm. D, E, Inset from C of lateral and ventral funiculi, respectively, displaying VCAT-positive neurites. F-N, The left sciatic nerve trunk was stimulated with increasing intensity while recording from both left (G, J, M) and right (H, K, N) sciatic nerves. F, At low currents, some motoneurons were activated, resulting in a small compound action potential (CAP) in the sciatic nerve. However, this did not elicit a burst within the spinal motor circuit (G, H). I, At a higher current and with a larger number of motoneurons activated, as assessed from the CAP, a burst was elicited within the local circuit on the left (J) but did not activate an episode throughout the spinal cord (K). At maximal stimulus for motoneuron activation (L), an episode was elicited that propagated throughout the spinal cord (M, N).

Antidromic activation of motoneurons can elicit either local or propagating episodes

When a burst is activated by stimulating a motor nerve, only motoneurons, which have axons in that nerve, can initiate theburst. In all previous experiments, we used a stimulus that eliciteda maximal compound action potential and were presumably activatingall of the motoneurons within that nerve trunk. To determine whetherthe generation of a burst within those motoneurons and the subsequentpropagation of an episode of activity throughout the cord requiredactivation of a given proportion of motoneurons, stimulation ofthe motor nerve was performed at increasing stimulus intensities.To avoid circuit depression, compound action potentials and burstswere elicited only during the period when stimuli were capableof activating the entirecircuit.

At low current levels, single stimuli evoked small-amplitude compound action potentials (Fig. 4F, left) that did not activatea burst within the circuit of stimulated motoneurons (Fig. 4G,H).As the stimulus intensity was increased, activating a larger proportionof the motoneurons, as evidenced by the compound action potential(Fig. 4I), a burst could be elicited locally within the stimulatedmotoneurons (Fig. 4J). However, it did not propagate throughoutthe cord, as seen by the absence of a burst on the contralateralside (Fig. 4K). However, if the stimulus was further increased(Fig. 4L) to activate a larger proportion of motoneurons, thelocalized burst propagated throughout the cord, activating thecontralateral sciatic motoneurons (Fig. 4M,N). Because the amplitudeof the bursts, once triggered, did not increase with increasingstimulus intensity, our data suggest a triggered all-or-none responsewith a threshold for initiation (Ritter et al., 1999). These datasuggest that for the generation of a local burst, a sufficientnumber of motoneurons within a population must be activated. Furthermore,an even larger number of motoneurons within that population mustbe activated for that local burst to generate an episode thatpropagates throughout thecord.

Local and propagating episodes differ in their sensitivity to circuit depression

The experiments described above revealed the existence of a local circuit that could be activated by antidromic activationof the motoneurons. Furthermore, by applying superthreshold stimuli,we observed that this local circuit could be activated duringthe period of overall circuit depression, but that such localepisodes did not propagate throughout the cord. In the E9-E11chick cord, an episode of spontaneous activity elicits depressionof the circuit so that a second stimulated episode cannot be elicitedfor a significant portion of the interepisode interval (Chub andO'Donovan, 1998, 2001; Fedirchuk et al., 1999). Similar resultswere observed in the E12.5 circuit. Two spontaneous episodes ofactivity in the right (top) and left (bottom) sciatic nerves areshown in Figure 5B. Attempts to activate the circuit via descendinginputs were not successful if stimuli were applied at any pointleft of the dotted line. In the example shown in Figure 5C, thefirst two stimuli (asterisks) did not elicit a burst, whereasthat delivered after the period of circuit depression did (Fig.5B).

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Figure 5. A local circuit can be activated during the period of spinal motor circuit depression. A, B, Spontaneous episodes of activity were recorded in the left and right sciatic nerves with an interepisode interval of 96.4 ± 5.32 sec (mean ± SE). The dotted line indicates the earliest time that a stimulus could evoke an episode of activity that propagated throughout the cord. C, Stimulation of descending input (asterisks) could not elicit a burst in the left or right sciatic nerve until the period after the dotted line. D, Maximal antidromic activation (pound sign) of the motoneurons by stimulating the left sciatic nerve shortly after a spontaneous episode elicited bursts of activity in the stimulated sciatic nerve (top trace) but not in the contralateral nerve (bottom trace). D1, D2, Expanded time base of portions of the record. Retrogradely stimulating the left sciatic (D1), even at early times after a spontaneous episode, was capable of eliciting a burst in those motoneurons (top trace). However, such a burst did not spread throughout the lumbar cord, as indicated by the absence of a burst in the right sciatic nerve (bottom trace). Stimulation later in the interepisode interval (D2), however, when the entire lumbar circuit had recovered from depression, elicited a burst in the stimulated motoneurons (top trace), which subsequently elicited a burst with greater latency in the contralateral sciatic nerve (bottom trace).

