Limits to the Development of Fast Neuromuscular Transmission in Zebrafish

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Limits to the Development of Fast Neuromuscular Transmission in Zebrafish

Pierre Drapeau,¹ Robert R. Buss,¹ Declan W. Ali,¹ Pascal Legendre,² and Richard L. Rotundo³

¹Centre for Research in Neuroscience, Montreal General Hospital Research Institute, Department of Neurology and Neurosurgery, and Department of Biology, McGill University, Montreal, Quebec H3G 1A4, Canada; ²Institut des Neurosciences, Centre National de la Recherche Scientifique-Unité Mixte de Recherche 7624, Université Pierre et Marie Curie, 75252 Paris, France; and ³Department of Cell Biology and Anatomy, University of Miami School of Medicine, Miami, Florida 33136

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Drapeau, Pierre, Robert R. Buss, Declan W. Ali, Pascal Legendre, and Richard L. Rotundo. Limits to the Development of Fast Neuromuscular Transmission in Zebrafish. J. Neurophysiol. 86: 2951-2956, 2001. Zebrafish embryos have small and slow miniature end-plate currents (mEPCs), whereas only a few days later larval mEPCs arean order of magnitude larger and faster, being among the fastestof all neuromuscular synapses. To identify the bases for thesechanges we compared, in embryos and larvae, the properties anddistributions of acetylcholine (ACh) receptors (AChRs) and acetylcholinesterase(AChE) as well as the ultrastructure of the developing neuromuscularjunctions (NMJs). To mimic synaptic release, patches of musclemembrane were exposed briefly (for 1 ms) to a saturating concentration(10 mM) of ACh. The AChR deactivation kinetics were twice as slowin embryos compared with larvae. In both embryos and larvae, AChRsdemonstrated open channel block by millimolar ACh, and this wasdetected during mEPCs, indicating that a high concentration ofACh is released at immature and mature NMJs. AChR and AChE distributionswere compared using the selective fluorescently conjugated labels $alpha$ -bungarotoxin and fasciculin 2, respectively. In larvae, punctateAChR clusters were detected whereas junctional AChE staining wasless intense than that found at adult NMJs. Transmission electronmicroscopy revealed immature nerve endings in embryos that wereclosely juxtaposed to the surrounding muscle cells, whereas maturelarval NMJs had a wider synaptic cleft with a conspicuous basallamina over a limited region of synaptic contact. Our resultsindicate that ACh is released at high concentrations at immatureNMJs, but its clearance is prolonged and the AChRs are dispersed,resulting in a slow mEPC time course until a mature cleft appearswith densely packed faster AChRs and abundantAChE.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Although much is known about the molecular aspects of neuromuscular junction (NMJ) assembly (Hall and Sanes 1993; Sanes andLichtman 1999), there is less information about how functionaltransmission is established in vivo. Embryonic junctional potentialsin a variety of preparations are small, slow, and variable (Grinnell1995), and how they are transformed into large, fast and uniformmature events is unclear. The speculation ranges from changesin presynaptic release of acetylcholine (ACh) to the postsynapticdensity of ACh receptors (AChRs) and acetylcholinesterase (AChE)but the exact mechanism remainsunknown.

The zebrafish is an interesting preparation for the physiological study of NMJ development due to the accessibility of theembryo (Buss and Drapeau 2000; Liu and Westerfield 1988; Nguyenet al. 1999; Westerfield et al. 1986). The miniature end-platecurrents (mEPCs) in day-old zebrafish embryos, particularly insuperficial muscle cells, have small and variable amplitudes andslow time courses (Nguyen et al. 1999). Two days later in newlyhatched larvae, mEPCs are observed more frequently and are muchlarger and faster. Indeed these mEPCs are among the fastest NMJs(Macdonald and Balnave 1984), consistent with the zebrafish beingone of the fastest swimming teleosts of its size (Plaut 2000).

