Synapse-Glia Interactions at the Mammalian Neuromuscular Junction

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The Journal of Neuroscience, June 1, 2001, 21(11):3819-3829

Synapse-Glia Interactions at the Mammalian Neuromuscular Junction
Danielle Rochon, Isabelle Rousse, and Richard Robitaille
Centre de Recherche en Sciences Neurologiques and Département de Physiologie, Université de Montréal, Montréal, Quebec, Canada H3C 3J7

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Perisynaptic Schwann cells (PSCs) play critical roles in regulating and stabilizing nerve terminals at the mammalian neuromuscularjunction (NMJ). However, although these functions are likely regulatedby the synaptic properties, the interactions of PSCs with thesynaptic elements are not known. Therefore, our goal was to studythe interactions between mammalian PSCs in situ and the presynapticterminals using changes in intracellular Ca²⁺ as an indicator of cell activity. Motor nerve stimulation inducedan increase in intracellular Ca²⁺ in PSCs, and this increase $y$ as greatly reduced when transmitterrelease was blocked. Furthermore, local application of acetylcholineinduced Ca²⁺ responses that were blocked by the muscarinic antagonist atropineand mimicked by the muscarinic agonist muscarine. The nicotinicantagonist $alpha$ -bungarotoxin had no effect on Ca²⁺ responses induced by acetylcholine. Local application of thecotransmitter ATP induced Ca²⁺ responses that were unaffected by the P2 antagonist suramin,whereas local application of adenosine induced Ca²⁺ responses that were greatly reduced by the A1 receptor antagonist8-cyclopentyl-1,3-dimethylxanthine (CPT). However, the presenceof the A1 antagonist in the perfusate did not block responsesinduced by ATP. Ca²⁺ responses evoked by stimulation of the motor nerve were reducedin the presence of CPT, whereas atropine almost completely abolishedthem. Ca²⁺ responses were further reduced when both antagonists were presentsimultaneously. Hence, PSCs at the mammalian NMJ respond to therelease of neurotransmitter induced by stimulation of the motornerve through the activation of muscarinic and adenosine A1receptors.

Key words: adenosine; acetylcholine; Ca²⁺; perisynaptic Schwann cell; transmitter release; neuromuscular junction; synapse-glia interactions

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Recent evidence indicates that there are dynamic, bidirectional interactions between glial cells and neurons. Indeed, notonly are glial cells modulated by nerve-evoked transmitter releasebut they, in turn, modulate neuronal activity (Nedergaard, 1994;Parpura et al., 1994; Pfrieger and Barres, 1997; Bezzi et al.,1998; Newman and Zahs, 1998; Robitaille, 1998).

The vertebrate neuromuscular junction (NMJ) is an interesting preparation to study synapse-glia interactions because it isa simple synapse where the anatomical relationship between presynaptic,postsynaptic, and glial elements is maintained. Perisynaptic Schwanncells (PSCs) or terminal Schwann cells, glial cells at this synapse,have been studied at the amphibian NMJ and have been shown todetect synaptic activity, as revealed by an elevation in intracellularcalcium (Jahromi et al., 1992; Robitaille, 1995). PSCs possesspurinergic and muscarinic receptors as well as neurokinin-1 (NK-1)receptors for substance P (Robitaille, 1995; Robitaille et al.,1997; Bourque and Robitaille, 1998), and their activity is governedby these receptors (Georgiou et al., 1994, 1999; Bourque and Robitaille,1998). Moreover, as a consequence of synaptic activity, PSCs modulatethe efficacy of the synapse by regulating transmitter release(Robitaille, 1998; Castonguay and Robitaille, 2001).

PSCs also modulate nerve growth and synapse maintenance. Although recent evidence has been obtained at the amphibian NMJ (Herreraet al., 2000; Koirala et al., 2000), most evidence has been obtainedat the mammalian NMJ. For instance, processes extended by PSCsafter denervation influence the regrowth of motor axons to themuscles and their guidance back to denervated NMJs (Son et al.,1996). Furthermore, immunocytochemical markers specific for Schwanncells, synapses, and motor axons were used to show that motoraxons navigate along the processes extended by PSCs from the damagednerve endings (Son and Thompson, 1995a,b). The guidance of axonsby PSCs lead to clustering of motor units, a phenomenon typicalof many neurogenic pathologies (Son et al., 1996). Notwithstandingthe functional importance of PSCs, very little is known abouttheir properties at the mammalian NMJ where, in fact, no evidenceof direct modulation of synaptic activity is available andä wherethe properties are not characterized. Moreover, although synapse-gliainteractions appear to be a common phenomenon at chemical synapses(Araque et al., 1999; Castonguay et al., 2001), it is still unclearhow much the properties of these interactions differ between relatedsynapses. Hence, this study aimed to characterize PSCs propertiesat the mammalian NMJ to determine functional similarities anddifferences with the properties of the amphibianNMJ.

We report that, similar to PSCs at amphibian NMJ, PSCs at the mammalian NMJ respond to the release of neurotransmitters inducedby stimulation of the motor nerve via activation of muscarinicreceptors. However, the role of the purinergic receptors of PSCsat the mammalian NMJ differs where A1 adenosine receptors, butnot P2 receptors, contribute to the activation of PSCs. Hence,these results indicate that although synapse-glia interactionsare present at chemical synapses in situ, these interactions aregoverned by specialized features related to the synapse with whichglial cells areassociated.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Nerve-muscle preparation. Experiments were performed at room temperature on levator auris longus nerve-muscle preparationsdissected from CD1 mice (22-24 gm; Charles River Laboratories,Wilmington, MA). Muscles were removed under deep anesthesia (midazolamand hypnorm dissolved in water). The normal Ringer's solutioncontained (in mM): 124 NaCl, 5 KCl, 1.25 NaH₂PO_4, 2 MgCl₂, 2 CaCl₂,26 NaHCO₃, and 10 glucose. A 0 Ca²⁺/5 mM Mg²⁺ physiological solution contained (in mM): 124 NaCl, 5 KCl, 1.25NaH₂PO₄, 5 MgCl₂, 26 NaHCO₃, and 10 glucose. Solutions were oxygenatedwith a gas mixture of 95% O₂ and 5% CO₂.