In contrast, it was possible to elicit a local burst via antidromic activation of the right sciatic nerve, even after shortintervals following a spontaneous episode (Fig. 5D, 1, pound sign).However, such episodes did not propagate throughout the cord,as shown by the lack of a burst in the left sciatic nerve. Afterrecovery from circuit depression (Fig. 5D, 2, pound sign), activationof an episode from the right sciatic nerve propagated throughoutthe cord, resulting in a burst in the left sciatic nerve. Theexpanded time base records at right show that local bursts elicitedduring circuit depression, although slightly smaller (Fig. 5D,1), were quite similar to bursts (Fig. 5D, 2) that propagatedthroughout the cord. In summary, the data indicate the existenceof a local circuit that can be activated within the larger spinalmotor circuit. Furthermore, these results also show that thisearly (E12) mouse spinal motor circuit undergoes circuit depression,similar to that found in the more developed chick spinal motorcircuit (E9-E11; Chub and O'Donovan, 1998, 2001; Fedirchuk etal., 1999). Together, these data suggest that multiple local circuitsmight together constitute the overall motor circuit, and thattheir synchronous activation produces the rhythmic spontaneousactivity observed in the E12 mouse spinalcord.

Local and propagating episodes differ in their requirement for electrical transmission

Previously we demonstrated that rhythmic spontaneous activity required both electrical and chemical transmission. In addition,we have described a localized circuit in the E12 mouse spinalcord that can be activated by the activation of motoneurons. Thiscircuit is capable of eliciting propagating episodes and is ableto be activated during times when the overall circuit remainsdepressed. We next wished to address whether electrical or chemicaltransmission or both contribute to the activation of the localcircuits. To block electrical transmission, carbenoxolone, a gapjunction inhibitor, was added, and this abolished spontaneouspropagating episodes (Fig. 1F). Subsequent antidromic activationof the motoneurons was still able to elicit a local burst of activity,similar in amplitude and duration to the control local burst (Fig.6A). Thus, motoneurons do not require gap junction coupling toelicit a burst within the local circuit.

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Figure 6. Antidromic stimulation activates the local circuit through chemical transmission. A, Antidromic activation of the local circuit was not affected by application of the gap junction blocker carbenoxolone (100 µM). B, Local circuit activation was abolished in a solution of high Mg²⁺and low Ca ²⁺. Insets on a faster time base below the traces show the compound action potential produced by stimulation of the motor nerve trunk (A, B).

The importance of chemical transmission was investigated by perfusing the spinal cord with low Ca²⁺ (0.2 mM) and high Mg²⁺ (7.0 mM) to block transmitter release. This completely abolishedspontaneous propagating episodes as well as the ability of antidromicactivation of the motoneurons (Fig. 6B, inset) to elicit a localepisode. Thus, activation of the local circuit is brought aboutby chemicaltransmission.

Neither GABAergic nor glycinergic transmission is necessary for activation of the local circuit by antidromic motoneuron stimulation

The motoneuron axon collaterals could be making synaptic contacts with either interneurons or motoneurons. We demonstratedthat both GABA and Gly transmission influenced spontaneous activityin an excitatory manner. Glutamic acid decarboxylase 65 (GAD65),a marker for GABAergic neurons, has been detected as early asE13 in the rat in ventrally located neurons that not only projectto the ventral commissure but also have projections into the regionof the ventral horn and surrounding funiculi (Phelps et al., 1990).GAD65 staining of the E12.5 mouse spinal cord produced similarresults (data not shown). Therefore, we examined whether GABAergicor glycinergic transmission was required to elicit a burst withinthe local circuit by antidromic motoneuron activation. When glycinergictransmission was blocked by strychnine (5 µM), stimulation ofdescending inputs no longer elicited an episode of activity, andthis occurred within 15 min of drug application (Fig. 7A, toptrace). However, direct activation of the motoneurons in the lumbarcord still elicited an episode (middle trace). Furthermore, retrogradeactivation of the circuit via stimulation of the motoneurons wasnot affected by strychnine throughout the time course of drugapplication (bottom trace). These data combined with our previousobservations indicate that although glycinergic transmission isrequired for the propagation of spontaneous episodes throughoutthe cord, it is not required for the activation of the local circuit.