The developmental increase in frequency of zebrafish mEPCs is thought to be due to an increased density of innervation asthe muscle cells become poly-innervated (Myers 1985) and remainso in the adult (Westerfield et al. 1986). The increase in mEPCamplitude may be due to an increased density of AChRs (Liu andWesterfield 1992). It could also reflect a slowing of ACh clearanceor an increase in the content of the transmitter quantum. Theorigin of the acceleration in the time course of the mEPCs remainsunresolved. It is due partly to a gradual loss of the electricalcoupling between muscle fibers that filters extraneous eventsbut also reflects the appearance of faster synaptic events (Bussand Drapeau 2000). How these faster events develop remainsunknown.

AChR channels with similar brief openings were observed during stationary exposure to submicromolar ACh in both embryonicand larval muscle cells, and blocking AChE with eserine slowedthe mEPC time course in larvae, but not embryos, by twofold (Nguyenet al. 1999). These observations suggested that a change in AChRor AChE properties is insufficient to account entirely for theorder of magnitude acceleration in mEPC time course. When larvalAChRs are activated under more physiological conditions with brief(1 ms) application of saturating (1-10 mM) ACh, they are blockedinitially by positively charged ACh (K_0.5 = 0.5 mM) entering theopen channels (Legendre et al. 2000). During synaptic transmissionat mature larval NMJs, this yields a rebound current on recoveryfrom open channel block when ACh is removed from the cleft. Theoccurrence of open channel block can thus serve to detect thepresence of a high concentration of released ACh. In the presentstudies, we examined the properties and distributions of AChRsand AChE and the ultrastructure of the NMJ in zebrafish embryosand larvae to determine their relative contributions to the maturationof fast neuromusculartransmission.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Zebrafish (Danio rerio) were obtained from breeding colonies (Westerfield 1995) and were anesthetized with tricaine beforestarting the experimentalprocedures.

Electrophysiology

Isolated patch recordings were obtained as described by Legendre (1998), and the extracellular recording solution (Legendreand Korn 1994) was modified to contain less Ca (0.6 mM) and moreMg (10 mM) to suppress contractions. Outside-out patches (Hamillet al. 1981) were obtained from near the middle of the musclefibers as the small size of the NMJs prevented us from directlylocating them. Fast-flow applications were performed by rapidlymoving (in <0.1 ms) a twin-barreled application pipette acrossthe patch pipette, which was displaced with a piezoelectric translator(Model No. P245.30, Physic Instruments). One barrel containedextracellular solution and the other contained in addition 10mM ACh. Current was recorded with an Axopatch-1D amplifier (AxonInstruments), filtered at 10 kHz ( $-$ 3 dB), and stored using a digitaltape recorder. Data were acquired with pClamp 6.0 software (AxonInstruments) by digitizing at 50 kHz and were analyzed off-linewith Axograph 3.5 software (AxonInstruments).

Extracellular focal mEPC recordings were obtained as described in Xenopus by Kullberg et al. (1977, 1980) by placing an extracellularelectrode at the myoseptal junctions of superficial muscle fibers.Spontaneously occurring synaptic activity was recorded using anAxoclamp 2A (Axon Instruments) in bridge mode. Recordings wereperformed and analyzed as described in the precedingtext.

The mEPCs were recorded in the whole cell mode as described previously (Nguyen et al. 1999) in the presence of 250 nM tetrodotoxinusing pipettes with a series resistance of 4-5 M $Omega$ that was compensatedby 70-80%. The recordings were made using an Axopatch 1-D (AxonInstruments), were filtered at 2 kHz, and were analyzed as describedin the precedingtext.

Histology

Zebrafish were anesthetized, skinned and fixed for 1 h at room temperature in phosphate-buffered saline (PBS) containing 2%paraformaldehyde. Small clusters of fixed muscle fibers were isolatedfrom the adult trunk musculature. The fixed preparations wererinsed with PBS and labeled with $alpha$ -bungarotoxin ( $alpha$ -BTX) conjugatedto Oregon Green and fasciculin (Fas2) conjugated to rhodamineor Oregon Green as described by Peng et al. (1999). The tissueswere incubated for 10 min in PBS containing 10% horse serum (PBS/HS)to reduce background, then incubated for 30-60 min in the samebuffer containing 1 µg/ml fluorescent $alpha$ -BTX and Fas2. After washingfor 30 min in several changes of PBS/HS, the muscle fibers weremounted in 90% buffered glycerol (pH 8.5) containing 1 mg/ml p-phenylenediamineto reducephotobleaching.