Calcium imaging of mammalian PSCs. Muscles were incubated for 90 min at room temperature in a physiological solution saturatedwith 95% O₂ and 5% CO₂ and containing 20 µM fluo-3 AM (MolecularProbes, Eugene, OR; Tsien, 1989), 0.02% pluronic acid (MolecularProbes), and 0.5% dimethylsulfoxide (Sigma, St. Louis, MO). Muscleswere then pinned down in a recording chamber coated with Sylgard.Partial chelation of heavy metal ions was achieved using 20 µMtetrakis (2-pyridylmethyl) ethylenediamine (Molecular Probes)to limit binding of these ions to fluo-3. Changes in fluorescenceintensity were monitored using a Bio-Rad (Hercules, CA) 600 laser-scanningconfocal microscope equipped with an argon ion laser. The 488nm laser line was attenuated to 1% intensity, and a long-passfilter with cutoff at 515 nm was used to detect the emitted fluorescence.A 40× water immersion lens was used (0.75 NA; Olympus, Tokyo,Japan). Surface NMJs were located using transmitted light microscopy.The intensity of fluorescence (F) was measured over the area ofthe PSCs cell body, and the relative changes in fluorescence intensitywere expressed as % $Delta$ F/F = (F $-$ F _rest)/F_rest ×100.

Drug applications. ATP, adenosine, muscarine, and acetylcholine (20 µM) were dissolved in the same saline as that in the recordingchamber. Drugs were applied directly by micropressure (5-10 PSI;pulse duration, 200 msec) to selected cells with a micropipette(tip diameter, 2-4 µM) using a Picospritzer II (General Valve,Fairfield, NJ). The local application of the agonists induceda slight movement of the muscle fiber that moved briefly out offocus resulting in a small deflection in the fluorescence level(see Figs. 3-7). The micropipette was positioned near the PSC somataunder visual control at high magnification (40× water immersionobjective). There was no increase in fluorescence when Ringer'ssolution was applied alone. When several applications were performedon the same cells, a recovery period of at least 15 min was allowedbetween each application. For the Ca²⁺-free/5 mM Mg²⁺ experiments, preparations were perfused in the modified physiologicalsolution for 25-30 min before the experiments. Some antagonists( $alpha$ -bungarotoxin, $omega$ -conotoxin MVIIC) were applied directly in therecording chamber in a closed bath, whereas suramin, 8-cyclopentyl-1,3-dimethylxanthine(CPT), and atropin were applied by bathperfusion.

Stimulation of the motor nerve. Nerve-muscle preparations were processed for fluo-3 AM loading as described above. Stimulationof the distal end of the cut motor nerve (50 Hz, 30 sec) was achievedusing a suction electrode. To prevent muscle contractions evokedby transmitter release, cholinergic receptors were blocked with $alpha$ -bungarotoxin ( $alpha$ -BuTx; 20 µM; Molecular Probes). Preparationswere allowed to rest for 20-25 min between trains of stimuli whenseveral trains were performed on the samepreparation.

Immunocytochemistry. After some experiments, muscles were fixed using 4% paraformaldehyde for 10 min and rinsed for at least30 min in three changes of Ringer's solution. Muscles were thenpermeabilized in $-$ 20°C methanol for 6 min, washed again in Ringer'ssolution for 30 min, and nonspecific staining was blocked usingRinger's solution's containing 0.3% Triton X-100 and 0.2% drymilk. Muscles were incubated overnight at room temperature witha rabbit antibody solution raised against cow S-100 (Dako, Carpinteria,CA) prepared in the solution indicated above (dilution 1:400).After incubation in the primary antibody, muscles were rinsedin three changes of Ringer's solution for 30 min and incubatedin secondary antibody for 1 hr at room temperature. The secondaryantibody was an anti-rabbit conjugated to biotin-SP (Jackson ImmunoResearch,West Grove, PA: 1:500) and revealed using avidin FITC (1:100;for 2 hr). Finally, muscles were rinsed for 10-15 min in Slowfadeantifade reagent (Molecular Probes). Preparations were mountedonto glass slides in Slowfade antifade under a coverslip. Imagesof the same NMJs studied for Ca²⁺ imaging were collected under immersion oil with a 40× lens (Nikon),using the Bio-Rad 600 confocalmicroscope.

Statistics. Results are presented as mean ± SEM. A Student paired t test was used when a treatment was performed on the samecell (control vs drug), and an ANOVA was used for comparison betweendifferent groups. Both tests were used at a confidence level of95% ( $alpha$ = 0.05).

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Identification of PSCs at the mammalian NMJ

The validity of the study of synapse-glia interactions at the mammalian NMJ relies on our ability to identify PSCs. However,unlike PSCs at the frog NMJ, mammalian PSCs are not so easilyrecognized in bright-field illumination. Mammalian NMJs have anoval shape and are more compact than amphibian NMJs. They terminatein a slight elevation of the muscle fiber, just after the myelinsheath where the nerve terminal forms a compact junction (Salpeter,1987). The identification of PSCs was achieved based on thesecharacteristics.

We first confirmed that these criteria of identification were reliable by labeling PSCs using an antibody against the calcium-bindingprotein S-100, which is used as a general marker for Schwann cells(Son and Thompson, 1995a). First, cells were identified by transmittedlight according to the criteria indicated above, and preparationswere loaded with the permeant fluorescent Ca²⁺ indicator fluo-3 AM (Fig. 1A). A brief local application of muscarineincreased Ca²⁺ fluorescence in the cell body of the presumed PSCs (Fig. 1B)that subsequently decreased back to baseline (see also Figs. 3and 4). The nerve-muscle preparation was then processed for immunohistochemistry,and the presence of S-100 was revealed. The same NMJ was thenfound, and an image of S-100 labeling was taken using the confocalmicroscope. As shown in Figure 1C, the same cells identified asPSCs corresponding to our criteria and that showed a Ca²⁺ response induced by muscarine were also labeled by S-100. Theseresults indicate that they were Schwann cells at the NMJ, andhence, that the criteria used to identify PSCs were appropriate.Also, the myelinating Schwann cells that were also loaded withfluo-3 were also labeled by S-100 (data not shown).