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Figure 7. Activation of the local circuit by antidromic stimulation of motoneurons is independent of GABAergic and glycinergic transmission. A, Although strychnine (5 µM) did block the ability of a descending input to elicit an episode, bursts elicited by direct or antidromic activation of the motoneurons were only slightly affected. B, In addition, picrotoxin (50 µM) had no effect on activation via the descending input and little effect on direct or antidromic activation of the motoneurons. C, The combination of both drugs slightly decreased the response elicited by direct activation of the cord segments containing the motoneurons (top trace) but had no effect on the burst elicited by antidromic activation of the motoneurons (bottom trace).

To assess the role of GABAergic transmission in the antidromic activation of the local circuit, picrotoxin (50 µM) was applied(Fig. 7B). As shown previously, blocking GABA_A receptors slightlyslowed the frequency of spontaneous episodes but had no affecton the ability of descending input to elicit a burst (Fig. 7B,top trace) or through direct cord activation of the motoneurons(middle trace). The activation of the local circuit via antidromicstimulation of the motoneurons was also unaffected by picrotoxin(bottom trace). To remove both glycinergic and GABAergic transmissionfrom interneurons, both picrotoxin and strychnine were appliedtogether (Fig. 7C), slightly decreasing the amplitude of the burstgenerated by directly activating the motoneurons at the lumbarlevel of the spinal cord (top trace). However, activation of localepisodes via antidromic activation of the motoneurons was unaffected(bottom trace). Glutamate antagonists APV and CNQX also had noeffect on the activation of local episodes by antidromic motoneuronactivation (data not shown). We sometimes observed slight changesin burst duration and amplitude with drug treatments, perhapsbecause of less synchronous activation of the circuit (Fig. 7B,C),but these were notquantified.

Motoneuron activation elicits local episodes via nicotinic receptors that differ from those required for spontaneous propagating episodes

We have demonstrated that cholinergic transmission is required for spontaneous propagating episodes in the E12 mouse spinalcord. However, many of the general nicotinic ACh receptor antagonists,such as dTC and mecamylamine, did not completely abolish spontaneousactivity (Fig. 2B). Within the ventral horn at later stages ofdevelopment, cholinergic synapses have been shown to originateboth from collaterals of neighboring motoneurons and from nearbyinterneuron populations (Cullheim et al., 1977; Lagerbäck etal., 1981; Wetts and Vaughn, 2001). It was therefore importantto determine the extent to which cholinergic transmission betweenmotoneurons, versus that between interneurons and motoneurons,contributed to the activation of bursting episodes. Although avariety of cholinergic antagonists are available that are thoughtto be specific for various nicotinic subunit combinations (Dwoskinand Crooks, 2001), these specificities have not been demonstratedfor developing nicotinic receptors. Therefore, dTC, which is considereda nonspecific nAChR antagonist in more mature systems, may onlyblock a subset of nAChR in the early spinal motor circuit. Thus,to completely abolish cholinergic transmission, we chose to preventthe uptake of ACh into synaptic vesicles with vesamicol (100 µM;Marshall and Buccafusco, 1987; Prior et al., 1992). This abolishedrhythmic spontaneous activity (~30 min; data not shown), antidromicactivation of the local circuit (Fig. 8A), as well as activityelicited by direct stimulation of the local circuit (Fig. 8A).