Histochemical staining for AChE was performed according to Vacca (1995). Briefly, whole embryos or larvae were fixed overnightin maleate buffer containing 4% paraformaldehyde and treated for2 h with Triton X-114 prior to incubation with the buffer-substratemixture containing acetylthiocholine. AChE was not detected incontrol preparations incubated without substrate or with substrateand 0.5 mM eserine to inhibit esterase activity (notshown).

Biochemical assay of AChE activity

AChE was extracted from whole larvae or isolated adult muscle by homogenization in 10 volumes (wt:vol) borate extraction buffer[20 mM Na borate, pH 9.0, 1.0 M NaCl, 5 mM EDTA, 1% Triton X-100,and a protease inhibitor cocktail (as described in Rotundo 1984)]and centrifuged for 20 min at 14,000g. Aliquots of the supernatantwere analyzed by velocity sedimentation on 5-20% sucrose gradientsas previously described (Rotundo 1984). The AChE activity in eachfraction was determined using a radiometric assay (Johnson andRussell 1975) and the resulting relative counts per minute (CPM)plotted. Markers consisting of Escherichia coli $beta$ -galactosidase(16 s) and alkaline phosphatase (6.1 s) were routinely includedin the samples and assayed using standardprocedures.

Electron microscopy

Dechorionated embryos and larvae were anesthetized and fixed overnight at 4°C in PBS containing 3% glutaraldehyde, washedwith PBS, and postfixed for 1 h at room temperature in 2% OsO₄in PBS. The samples were then washed and dehydrated in an alcoholseries and embedded in Epon. Thin cross sections were counter-stainedwith lead citrate and viewed using a JEOL CX-100 transmissionelectronmicroscope.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Fast AChR kinetics and open channel block

We compared the properties of embryonic and larval AChRs using fast-flow perfusion of membrane patches isolated from musclecells. As shown in Fig. 1A, application of 10 mM ACh for 1 msto an outside-out patch from a 1-day-old embryo activated a steadyoutward current at +50 mV (average of 8 trials shown). On removalof the ACh, the current decayed monoexponentially (decay timeconstant $tau$ = 0.39 ms). At $-$ 50 mV, the same patch showed initiallya smaller steady inward current in the presence of ACh (Fig. 1A)due to open channel block (Legendre et al. 2000). On removal ofthe ACh there was a large, delayed rebound current that decayedmore slowly ( $tau$ = 0.51 ms) during recovery from the block. Whenthe same protocol was used with a patch from a 3-day-old larva,a similar result was obtained (Fig. 1B). The AChR currents observedat $-$ 50 mV at both stages had similar activation time courses (20-80%rise time, RT = 0.05-0.06 ms; Fig. 1C), but the embryonic currentsdecayed twice as slowly [ $tau$ = 0.55 ± 0.24 (SD) ms, n = 7] as thelarval currents ( $tau$ = 0.27 ± 0.06 ms, n = 10; P < 0.01; Fig. 1D).However, this was only a minor difference in time course whencompared with the much slower mEPCs (RT ~ 2 ms, $tau$ = 5-10 ms) observedin superficial embryonic muscle cells (Nguyen et al. 1999) (Fig.1E). Open channel block (K_0.5 = 0.5 mM) was not observed at submillimolarconcentrations of ACh, resulting in voltage-independent time courses(Legendre et al. 2000; Nguyen et al. 1999).

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Fig. 1. Fast kinetics of acetylcholine (ACh) receptors (AChRs). Responses of outside-out patches from embryonic (A) and larval (B) muscle to 1 ms application of 10 mM ACh, shown by the line drawings at top. Top traces: averages of 8 responses from the same patches that were recorded at either +50 mV (top) or $-$ 50 mV (bottom). The decay phases are fit with monoexponential functions with the indicated values of $tau$ . Histograms (bars indicate ± SE) of (C) the 20-80% rise times (RT) and (D) the values of $tau$ recorded in patches from embryos (day 1,

, n = 7) and in patches (

, n = 10), and extracellular recordings (

, n = 3) from larvae (day 3). E: scaled averages of miniature end-plate currents (mEPCs) recorded in an embryonic (27 h) muscle fiber at $-$ 30 mV (13 mEPCs) and $-$ 110 mV (27 mEPCs). F: average of 113 focal mEPCs from a 3-day-old larva fitted with a monoexponential function with the indicated value of $tau$ .