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Figure 1. Identification of PSCs at the mammalian NMJ. A, False color confocal image of a mammalian NMJ loaded with the fluorescent Ca²⁺ indicator fluo-3 AM. The range of false colors reflects the level of Ca²⁺ level, where blue indicates a low level of Ca²⁺, and green-red indicates a high level. Two PSCs (arrows) at rest before local application of muscarine. B, The same PSCs as in A, after application of muscarine (20 µM). Note the rise in fluorescence induced by muscarine. C, Labeling of PSCs of the same NMJ with anti-S100, a calcium binding protein used as a general marker for Schwann cells. Note that the two cells that responded to muscarine were also labeled by the S100 antibody. Scale bar, 20 µm.

Nerve-evoked Ca²⁺ responses in perisynaptic Schwann cells

The sensitivity of mouse PSCs to synaptic transmission and transmitter release was established by monitoring changes in intracellularCa²⁺ during synaptic activity induced by repetitive stimulation ofthe motor nerve. As shown in Figure 2A, a train of stimuli (50Hz, 30 sec) triggered an increase in fluorescence. This was observedin all PSCs tested (n = 10) with a mean of 157 ± 15% $Delta$ F/F. Thiselevation in intracellular Ca²⁺ occurred, on average, with a delay to onset of 1.5 sec afterthe beginning of the stimulation, and the time to reach the maximumamplitude was 15 ± 2 sec. Ca²⁺ responses decayed to baseline in 82.2 ± 12 sec, which occurredwell after the interruption of nerve stimulation. In addition,in all PSCs studied, the initial Ca²⁺ response was always followed by a second smaller elevation thatoccurred after a partial recovery of the initial response. Nervestimulation at lower frequencies (10, 15, or 25 Hz) resulted insmaller Ca²⁺ responses than the ones obtained with stimulation at 50 Hz (datanot shown). As seen in Figure 2A, a second train of stimuli given20 min after the first one (break in the x-axis) hardly eliciteda Ca²⁺ response. The mean amplitude of the response was only 14 ± 15% $Delta$ F/F(n = 5). These results indicate that PSCs detect and are sensitiveto synaptic activity. In contrast to the PSCs, and although loadedwith fluo-3, no Ca²⁺ responses were detected from the myelinating Schwann cells presentat the last myelinated segment of the motor nerve (data not shown).

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Figure 2. Nerve-evoked Ca²⁺ responses in PSCs. Ca²⁺ responses obtained using the fluorescent Ca²⁺ indicator fluo-3 AM and monitored using a Bio-Rad 600 confocal microscope. Blue indicates low level of calcium, and red indicates a high level. A, Changes in fluorescence (% $Delta$ F/F) before, during (bar), and after motor nerve stimulation (50 Hz, 30 sec). Note that relative increase in Ca²⁺ fluorescence to a second train of stimuli applied 20 min later (break in the x-axis) was much reduced. B, Ca²⁺ response in the same PSC as in A, before (1), during (2), and after (3-5) transmitter release induced by repetitive stimulation of the motor nerve (50 Hz, 30 sec). The corresponding time at which each image was taken is illustrated on the graph in A with the corresponding number of the figure above. C, Changes in fluorescence (% $Delta$ F/F) before, during (bar), and after motor nerve stimulation (50 Hz, 30 sec) in the presence of $omega$ -conotoxin MVIIC (1 µM). Note that the increase in the intensity of the fluorescence was strongly reduced when transmitter release was blocked by $omega$ -conotoxin MVIIC, a P/Q-type Ca²⁺ channel blocker. Different preparation than A and B. D, Mean ± SEM of amplitude of Ca²⁺ responses in PSCs elicited by nerve stimulation in the absence and in the presence of $omega$ -conotoxin MVIIC (p = 0.001; Student's paired t test). Scale bar: B, 10 µm.

Is transmitter release required to elicit Ca²⁺ responses?

The response of PSCs to synaptic activity could be attributable to an increase of extracellular K⁺ ions during high-frequency stimulation that would depolarizethe cell and open voltage-gated Ca²⁺ channels (MacVicar, 1984; Newman, 1986; Barres et al., 1990;Robitaille et al., 1996) or to the release of neurotransmitters(Jahromi et al., 1992; Reist and Smith, 1992; Robitaille, 1995).To distinguish between the two possibilities, the Ca²⁺-dependent release of neurotransmitters was prevented by blockingthe Ca²⁺ channels that trigger this process. If transmitter release isrequired to elicit Ca²⁺ responses observed in PSCs, these should be reduced in the presenceof the Ca²⁺ channel blocker. However, Ca²⁺ responses in PSCs should remain unchanged if they are causedby K⁺ accumulation. Transmitter release was blocked using the toxin $omega$ -conotoxin MVIIC ( $omega$ -CgTx), which binds irreversibly to P/Q-typeCa²⁺ channel. It was used at concentrations known to completely blockevoked transmitter release at the mouse NMJ (Katz et al., 1996).After blockade of transmitter release by $omega$ -CgTx (1 µM; data notshown), the nerve-evoked Ca²⁺ signal in PSCs was on average 9 ± 2% $Delta$ F/F (n = 6) (Fig. 2C).This represents a reduction of 94% in the size of the Ca²⁺ responses in comparison to the ones obtained in the absence of $omega$ -CgTx MVIIC (Fig. 2D). Thus, substances released by the nerveterminal during evoked activity are necessary for the inductionof Ca²⁺ responses in PSCs, suggesting that PSCs are sensitive to transmittersreleased during synaptic activity. The residual Ca²⁺ response in PSCs in the presence of $omega$ -CgTx MVIIC is likely attributableto the depolarization of the cell caused by K⁺ accumulation during synaptic activity (Jahromi et al., 1992;Robitaille et al., 1996).

Can ACh trigger Ca²⁺ responses at the mammalian NMJ?