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Figure 8. Cholinergic transmission is required to elicit episodes via both descending and antidromic stimulation of motoneurons, but the differing pharmacology suggests that different nicotinic subunits are used. A, Preventing cholinergic transmission with vesamicol, an inhibitor of ACh uptake into vesicles (100 µM), prevented bursts elicited by both antidromic activation and direct activation of the cord segments containing the motoneurons. Stim, Stimulus; Rec, recording. B, Activation of the circuit via a descending input was blocked by 5 µM DH $beta$ E (top trace), whereas direct activation of the circuit by stimulating the lumbar cord (middle trace) or antidromic activation via stimulation of motoneurons (bottom trace) was unaffected. C, The amplitude and duration of the burst elicited by antidromic activation of the motoneurons was reduced by either 20 µM mecamylamine (Mec, left) or 10 µM dTC (right middle trace). The combination of mecamylamine and dTC essentially blocked antidromic activation of the circuit via motoneuron stimulation (right bottom trace; arrows indicate time of stimulation).

Given that blockade of cholinergic transmission prevented local circuit activation, we examined several nAChR antagoniststo characterize the relevant receptors. After application of DH $beta$ E(5 µM), which blocked spontaneous propagating episodes, stimulationof descending inputs no longer elicited an episode (Fig. 8B, toptraces). In contrast, DH $beta$ E had no effect on local bursts of activity,activated by either direct stimulation of the lumbar cord containingthe recorded motoneurons (middle traces) or by antidromic activationof motoneurons (bottom traces). However, these bursts were confinedlocally and did not propagate throughout the cord, as they wouldhave in the absence of DH $beta$ E. Thus, it appears that endogenouslyreleased ACh acting via DH $beta$ E-sensitive receptors is required forpropagation of activity throughout thecord.

Endogenously released ACh was also required for effective activation of the local circuit but did so via different receptors.Although mecamylamine (20 µM) or dTC (10 µM) had no effect onthe activation of the cord circuit via descending input (datanot shown), each of these nicotinic antagonists reduced the amplitudeof bursts elicited by antidromic activation of the motoneuronsand when applied together almost completely suppressed such localbursts (Fig. 8C). These observations suggest that dTC and mecamylamineare mainly blocking cholinergic transmission in the local circuit,possibly betweenmotoneurons.

Either cholinergic or GABAergic transmission can elicit a local burst in response to direct cord stimulation

Direct stimulation of the ventral spinal cord would be expected to activate both motoneurons and nearby interneurons. As discussedabove, the combination of mecamylamine and dTC was able to essentiallyblock the local burst elicited by antidromic motoneuron activation.In contrast, these two drugs together (Fig. 9B), or even withthe addition of DH $beta$ E (data not shown), only modestly reduced theamplitude of a local burst elicited by direct cord stimulation.However, when the GABA_A antagonist picrotoxin (50 µM) was alsoadded, the burst was virtually abolished (Fig. 9C). As shown previously(Fig. 7A,B), picrotoxin or strychnine when applied alone had almostno effect on the burst elicited by direct cord stimulation. Thesedata taken together suggest that the local circuit comprises acholinergic pathway that presumably arises from motoneuron axoncollaterals acting on other motoneurons and that does not requireactivation of GABAergic or glycinergic interneurons and a secondpathway that activates GABAergic and glycinergic neurons and thatdoes not require the cholinergic transmission from the motoneuroncollaterals.

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Figure 9. Direct activation of the local circuit can occur via either cholinergic or GABAergic transmission. A, B, The combination of 20 µM mecamylamine (Mec) and 10 µM dTC only slightly decreased the amplitude and duration of bursts elicited by stimulating the lumbar cord segments containing the motoneurons recorded from the sciatic nerve. C, Addition of 50 µM picrotoxin (Picro) to mecamylamine and dTC abolished most of response elicited by direct cord stimulation of the circuit (solid arrows indicate times of initial stimulation; small arrows indicate subsequent stimulations).

Blockade of the local circuit abolishes rhythmic spontaneous activity

As shown previously, mecamylamine, dTC, or picrotoxin alone did not block the spontaneous propagating episodes (Fig. 3). Inaddition, blocking either of the local pathways described abovealone did not block spontaneous activity. However, blocking boththe local cholinergic pathway via dTC and mecamylamine and theGABA_A receptor pathway via picrotoxin blocked spontaneous activity(Fig. 10). These data appear to indicate that blocking transmissionwithin the local circuit abolishes the generation of spontaneousepisodes of activity. Therefore, both pathways for local circuitactivation contribute to the propagation of spontaneous episodesof activity that propagate throughout the spinal cord.