As the isolated patches were likely from extrasynaptic regions, we next examined whether synaptic AChRs had similar properties.The mEPCs recorded in whole cells (Legendre et al. 2000; Nguyenet al. 1999) were found to be somewhat slower than the singleAChR currents (Legendre et al. 2000). This could be due to a differencebetween synaptic and extrasynaptic AChRs or perhaps to a technicallimitation with whole cell recording due to the large size ofthe muscle fibers. To overcome this technical limitation, extracellularvoltage recordings were made of the junctional currents underlyingspontaneous events (focal mEPCs) in larval muscle fibers. The20% largest events were selected for averaging (Fig. 1F; mean= 90 ± 2 µV) as they were presumably the most accurate recordingsof events occurring closest to the electrode. The focal mEPCshad similar kinetics (RT = 0.07 ± 0.01 ms, $tau$ = 0.220 ± 0.003 ms)as the larval AChRs recorded in isolated membrane patches, indicatingthe presence of similar synaptic and extrasynaptic AChRs, as reportedfor other NMJs (Edmonds et al. 1995; Schuetze and Role 1987).

One possible explanation for the slow activation of embryonic mEPCs is that a low (submillimolar) concentration of ACh isreleased at immature synapses. If this was so, then open channelblock should be less effective. Because embryonic muscles contractedat strongly depolarized potentials, we compared the time courseof whole cell mEPCs in fibers held at $-$ 30 mV, where the blockshould be lower, and at $-$ 110 mV, where the block should be maximal(Legendre et al. 2000). As shown in Fig. 1E, for the averagesof the largest 20% of the recorded mEPCs, which permitted reliabledetection and comparison, similar rise times were observed ateither potential: 0.60 ± 0.08 ms at $-$ 30 mV and 0.72 ± 0.08 msat $-$ 110 mV (n = 6; P = 0.36 by signed-rank test). However, thedecay time course of embryonic mEPCs was 26 ± 6% slower at themore negative potential ( $tau$ = 4.4 ± 0.6 ms at $-$ 30 mV and $tau$ = 5.7± 0.5 ms at $-$ 110 mV; n = 6; P = 0.03). [These values for RT and $tau$ are somewhat smaller than those reported by Nguyen et al. (1999)due to selection of the largest events.] The larger value of $tau$ at the more negative potential indicates that open channel blockalso occurred at embryonic NMJs, reflecting the release of a high(millimolar) concentration of ACh that should not limit the timecourse of the mEPCs to the extentobserved.

Slower increase in density of AChE vs. AChR

As the twofold change in AChR kinetics was insufficient to account for the order of magnitude acceleration in time courseof the junctional currents, we examined the distribution and propertiesof AChRs and AChE. AChRs cluster a few hours after motoneuronscontact muscle cells (Liu and Westerfield 1992). In embryos, AChEis present at myoseptal junctions (Hanneman and Westerfield 1989),and in adult zebrafish, it is localized both at the myoseptaljunctions and at the multiple, poly-innervating NMJs running orthogonallyacross deeper fibers (Mos et al. 1983). We examined the patternof AChE distribution in comparison with AChRs to determine whetherit is synaptically localized by the time of maturation of junctionaltransmission inlarvae.

The distribution of these molecules was compared simultaneously by labeling them with the AChE-selective toxin Fas2 and AChR-selective $alpha$ -BTX (Peng et al. 1999). Clustered AChE was undetectable withFas2 at either embryonic or larval NMJs (the latter is illustratedin Fig. 2A). Because the presence of AChE was detected pharmacologicallyin larvae as a twofold reduction in mEPC time course followingblock by eserine (Nguyen et al. 1999), we also carried out a standardhistochemical stain. We were thus able to detect AChE at myoseptaljunctions in embryos, as reported previously (Hanneman and Westerfield1989), and at myoseptal junctions and end plate regions alongdeep muscle fibers in larvae (Fig. 2B).