Our data indicate that neurotransmitter substances released during synaptic activity are necessary to elicit fully developedCa²⁺ responses in PSCs. As primary candidates, ACh and ATP appearparticularly important because ACh is the main neurotransmitterat this synapse and ATP is coreleased at an equimolar concentration(Silinsky, 1975; Smith, 1991). If substances such as the cotransmittersATP and ACh released by the active nerve terminal induce PSC Ca²⁺ signals, then application of these substances alone should mimicthe effects induced by stimulation of the motornerve.

The ability of PSCs to respond to ACh applied locally was examined first. ACh was applied directly by micropressure (5-10PSI) to selected PSCs. As shown in Figure 3A, local applicationof ACh (20 µM) induced a Ca²⁺ response in all PSCs tested (350 ± 18% $Delta$ F/F; n = 10). Becausethe Ca²⁺ response obtained by stimulation of the motor nerve decreasedduring consecutive trains of stimuli (Fig. 2A), we wondered whetherthe Ca²⁺ responses induced by local applications of ACh would also besusceptible to rundown. Indeed, a second application of ACh evokedresponses that were significantly smaller than the first ones(249 ± 19% $Delta$ F/F vs 357 ± 30% $Delta$ F/F for control; n = 5; p = 0.0006;Student's paired t test) (Fig. 3A, break in the x-axis).

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Figure 3. Ca²⁺ responses of PSCs to local application of ACh. A, Changes in fluorescence over time caused by the local application of ACh (20 µM) for 200 msec in normal physiological solution. Application of ACh caused a Ca²⁺ response in all PSCs studied. A second application 20 min later (break in the x-axis) induced smaller changes in fluorescence. B, Changes in fluorescence caused by the local application of ACh (20 µM, 200 msec) in the presence (solid line) and in the absence (dashed line) of external Ca²⁺ for the same PSCs. Ca²⁺ was replaced by 5 mM Mg²⁺. Note that ACh application induced larger changes in fluorescence in the absence of external Ca²⁺. C, Mean ± SEM of relative changes in Ca²⁺ responses induced by a first and a second application of ACh (20 µM) and for application of ACh in absence of external Ca²⁺.

We next investigated whether the rise in intracellular Ca²⁺ triggered by ACh was attributable to an entry of extracellular Ca²⁺ or caused by the release from intracellular stores. To distinguishbetween the two possibilities, extracellular Ca²⁺ was removed and replaced by a 5 mM Mg²⁺ physiological solution, and the ability of PSCs to respond tolocally applied ACh was tested again. As shown in Figure 3B, onall PSCs tested, Ca²⁺ responses were elicited by a local application of ACh in 0 Ca²⁺/5 Mg²⁺ 20 min after a first application in normal Ca²⁺, indicating that ACh induced the release of Ca²⁺ from internal stores. Surprisingly, the size of Ca²⁺ responses induced by ACh in 0 Ca²⁺/5 Mg²⁺ was significantly larger than the size of the responses obtainedin the presence of extracellular Ca²⁺ (421 ± 15% $Delta$ F/F vs 343 ± 22% $Delta$ F/F for control; n = 5; p = 0.001;Student's paired t test) (Fig. 3B,C). This indicates that, althoughthe contribution of internal stores is essential for the inductionof Ca²⁺ responses by ACh, the presence of extracellular Ca²⁺ downregulates the activation of the release of Ca²⁺ from internal stores by ACh (Fig. 3C).

Muscarinic receptors mediate ACh effects

For a better understanding of the role of glial cells at the synapse, it is necessary to further characterize the cellularreceptors and functions of these glial cells. To determine thetype of cholinergic receptors involved, we first used $alpha$ -BuTx,an antagonist of the nicotinic ACh receptors (AChRs). If Ca²⁺ responses to ACh were caused by nicotinic AChRs, they shouldbe blocked by the nicotinic cholinergic antagonist $alpha$ -BuTx. Totest the effectiveness of $alpha$ -BuTx (20 µM), preparations were perfusedwith the antagonist for at least 30 min before local applicationof ACh on PSCs was performed. This concentration blocks completelythe activity of the nicotinic postsynaptic receptors at the frogNMJ (Jahromi et al., 1992). As shown in Figure 4, A and B, theability of PSCs to respond to ACh was not affected by the presenceof $alpha$ -BuTx. Indeed, Ca²⁺ responses to ACh were still obtained in the presence of the toxinin all cells tested, and the size of the Ca²⁺ responses (317 ± 13% $Delta$ F/F; n = 5) was not significantly differentfrom the control responses obtained on the same cells before theapplication of $alpha$ -BuTx (Student's paired t test; p > 0.05).

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Figure 4. Ca²⁺ responses of PSCs to local application of muscarine. A, Changes in fluorescence caused by the local application of acetylcholine (20 µM, 200 msec) in the presence of $alpha$ -BuTx (20 µM). The increase in the intensity of fluorescence induced by the local application of ACh was unaffected by $alpha$ -BuTx. B, Comparison of mean ± SEM of Ca²⁺ responses induced by ACh alone, in the presence of $alpha$ -BuTx, and in the presence of atropine. C, Changes in fluorescence over time caused by the local application of muscarine (20 µM) for 200 msec in normal physiological solution. Application of muscarine caused a Ca²⁺ response in all PSCs studied. A second application 20 min later (break in the x-axis) induced smaller changes in fluorescence. D, Changes in fluorescence caused by the local application of muscarine (20 µM) in the presence (solid line) and in the absence (dashed line) of external Ca²⁺ for the same PSCs. Ca²⁺ was replaced by 5 mM Mg²⁺. Note that muscarine induced larger changes in fluorescence in the absence of external Ca²⁺. E, Comparison of mean ± SEM of Ca²⁺ responses induced by a first and a second application of muscarine (left) and application of muscarine in presence and absence of external Ca²⁺ (right).

The lack of effect of the nicotinic antagonist suggests that PSC AChRs are not nicotinic but rather, that the Ca²⁺ response induced by ACh was likely because of the activationof muscarinic receptors. If this were the case, muscarinic antagonistssuch as atropine should prevent Ca²⁺ responses to ACh. As shown in Figure 4B, the presence of atropinealmost completely abolished Ca²⁺ responses elicited by ACh in all cells tested (n = 15). The meansize of the responses was only 14 ± 6% $Delta$ F/F, which is significantlysmaller than the responses obtained from the same cells by a firstapplication of ACh (Student's paired t test; p = 0.001).