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Figure 10. Blockade of the local circuit abolishes rhythmic spontaneous activity. The intervals between spontaneous episodes of activity were increased after application of 10 µM dTC. The addition of 20 µM mecamylamine (Mec) to dTC did not significantly increase interepisode intervals further. However, rhythmic spontaneous activity was abolished when 50 µM picrotoxin (Picro) was added to the bath containing dTC and mecamylamine.

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The nervous system is unique among developing systems in that electrical activity generated by emergent neural circuits caninfluence subsequent developmental processes (Katz and Shatz,1996; Feller, 1999; O'Donovan, 1999; Ganguly et al., 2001). Inthis study, we have characterized the circuit that generates spontaneousrhythmic activity at the earliest times in mouse spinal motorcircuit formation. Among our major findings are that both chemicaland electrical transmission are required for such activity. Furthermore,we have shown that motoneurons themselves, acting via DH $beta$ E-insensitivenicotinic receptors, play an important role in generating thisactivity by participating in local circuits with GABAergic interneuronsto provide the excitatory drive needed to elicit a local burst.However, for these bursts to propagate throughout the cord, cholinergictransmission via DH $beta$ E sensitive receptors, glycinergic transmission,and electrical coupling via gap junctions is required. We willpropose a model circuit that incorporates these findings, discussthis in relation to other developing motor circuits, and compareour results with rhythmic spontaneous activity elsewhere in thenervous system and its potential role indevelopment.

Spontaneous episodes of activity and the maturation of the embryonic mouse spinal motor circuit

Our observations indicate that endogenously released ACh most likely from the motoneurons themselves and acting on nicotinicreceptors is essential for the generation of spontaneous rhythmicactivity in the E12-E12.5 mouse spinal cord, similar to resultsfrom the St25 (E4-E5) chick cord (Milner and Landmesser, 1999).In contrast to the more mature mouse, rat, and chick circuits,in which glutamate drives spontaneous activity (Nishimaru et al.,1996; Chub and O'Donovan, 1998; Branchereau et al., 2002), glutamateantagonists had no effect on spontaneous bursting activity inthe E12 mouse cord, as was also observed for E14.5 rat cord (Nishimaruet al., 1996). A similar switch in excitatory drive from cholinergicto glutamatergic also occurs in spontaneous retinal waves duringdevelopment (Feller et al., 1996; Catsicas et al., 1998; Wonget al., 1998; Zhou and Zhao, 2000).

In many developing systems, the classical inhibitory transmitters GABA and Gly have been shown to act in an excitatory manner(Wu et al., 1992; Owens et al., 1996). Consistent with these observations,we found that their pharmacological blockade either slowed (forGABA) or blocked (for Gly) spontaneous episodes of activity. Blockadeof glycinergic transmission has also been shown to block spontaneousepisodes of activity in E15 rat cord (Nishimaru et al., 1996).With maturation, these excitatory responses to GABA and Gly becomeinhibitory (Wu et al., 1992) as the intracellular levels of chlorideare lowered, resulting in more negative equilibrium potentialsfor these transmitters. The intracellular chloride concentrationis determined by the activity of a number of chloride transporters.In the mouse cord one of these, potassium-chloride cotransporter(KCC2), which extrudes chloride, thus reducing the intracellularchloride concentration (Payne, 1997), increases during development(Lu et al., 1999) and is in fact required for the switch of GABAtransmission to inhibitory (Hubner et al., 2001). Intriguingly,in cultured hippocampal neurons, the expression of this transporteris itself controlled by GABA-mediated depolarization (Gangulyet al., 2001).

Local circuits of motoneurons and GABAergic interneurons underlie the central pattern generator for rhythmic spontaneous activity

Central pattern generators (CPGs) that produce rhythmic movements, such as respiration and locomotion, have been characterizedin many systems. Most studies of the locomotor CPG in mouse orrat cord have focused on the neonatal period, when activity isusually evoked by the addition of neuromodulators such as serotonin(Cazalets et al., 1995; Kjaeruluff and Kiehn, 1996; Whelan etal., 2000). Clearly, early embryonic circuits in chick (Milnerand Landmesser, 1999) and mouse differ from these more maturecircuits in several important ways. Furthermore, this activityoccurs spontaneously without the need for descending or afferentinput. What drives this early bursting activity? Observationsin the E10-E12 chick cord support a model in which recurrent excitatoryconnections between motoneurons and glutamatergic and possiblyGABAergic interneurons result in a level of network excitationthat reaches threshold for propagation throughout the cord (Ritteret al., 1999).