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Fig. 2. Distribution of AChRs and AChE. A: staining of 4-day larval muscle AChE with Oregon Green-Fas 2. B: standard histochemical stain for AChE in a 3-day larva. Note the V-shaped myotomal junctions. C: staining of AChE in adult muscle fibers and at mysoseptal junctions (D: horizontal bands at top) with Oregon Green-Fas 2. E: staining of AChRs in 4-day larval muscle with Oregon Green- $alpha$ -bungarotoxin ( $alpha$ BTX; same preparation as in A). F: staining of AChRs in adult muscle fibers with Oregon Green- $alpha$ BTX. The dark spots in A, B, and E are pigmented skin cells. The scale bar is 46 µm in A and in C-F and 50 µm in B.

As a control to be sure that Fas2 could effectively stain zebrafish AChE and that a lack of staining in embryos and larvaewas thus not an artifact due to a lack of Fas2 binding, we alsoexamined the staining pattern in adult muscle fibers. Strong fluorescentstaining was detected as string-like clusters of AChE (Fig. 2C)and at myoseptal junctions (Fig. 2D) in the adult fibers. ThusFas2 could label zebrafish AChE but it appeared to be less welllocalized in larvalmuscle.

In contrast to the weak AChE staining in larvae (Fig. 2A), small and broadly distributed AChR clusters were detected alongthe fibers and at the myoseptal junctions (Fig. 2E; same preparationas in A). In isolated adult muscle fibers, long continuous stringsof AChRs were observed to run across the fibers (Fig. 2F), similarto the pattern of Fas2 staining of AChE (Fig. 2C; same preparationas in F). Thus AChE appeared to be less well localized than AChRsin larval muscle even though the synaptic currents in larvae appearedto bemature.

The weaker AChE staining in larvae could be due to lower expression of synaptic AChE or less dense clustering compared withadult NMJs. To distinguish between these alternatives, we extractedAChE from whole larvae and from adult muscle and analyzed themolecular forms by velocity sedimentation. In all vertebrate species(Massoulié et al. 1993), including adult zebrafish (Bertrandet al. 1998), AChE is present as both globular forms and as predominantlysynaptically-localized, collagen-tailed forms associated withthe synaptic basal lamina. As shown in Fig. 3 (top) an extractof whole larvae showed two major peaks of activity. The heavierpeak (to the left) corresponds to the collagen-tailed form ofAChE, whereas the second set of peaks corresponds to the globularmonomeric, dimeric and tetrameric forms. A similar but betterresolved pattern was observed with adult muscle extracts (Fig.3, bottom). However, the use of entire larvae (including all tissues)and isolated adult muscle prevented a more quantitative comparison.Nonetheless, comparable proportions of globular and collagen-tailedAChE were present, indicating that synaptic AChE was less denselyclustered at larval NMJs.

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Fig. 3. Molecular forms of AChE in larvae and adult muscle. Equal volumes of extracts of entire larvae (top) and adult muscle (bottom) were centrifuged on 5-20% sucrose gradients. Fractions were collected from the bottom of the tube and assayed radiometrically for AChE activity. The activity is plotted for each fraction collected. The internal sedimentation coefficient markers are $beta$ -galactosidase (left, 16S) and alkaline phosphatase (right, 6.1S).

Ultrastructural maturation of NMJs

While changes in AChR kinetics (preceding text) and AChE activity (Nguyen et al. 1999) could each account for a twofold accelerationin mEPC decay time course during maturation of the NMJ, a largefraction of the order of magnitude changes in synaptic currentduring maturation remained unaccounted for. We used transmissionelectron microscopy to examine whether a structural feature ofthe synapse could contribute to its functional maturation. Maturelarval NMJs were readily identifiable, as reported previously(Waterman 1969; Westerfield et al. 1990) and as found for adultzebrafish (Mos et al. 1983). The NMJs were observed at the pointwhere several muscle fibers surrounded the nerve terminals, wherea limited region of the terminal showed a synaptic specialization(Fig. 4, bottom). On average the terminals (n = 22) were 1.2 ±0.5 µm in diameter (mean of large and small axes). These synapticregions contained small clear vesicles that clustered at the activezones, which on average (n = 31) were 1.8 ± 0.8 µm in length.We counted 156 vesicles within one vesicle diameter along a totalof 43 µm of presynaptic membrane at the active zones, for an averageof 3.7 vesicles/µm. The NMJs had a presynaptic thickening, a postsynapticdensity and a wide cleft (on average 0.12 ± 0.03 µm) with a denseextracellular matrix.