We next investigated the ability of the muscarinic agonist muscarine to evoke Ca²⁺ responses. Local application of muscarine (20 µM) induced a Ca²⁺ response in all cells on which it was applied (n = 15) with amean amplitude of 275 ± 43% $Delta$ F/F (Fig. 4C). Similar to our observationusing ACh, a second application of muscarine caused Ca²⁺ elevations that were significantly smaller than the ones obtainedwith a first application (150 ± 12% $Delta$ F/F; n = 9; p = 0.02; Student'spaired t test) (Fig. 4C,E).

If indeed ACh-induced Ca²⁺ responses are solely mediated by muscarinic receptors, muscarine-induced Ca²⁺ responses in PSCs should also be mediated by internal storeswith a regulation by extracellular Ca²⁺. This was tested by measuring Ca²⁺ responses in the absence of external Ca²⁺ where muscles were perfused with 0 mM Ca²⁺ and 5 mM Mg²⁺ for 30 min. In these conditions, application of muscarine (20µM) evoked Ca²⁺ responses that were significantly larger (360 ± 30% $Delta$ F/F; n =6; p = 0.003; Student's paired t test) (Fig. 4D,E) than the responsesobtained after a first application on the same cell in the presenceof Ca²⁺. These results indicate that, similarly to ACh-mediated Ca²⁺ responses, Ca²⁺ responses induced by muscarine were attributable to the releaseof Ca²⁺ from internal stores and regulated by extracellular Ca²⁺. As a whole, these data indicate that AChRs of the mammalianPSCs are of the muscarinictype.

Can ATP and adenosine trigger Ca²⁺ responses at the mammalian NMJ?

At the frog NMJ, application of ATP to PSCs induces the release of Ca²⁺ from internal stores (Jahromi et al., 1992; Robitaille, 1995)because of the activation of P_2X and P_2Y receptors (Robitaille,1995). To examine the involvement of endogenous purines in themodulation of mammalian PSCs in situ and to test whether ATP andadenosine can activate PSCs, changes in intracellular Ca²⁺ induced by local application of ATP and adenosine weremonitored.

ATP (20 µM) induced Ca²⁺ responses in all PSCs tested (299 ± 30% $Delta$ F/F; n = 41) (Fig. 5A), whereas local applications of adenosine(20 µM) resulted in a rise of fluorescence of 441 ± 51% $Delta$ F/F alsoin all PSCs tested (n = 19) (Fig. 5B). A second application ofATP evoked responses that were significantly smaller than thefirst response (207 ± 30% $Delta$ F/F vs 246 ± 38% $Delta$ F/F for control;n = 8; p = 0.0004) (Fig. 5A). Similarly, a second applicationof adenosine evoked responses that were significantly smallerthan the first response (314 ± 52% $Delta$ F/F vs 450 ± 77% $Delta$ F/F; n =11; p = 0.0004; Student's paired t test) (Fig. 5B).

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Figure 5. Ca²⁺ responses of PSCs to local application of ATP and adenosine. A, Changes in fluorescence over time caused by the local application of ATP (20 µM) for 200 msec in normal physiological solution. Application of ATP caused a Ca²⁺ response in all PSCs studied. A second application 20 min later (break in the x-axis) induced smaller changes in fluorescence. B, Changes in fluorescence over time caused by the local application of adenosine (20 µM) for 200 msec in normal physiological solution. Application of adenosine caused a Ca²⁺ response in all PSCs studied. A second application 20 min later (break in the x-axis) induced smaller changes in fluorescence. C, Changes in fluorescence caused by the local application of ATP (20 µM, 200 msec) in the presence (solid line) and in the absence (dashed line) of external Ca²⁺ for the same PSCs. Note that ATP induced larger changes in fluorescence in the absence of external Ca²⁺. D, Changes in fluorescence caused by the local application of adenosine in the presence (solid line) and in the absence (dashed line) of external Ca²⁺ for the same PSCs. Note that adenosine induced larger changes in fluorescence in the absence of external Ca²⁺. E, Comparison of mean ± SEM of Ca²⁺ responses induced by a first and a second application of ATP (left) and the application of ATP in the presence and in the absence of external Ca²⁺ (right). F, Comparison of mean ± SEM of Ca²⁺ responses induced by a first and a second application of adenosine (left) and application of adenosine in the presence and in the absence of external Ca²⁺ (right).

In most glial cells (Salter and Hicks, 1994), including PSCs at the amphibian NMJ (Jahromi et al., 1992; Robitaille, 1995),purinergic agonists elicit an elevation in intracellular Ca²⁺ that involves the release of Ca²⁺ from internal stores. This possibility was tested by replacingextracellular Ca²⁺ ions by Mg²⁺ (5 mM). As shown in Figure 5C, Ca²⁺ responses induced by local application of ATP still induced Ca²⁺ responses in all mammalian PSCs tested, even in the absence ofCa²⁺ in the solution, pointing toward a critical role of Ca²⁺ internal stores in the production of the Ca²⁺ responses. On average, the amplitude of the Ca²⁺ responses was 461 ± 98% $Delta$ F/F. However, similar to ACh-inducedCa²⁺ responses, local application of ATP in absence of extracellularCa²⁺ evoked Ca²⁺ responses that were significantly larger than the ones evokedby a first application of ATP on the same cells (273 ± 42% $Delta$ F/Ffor control; n = 11; p = 0.02; Student's paired t test) (Fig.5C). Similarly, adenosine also caused Ca²⁺ responses in absence of external Ca²⁺ that were significantly larger than those obtained in the presenceof Ca²⁺ (497 ± 72% $Delta$ F/F vs 428 ± 6% $Delta$ F/F; n = 8; p = 0.001; Student'spaired t test) (Fig. 5D). These results indicate that PSCs atthe mammalian NMJ detect adenosine and ATP and that these substancesinduce the release of Ca²⁺ from internal stores via a mechanism that is negatively regulatedby external Ca²⁺ (Fig. 5E,F).