Our data on E12 mouse cord are consistent with such a model and provide strong support for motoneurons themselves playinga critical role in generating episodes of activity. We have shownthat local circuits of motoneurons and GABAergic interneuronsconnected in an excitatory manner are essential for spontaneousepisodes to occur (Fig. 11; top). When a sufficient number of motoneuronswere retrogradely activated, a local episode of activity was triggered.Motoneuron axon collaterals that contact other motoneurons havebeen observed in adult cat cord (Cullheim et al., 1977), and weobserved motoneuron axon collaterals terminating in multiple brancheswithin the lateral motor column, which at E12 is almost exclusivelycomposed of motoneuron somas. We also observed these collateralsterminating outside the lateral motor column in regions knownto contain interneurons, some of which are GABAergic (Pieraniet al., 2001). In fact, the GABAergic interneurons in the localcircuit we have characterized might correspond to some of theV1 engrailed-positive population of interneurons, whose axonsproject short distances rostrally within the ventrolateral funiculusbefore terminating in the lateral motor column (Saueressig etal., 1999). In Xenopus tadpoles, cholinergic transmission betweenmotoneurons has been demonstrated (Perrins and Roberts 1995a),most likely from motoneurons that excite interneurons (Perrinsand Roberts, 1995b). Both contribute to the fidelity of the CPGthat drives swimming. Based on ChAT expression, a small numberof cholinergic interneurons have been identified in E14 rat cord(Phelps et al., 1990). However, we have not observed any ChAT-or VCAT-positive neurons that could be unambiguously identifiedas interneurons in E12 mouse cord. Thus, we believe that all ofthe cholinergic inputs that contribute to the E12 mouse CGP mostlikely arise from motoneurons.

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Figure 11. Proposed model of the E12 mouse spinal motor circuit. Top, The local circuit consists of two pathways for activation, GABAergic neurons that activate motoneurons and probably other GABAergic interneurons (not shown) and motoneurons, which activate other motoneurons and GABAergic interneurons via axon collaterals. Activation of either of these pathways by direct cord stimulus or by antidromic stimulation of motoneurons from the peripheral nerve results in a burst in the local circuit. Middle, Local episodes of activity propagate to other regions of the cord by motoneuron axon collaterals activating glycinergic interneurons. These subsequently activate local circuits at other segmental levels as well as contralaterally (not shown; see Discussion for additional detail). Bottom, Summary table comparing the properties of the local response, the propagating response, and the spontaneous episodes of activity for the E12 mouse spinal motor circuit. Note that cholinergic transmission in the local circuit is DH $beta$ E-insensitive, whereas that used in the propagating circuit and in spontaneously generated episodes is blocked by DH $beta$ E. Similarly, both the propagating circuit and spontaneous activity require electrical transmission, whereas the local circuit does not. MN, Motoneuron; Mec, mecamylamine; Sen R, sensitive receptor; Stryc, strychnine.

To propagate throughout the cord and elicit an episode of spontaneous activity, local circuit bursts require glycinergic interneurons

The existence of a separate, glycinergic interneuron-containing pathway (Fig. 11, middle) for the propagation of local episodesis supported by the failure of local episodes to propagate inthe presence of strychnine. In addition, the cholinergic antagoniststhat blocked local episodes differed from those that blocked propagation(pharmacological data summarized in Fig. 11, bottom). The nicotinicreceptors involved in the local episodes (on motoneurons and perhapsGABAergic interneurons) were DH $beta$ E-insensitive, whereas those presumablyon the glycinergic interneurons were DH $beta$ E-sensitive. Furthermore,because direct cord stimulation simultaneously activates motoneuronsand GABAergic neurons, and spontaneous activity still persistedin the presence of mecamylamine and dTC, we cannot rule out thatthe glycinergic neurons also excite the local GABAergic populationof neurons. Finally, the circuit for propagation exhibited strongcircuit depression so that another propagating episode could notbe generated for at least 1 min after a spontaneous episode, similarto what has been observed in the E10-E12 chick (Fedirchuk et al.,1999). In contrast, the lo