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Fig. 4. Ultrastructure of embryonic and larval NMJs. Transmission electron micrograph of a 30-h embryonic NMJ (top) and a 3-day larval NMJ (bottom). The scale bar at the bottom right-hand corner of the top micrograph is 1 µm for both micrographs. Notice the large, poorly differentiated nerve ending in the embryo and the smaller terminal in the larva with a well formed, dense basal lamina in the broad synaptic cleft.

In embryos (30 h), immature nerve endings were occasionally observed at similar points of contact between surrounding musclefibers (Fig. 4, top) but these lacked an obvious synaptic specialization.The endings were recognized by their larger size (1.8 ± 1.4 µmin diameter, n = 5) compared with the microtubule-containing axonsobserved in the spinal cord (0.30 ± 0.06 µm in diameter, n = 9;not shown). As expected from the low frequency of mEPCs at thisstage (Nguyen et al. 1999), embryonic nerve endings were observedless frequently compared with larval NMJs. Whereas several NMJswere commonly observed in a single cross-section of a given larva(total of 22 NMJs documented in 3 larvae), many cross-sectionshad to be examined before finding an immature profile in a givenembryo (total of 5 documented in 4 embryos). The nerve endingswere immature in appearance and could be larger than in larvae(Fig. 4, top) but contained only occasional and sometimes irregularlyshaped vesicles, with 13 vesicles observed within one vesiclediameter along 57 µm of presynaptic membrane for an average of0.2 vesicles/µm. Furthermore, the nerve endings were closely juxtaposedto the muscle cells, with a gap of 0.06 ± 0.01 µm (n = 5), andlacked a synaptic cleft or other specialization. These observationsindicate that the nerve-muscle gap in embryos is narrower andmore extensive than the wider, less restricted cleft at larvalNMJs and could act as a greater diffusion barrier resulting inslower clearance of ACh and prolongation of the time course ofembryonicmEPCs.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

We examined a number of physiological and morphological parameters at zebrafish NMJs as they developed from an immature embryonicform (on day 1) to become mature larval synapses a few days later.Previous work (Nguyen et al. 1999) indicated an order of magnitudeacceleration in time course of the mEPC (both for rise time anddecay) during NMJ maturation. We consider how the properties anddistributions of key determinants may contribute to shaping neuromusculartransmission in thispreparation.

Clustering of AChE is delayed compared with AChRs

The maturation of the zebrafish NMJ was in part due to the delayed appearance of ACh hydrolytic activity as blocking AChEwith eserine did not affect embryonic mEPCs but resulted in atwofold slowing of larval mEPCs (Nguyen et al. 1999). An apparentdelay of ~1 day occurs between clustering of AChR and AChE inXenopus (Peng et al. 1999) where blocking AChE activity causedonly a minor slowing of the time course of early junctional events(Kullberg et al. 1980). We observed comparable proportions ofthe collagen-tailed (synaptic) and globular (extrasynaptic) formsof AChE in larvae and adults but detected less intense AChE stainingco-localized with AChR staining in larval muscle compared withadult muscle. These results suggest that the increase in synapticAChE density at the zebrafish NMJ takes many days to occur, longerthan for AChR clustering and mEPC maturation. A high level ofunclustered AChE could account for the higher level of diffusestaining in larval muscle observed withFas2.

Release of a high ACh concentration from the onset

Explanations for slow embryonic mEPCs include slow clearance of ACh leading to channel re-openings, a lower concentrationof released ACh, slower AChRs or a lower density of postsynapticAChRs at embryonic NMJs. Due to the lack of significant hydrolysisexpected at embryonic NMJs, released ACh should remain at an elevatedconcentration. The gap between embryonic nerve endings and musclecells was half that observed over the junctional region of larvalterminals and could contribute to slowing ACh clearance and thustrapping released ACh. This would promote channel re-openingsand would contribute to both the slow rise time and decay of embryonicmEPCs.