Are purinergic receptors present on PSCs?

To verify the presence of adenosine and ATP receptors on the mammalian PSCs, the ability of these agonists to evoke Ca²⁺ responses in PSCs was tested in the presence of antagonists forP2 and P1 receptors. Suramin, a nonselective P2 receptor antagonistwas first tested. Ca²⁺ responses induced by ATP should be abolished in the presenceof this antagonist if they are mediated by the activation of P2receptors. After eliciting a Ca²⁺ response by ATP on PSCs, the preparations were perfused withsuramin (100 µM), and the ATP was applied locally on the samecells. As shown in Figure 6, Ca²⁺ responses were still induced by local applications of ATP (20µM) (289 ± 34% $Delta$ F/F; n = 6) (Fig. 6A), and the average amplitudeof the responses was not significantly different from responsesevoked by the same cells before application of the antagonist(Student's paired t test; p = 0.239). It is unlikely that thelack of effect was attributable to the inability of suramin toblock P2 receptors because the same solution blocked ATP-inducedresponses at PSCs of amphibian NMJs (Robitaille, 1995). Hence,this result suggests that ATP raised intracellular Ca²⁺ by mechanisms that do not activate P2 receptors.

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Figure 6. Ca²⁺ responses of PSCs to local application of ATP and adenosine in presence of purinergic antagonists. A, Changes in fluorescence caused by the local application of ATP before and after (break in the x-axis) a 20 min perfusion with suramin (100 µM), a nonspecific P2 antagonist. Note that the increase in the intensity of fluorescence induced by the local application of ATP was unaffected by the presence of suramin. B, Changes in fluorescence caused by the local application of adenosine before and after a 20 min perfusion with CPT (10 µM). C, Changes in fluorescence in four PSCs of an NMJ caused by the local application of ATP in the presence of the A1 receptor antagonist CPT (20 µM). Inset, False color confocal images of the four PSCs at rest (Rest), at the peak of the Ca²⁺ response (Peak), and after recovery (Recov). Note that the increase in the intensity of fluorescence induced by the local application of ATP was unaffected by the presence of CPT. Scale bar, 10 µm.

However, Ca²⁺ responses evoked by adenosine were almost completely abolished in the presence of CPT (10 µM), an A1 receptorantagonist (32 ± 6% $Delta$ F/F; n = 5) (Fig. 6B). This value was significantlysmaller than the responses obtained on the same cells before theapplication of the antagonist in the perfusate (Student's pairedt test; p = 0.001). This suggests that the adenosine-induced Ca²⁺ responses were mediated by the activation of A1receptors.

Ectoenzymes present in the synaptic cleft (Salter et al., 1993; Ziganshin et al., 1993) will cause the dephosphorylation ofATP and lead to adenosine formation. Because adenosine appearsas an active substance at the mammalian NMJ and because ATP canbe exogenously degraded into adenosine, it is possible that theCa²⁺ responses evoked by local applications of ATP were attributableto the indirect activation of A1 receptors. This possibility wastested by locally applying ATP in the presence of CPT. As shownin Figure 6C, the presence of CPT (10-20 µM) in the perfusiondid not block Ca²⁺ responses induced by ATP. The average amplitude of the Ca²⁺ responses was 384 ± 86% $Delta$ F/F (n = 7), which is not significantlydifferent from control (ANOVA; p > 0.05). These results suggestthat the action of ATP was not mediated by an indirect activationof A1 receptors and, hence, would be produced by other ATP-dependentmechanisms.

Endogenous ACh and adenosine mediate nerve-evoked Ca²⁺ responses in PSCs

Our results indicate that functional muscarinic and A1 adenosine receptors are present on PSCs of the mammalian NMJ. We nextwondered whether ACh and adenosine released by the presynapticterminal during synaptic activity could mediate the activationof PSCs and the triggering of the nerve stimulation-evoked Ca²⁺ responses in PSCs. Because nerve-evoked Ca²⁺ responses decrease during consecutive trains of stimuli (Fig.2A), the effects of the two different blockers on nerve-evokedCa²⁺ responses were tested on different preparations, and each preparationwas stimulated onlyonce.

We first examined the impact of blockade of ACh receptors on nerve-evoked Ca²⁺ responses. The blockade of ACh receptors with atropine (20 µM)greatly reduced the amplitude of Ca²⁺ responses induced by stimulation of the motor nerve to 33 ± 3% $Delta$ F/F (n = 5) (Fig. 7A). This value is significantly smaller thanthe one obtained in the absence of atropine (157 ± 15% $Delta$ F/F; one-wayANOVA, p < 0.05) (Fig. 7A, gray zone), indicating that the activationof ACh receptors was necessary for optimal Ca²⁺ responses and, hence, activation of PSCs during synaptic transmission.The remnant of Ca²⁺ responses still induced by synaptic activity was not caused bythe inefficacy of atropine because local applications of muscarineon the same cells tested in these experiments could not elicitany Ca²⁺ responses (data not shown).

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Figure 7. Nerve-evoked Ca²⁺ responses in PSCs in presence of atropine and CPT. A, Changes in fluorescence of a PSC before, during (bar), and after repetitive motor nerve stimulation (50 Hz, 30 sec) after 20 min perfusion with atropine (20 µM), a muscarinic antagonist. The boxed gray zone illustrates the mean ± SEM of nerve-evoked Ca²⁺ responses obtained from the 10 PSCs in absence of any antagonists (Fig. 2A). B, Changes in fluorescence of a PSC before, during (bar), and after repetitive motor nerve stimulation (50 Hz, 30 sec) after 20 min perfusion with CPT (10 µM), an A1 antagonist. The gray zone illustrates the mean ± SEM of nerve-evoked Ca²⁺ responses obtained from the 10 cells in absence of any antagonists. C, Changes in fluorescence of a PSC before, during (bar), and after repetitive motor nerve stimulation (50 Hz, 30 sec) after 20 min perfusion with CPT (10 µM) and atropine (20 µM). Note that the repetitive stimulation of the motor nerve did not induce any Ca²⁺ response in the PSC. After a recovery period of 5 min, ATP (20 µM) was locally applied on the PSC, which elicited a Ca²⁺ response.

We next tested the impact of the A1 antagonist CPT on Ca²⁺ responses evoked by stimulation of the motor nerve. As shown in Figure7B, Ca²⁺ responses were reduced to 98 ± 6% $Delta$ F/F (n = 6) (Fig. 7B) in thepresence of CPT. Although the reduction in the size of Ca²⁺ responses was more modest than the effect of the muscarinic antagonist,the size of the Ca²⁺ responses was significantly smaller than the control ones (one-wayANOVA; p < 0.05) (Fig. 7B, gray zone). This indicates that theactivation of adenosine receptors is important to generate theCa²⁺ responses induced by nerve-evoked transmitter release. The partialblockade of the responses was not attributable to the inefficacyof CPT to antagonize the A1 receptors because local applicationof adenosine on the same cells did not induce any Ca²⁺ responses (data notshown).

Finally, we tested the impact on Ca²⁺ responses of both the muscarinic and A1 receptor antagonists together. As shown in Figure7C, Ca²⁺ responses were primarily reduced in the presence of the two antagonistsin which the mean Ca²⁺ response was only 22 ± 8% (N = 4; n = 8). This value is significantlydifferent from the mean response obtained in control condition(i.e., without any antagonist; one-way ANOVA, p < 0.05). The remainingCa²⁺ elevation is consistent with the Ca²⁺ response observed when transmitter release was blocked using $omega$ -CgTx MVIIC, possibly because of the depolarization of PSCs byK⁺ accumulation during repetitive nerve stimulation. The inabilityto elicit Ca²⁺ responses was not caused by a lack of cell responsivity becauselocal application of ATP (brake in x-axis) induced Ca²⁺ responses in all cells tested (N = 3; n =7).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We present here direct evidence that mammalian PSCs in situ respond to the release of neurotransmitters induced by stimulationof the motor nerve, as indicated by an elevation of intracellularCa²⁺ level. This elevation originated mainly from the release of Ca²⁺ from internal stores and muscarinic and adenosine A1 receptorsare the main two receptor systems involved in the communicationbetween the nerve terminal and the PSCs. Furthermore, extracellularCa²⁺ negatively affects the ability of PSCs to respond to neurotransmitters.It is concluded that, like glial cells at other synapses, synapse-gliainteractions are also taking place at the mammalian NMJ but withparticularities associated with thissynapse.

Cholinergic receptor on the mammalian PSCs

When expressed by glial cells, including PSCs of the amphibian NMJ (Robitaille et al., 1997), cholinergic receptors have alwaysbeen determined to be of the muscarinic type, mainly linked tointernal Ca²⁺ stores regulated by an inositol 1,4,5-trisphosphate receptor(Hamprecht, 1986). Here we show that PSCs of the mammalian NMJare no exception and that the cholinergic receptors are of themuscarinic type as indicated by the lack of effects of nicotinicantagonists and by the ability of muscarine to induce Ca²⁺ responses, whereas atropine blocked ACh-induced responses. Theblockade of Ca²⁺ responses by the nonspecific muscarinic antagonist atropine alsoindicates that PSCs of the mammalian NMJ, unlike the ones at theamphibian NMJ, express a typical muscarinic pharmacology (Robitailleet al., 1997). Moreover, muscarinic-dependent Ca²⁺ responses in glial cells also share another characteristic, thatis, the rundown of the response after repetitive applicationsof cholinergic agonists (Dave et al., 1991; Jahromi et al., 1992;Robitaille et al., 1997).

Purinergic receptors on the mammalian PSCs

It is now established that ATP is released during synaptic transmission (Smith, 1991; Zimmermann, 1994) and is involved inintercellular signaling in various systems (Sneddon and Burnstock,1984; Benham, 1989; Salter and Hicks, 1994; Zimmermann, 1994;Lyons et al., 1995). Adenosine and ATP receptors are widely distributed(Burnstock, 1990; Salter et al., 1993) and are present on severaltypes of glial cells such as cultured astrocytes (Lai and Wong,1991; Salter and Hicks, 1994), glioma cells (Chueh et al., 1994),microglial cells (Walz et al., 1993), and glial cells of the ratoptic nerve (Kriegler and Chiu, 1993). Moreover, ATP appears necessaryfor the spread of Ca²⁺ waves in a syncytium of astrocytes (Guthrie et al., 1999).

The results of the present study suggest that PSCs possess adenosine receptors of A1 type, as indicated by the blockade ofadenosine-induced Ca²⁺ responses by CPT, an A1 receptor antagonist. However, and somewhatunexpectedly, Ca²⁺ responses induced by local applications of ATP were not blockedby suramin, a nonspecific P2 receptor antagonist indicating thatthe effects observed with ATP were not attributable to the activationof P2 receptors. In addition, adenosine released during synapticactivity triggers Ca²⁺ responses, as indicated by the significant reduction of Ca²⁺ responses elicited by nerve stimulation in the presence of CPT.However, at the amphibian NMJ, ATP released during synaptic transmissionactivates PSCs, whereas endogenous adenosine had no apparent effecton nerve-evoked Ca²⁺ responses (Robitaille, 1995).

Because of the presence of ecto-ATPases (Zimmermann, 1994), one possibility might have been that ATP-induced responses werecaused by the indirect activation of adenosine receptors as aconsequence of ATP degradation into adenosine. However, our resultsare not consistent with this possibility because ATP-induced Ca²⁺ responses persisted even in the presence of the adenosine receptorantagonist. An alternative possibility might be that ATP actedvia ectoprotein-kinases because they are known to be located onthe surface of several cells (Zimmermann, 1994) and that theyrequire the presence of Mg²⁺ ions (Ehrlich et al., 1986), conditions in which our experimentswereperformed.