Alternatively, a very low (micromolar) concentration of ACh could be released to slowly activate AChRs. However, the presenceof open channel block (K_0.5 = 0.5 mM) (Legendre et al. 2000) atembryonic NMJs indicates that a high concentration of ACh is releasedfrom immature nerve endings. Because the embryonic AChR channelshave kinetics an order of magnitude faster than the mEPC timecourse and the latter showed open channel block even after severalmilliseconds, we presume that the mEPC time course reflects thetime course of AChclearance.

Extrasynaptic vs. synaptic AChRs

During fast-flow application of a saturating concentration of ACh, single AChR channel currents had decay times twofold slowerin embryos than in larvae; but in contrast to the mEPCs, the AChRchannel rise times were comparable. These results indicate thatthe channels undergo a minor kinetic modification affecting deactivationand not activation. Recordings of end-plate potentials in adultzebrafish (Westerfield et al. 1986) revealed fast rise times (~1ms) consistent with the time integral of the AChR currents determinedin this study and indicating that fast synaptic AChR kineticspersist in the adult zebrafish. The presence of mature larvaljunctional currents is consistent with the high contraction ratesduring swimming both in larvae (Budick and O'Malley 2000; Bussand Drapeau 2001; Eaton and Farley 1973; Kimmel et al. 1974) andin adult zebrafish (Plaut 2000).

The slower deactivation of embryonic AChRs could contribute partially to the shortening of the mEPC decay duration but isnot expected to affect the rise time. The slower rise time ofthe embryonic mEPC is likely due to a low density of extrasynapticAChRs. It has been estimated that ACh could diffuse several µmto activate extrasynaptic AChRs with the similar slow time courseobserved at embryonic Xenopus NMJs (Kullberg et al. 1980). Thiswould also account for the smaller amplitude of the embryonicevents weobserved.

Although tight clusters of AChRs form within a few hours of nerve-muscle contact (Liu and Westerfield 1992), a further increasein the density of AChRs is possible and would be consistent withthe formation of the postsynaptic density and the greater mEPCamplitudes observed at the larval stage. The extrasynaptic AChRsare likely reduced in density, perhaps as a consequence of synapticclustering, to prevent re-openings by ACh diffusing from the cleftwhich would eventually (after many days) be hydrolyzed by synaptic(and perhaps also by diffusely distributed extrasynaptic) AChE.We conclude that no single feature of AChE or AChR propertiesor distribution limits maturation of the zebrafish NMJ. Ratherit is a combination of convergent changes that determines theamplitude and time course of fast neuromusculartransmission.

	ACKNOWLEDGMENTS

We thank Drs. P. Gibbs for supplying some of the zebrafish used in this study, S. Rossi for staining some of the muscle samples,and K. J. Muller and M. Attiwell for help with the electronmicroscopy.

This work was supported by awards from the Human Frontier Science Program (Short-Term Fellowship to P. Drapeau), Natural Sciencesand Engineering Research Council (NSERC) of Canada (Fellowshipto D. W. Ali), and the Medical Research Council (MRC) of Canada(Doctoral Research Award to R. R. Buss) and by grants from theNSERC and MRC of Canada (P. Drapeau), Institut National de laSanté et de la Recherche Médicale (INSERM) of France (P. Legendre),Fonds de la Recherche en Santé du Québec (FRSQ)-INSERM (P. Drapeauand P. Legendre), and the National Institutes of Health (R. L.Rotundo).

Present address of D. W. Ali: Dept. of Biological Sciences, University of Alberta, Edmonton, Alberta T6G 2E9,Canada.

	FOOTNOTES

Address for reprint requests: P. Drapeau, Dept. of Neurology, Montreal General Hospital, 1650 Cedar St., Montreal, QuebecH3G 1A4, Canada (E-mail: pierre.drapeau{at}mcgill.ca).

Received 29 June 2001; accepted in final form 2 October 2001.

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