Glial cells detect neuronal activity and synaptic transmission

Glial cells at CNS synapses detect the release of neurotransmitters induced by neuronal activity (Porter and McCarthy, 1996,1997; Carmignoto et al., 1998; Grosche et al., 1999). This doesnot require the activation of a complex multicellular networkbecause similar results were obtained at the frog NMJ where PSCsdetect and are modulated by synaptic activity generated by a singlesynapse (Jahromi et al., 1992; Georgiou et al., 1994, 1999; Robitaille,1995; Robitaille et al., 1997; Bourque and Robitaille, 1998).

The data presented here demonstrate that mammalian PSCs can also detect synaptic activity and that a number of Ca²⁺-dependent cascades of events are likely triggered in PSCs asa consequence of the Ca²⁺ elevations. This observation is consistent with the propertiesreported for all other synapses at which synapse-glia interactionshave been studied (Araque et al., 1999; Castonguay et al., 2001).Indeed, synaptic activity will trigger an elevation of intracellularCa²⁺ in PSCs as a result of its release from internal stores. Moreover,this activation is frequency dependent and is regulated by themain neurotransmitters present at the synapse, regulating G-protein-coupledreceptors. Hence, the results obtained at the mouse NMJ furthersupport the concept that synapse-glia interactions are ubiquitousat chemical synapses where glial processes arepresent.

Because synapse-glia interactions are dependent on the release of neurotransmitters by chemical synapses (Araque et al., 1999;Castonguay et al., 2001), it is expected that the activity ofperisynaptic glial cells will be governed by the main neurotransmittersfound at the synapses with which they are associated. In the presentstudy, it is shown that PSCs activation requires the release ofneurotransmitter, as shown by the blockade of transmitter releasewith $omega$ -CgTx MVIIC. In particular, ACh released during synaptictransmission modulates the activity of the PSCs because Ca²⁺ responses were almost completely abolished in the presence ofthe muscarinic receptor antagonist atropine. Consistent with thisobservation and similar to ACh-induced Ca²⁺ responses, we found that Ca²⁺ responses induced by evoked transmitter release also showed apronounced rundown when elicited by repetitive trains of stimuli.This property was also present at PSCs of the amphibian NMJ (Jahromiet al., 1992) where a large part of this rundown was shown tobe caused by endogenously released substance P that activatesNK-1 receptors leading to reduced efficacy of purinergic and muscarinicreceptor systems (Bourque and Robitaille, 1998).

Functional differences of mammalian and amphibian PSCs

Although mammalian and amphibian PSCs share a number of properties, there are a few major functional differences (Table 1).First, the type of receptors present are different. Indeed, PSCsof the amphibian NMJ lack sensitivity to general muscarinic antagonists,in particular to atropine, whereas we showed in this study thatmammalian PSCs were atropine-sensitive. Also, the purinergic receptorsare different because, unlike mouse PSCs, there is evidence inamphibian PSCs of two ATP receptor subtypes (P_2X, P_2Y) in additionto A1 receptors (Robitaille, 1995). The second major differenceresides in the molecular machinery associated with the receptors.Indeed, repetitive Ca²⁺ elevations were observed in mammalian PSCs after single applicationsof muscarine or stimulation of the motor nerve. This was not observedat amphibian PSCs where muscarine induced a single, large increasein Ca²⁺ (Jahromi et al., 1992; Robitaille, 1995; Robitaille et al., 1997).Moreover, the Ca²⁺ responses appear negatively regulated by external Ca²⁺ at mammalian but not at amphibian PSCs. The presence of the negativeregulation by external Ca²⁺ are consistent with a calcium-dependent/calcium-release phenomenonthat would only be present in mammalian PSCs. This negative Ca²⁺ regulation may contribute to the genesis of the repeated Ca²⁺ elevations observed in PSCs and to the more pronounced rundownof consecutive Ca²⁺ responses elicited at mammalian PSCs. These differences willhave major impacts on the functions of PSCs because differenttypes of receptors will have different regulatory actions resultingthe production of different second messengers. Also, the differentCa²⁺ regulation in PSCs will result in the induction of differentCa²⁺-dependent mechanisms. Hence, although amphibian and mammalianNMJs show fundamental synapse-glia interactions, the propertiesof these interactions differ.


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Table 1. Comparison of the properties of PSCs at mammalian and amphibian NMJs

Properties of synapse-glia interactions as a function of synapse identity

Based on our data, we propose that, although synapse-glia interaction is a common phenomenon at chemical synapses associatedwith glial cells, the nature and the extend of the interactionswill be fine-tuned according to the properties and function ofthe synapse with which they are associated. Because perisynapticglial cells are involved in the modulation of synaptic transmission(Parpura et al., 1994; Robitaille, 1998; Araque et al., 1999;Castonguay et al., 2001), their involvement in the regulationof synaptic functions will be tuned according to their functionalproperties and, hence, adjusted to their synaptic environment.This adaptation to the synaptic environment is essential for perisynapticglial cells to actively and effectively modulate synaptic efficacyand neuronal activity. Thus, it will be critical to establishthe properties of the regulation of synaptic efficacy by PSCsat the mouse NMJ and determine how the different properties ofPSCs at this synapse will influence their regulation of synapticactivity. Moreover, because of the importance of PSCs in the regulationof numerous crucial aspects of the synapse, a malfunction of Schwanncells (Scherer, 1997) will undoubtedly impair itsfunctions.

  FOOTNOTES

Received Nov. 2, 2000; revised March 16, 2001; accepted March 19, 2001.

This work was supported by Grant MT14137 from the Canadian Institute of Health Research (CIHR), by awards from the EJLB ResearchFoundation and The Alfred P. Sloan Foundation, and by a team grantfrom Fonds pour la Formation de Chercheurs et de l'aide à laRecherche to R.R. I.R. was sponsored by a studentship from Schering,and R.R. was a Junior II Scholar from the Fonds de la Rechercheen Santé du Québec and a CIHR Investigator. We thank Rhoda L.Kenigsberg and Vincent F. Castellucci for their comments and suggestionson thismanuscript.
Correspondence should be addressed to Richard Robitaille, Département de physiologie, Université de Montréal, P. O. Box6128, Station "Centre-Ville", Montréal, Quebec, Canada H3C 3J7.E-mail: richard.robitaille{at}umontreal.ca.

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