Acetylcholinesterase mRNA Level and Synaptic Activity in Rat Muscles Depend on Nerve-Induced Pattern of Muscle Activation

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The Journal of Neuroscience, March 15, 1998, 18(6):1944-1952

Acetylcholinesterase mRNA Level and Synaptic Activity in Rat Muscles Depend on Nerve-Induced Pattern of Muscle Activation
Janez Sketelj¹, Neva $C$ rne-Finderle¹, Borut $S$ trukelj², Jo $z$ e V. Trontelj³, and Dirk Pette⁴
¹ Institute of Pathophysiology, School of Medicine, University of Ljubljana, 1000 Ljubljana, Slovenia, ² Jozef Stefan Institute, 1000 Ljubljana, Slovenia, ³ Institute of Clinical Neurophysiology, University Medical Center, 1000 Ljubljana, Slovenia, and ⁴ Fakultät für Biologie, Universität Konstanz, D-78457 Konstanz Germany

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Acetylcholinesterase (AChE) mRNA levels are severalfold higher in fast rat muscles compared with slow. We hypothesized thatAChE mRNA levels and AChE activity in the neuromuscular junctiondepend on a specific nerve-induced pattern of motor unit activation.Chronic low-frequency stimulation, mimicking the activation patternin slow muscles, was applied to fast muscles in rats. Molecularforms of AChE were analyzed by velocity sedimentation, and AChEmRNA levels were analyzed by Northern blots. AChE mRNA levelsin stimulated fast muscles dropped to 10-20% of control after1 week and became comparable to those in slow soleus muscles.The activity of the junctional A₁₂ AChE form in 35 d stimulatedfast muscles decreased to 56% of control value, reaching thatin the soleus muscle. Therefore, synaptic AChE itself dependson the muscle activation pattern. Complete inactivity after denervationalso decreased the AChE mRNA level in fast muscles to <10% in48 hr. In contrast, profuse fibrillations observed in noninnervatedimmature regenerating muscles maintain AChE mRNA levels at 80%of that in the innervated fast muscles. If protein synthesis wasinhibited by cycloheximide, AChE mRNA levels in 3-d-old regeneratingmuscle, still containing myoblasts, increased approximately twofold.No significant increase after cycloheximide application was observedeither in denervated mature fast muscles or in normal slow muscles.Low AChE mRNA levels observed in those muscles are probably notcaused by decreased stability of AChE mRNA as demonstrated inmyoblasts.

Key words: acetylcholinesterase; denervation; muscle; muscle stimulation; nerve-muscle interaction; nerve impulse pattern; neuromuscular junction; plasticity; regeneration; synapse

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
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Skeletal muscle fibers are able to change their phenotype in response to altered functional demands (Pette and Staron, 1997).Many functional elements in fast muscle fibers can be transformedby chronic low-frequency stimulation, e.g., contractile proteins,the Ca²⁺-handling system, and enzymes of energy metabolism (Pette andVrbovà, 1992). Therefore, fast muscles, stimulated by an impulsepattern similar to that in slow muscles, display several, althoughnot necessarily all, characteristics of a slow soleus muscle (Westgaardand Lømo, 1988; Termin et al., 1989; Schiaffino et al.,1990; Petteand Vrbovà, 1994). Acetylcholinesterase (AChE; EC 3.1.1.7)activity in muscle fibers can also be changed by electrostimulationor disuse of muscles, which adds this enzyme to the list of proteinsaffected by the pattern of muscle activation (Dettbarn et al.,1985; Lømo et al., 1985; Sketelj and $C$ re $s$ nar, 1995; Sketeljet al., 1997).

AChE, which is responsible for fast hydrolysis of acetylcholine in the neuromuscular junction (NMJ) (Marnay and Nachmansohn,1938; Eccles et al., 1942), is highly concentrated in the junctionalbasal lamina. It is present in a lower concentration throughoutthe length of muscle fibers (Sketelj, 1994). AChE displays a richmolecular polymorphism that encompasses globular and asymmetricmolecular forms (Massoulié and Bon, 1982). The asymmetric molecularforms of AChE, bound to the junctional basal lamina, contributemost to the junctional AChE activity in mammalian muscles (Hall,1973; Fernandez et al., 1984; Sketelj and Brzin, 1985; Inestrosaand Parelman, 1990; Rossi and Rotundo, 1996; Rotundo et al., 1997).

AChE regulation in predominantly fast rat muscles, such as extensor digitorum longus (EDL), is different from that in theslow soleus muscle (Bacou et al., 1982; Groswald and Dettbarn,1983; Lai et al., 1986; Sketelj et al., 1992a). Most conspicuously,total AChE activity per unit of muscle weight, as well as activityof the globular molecular forms, is higher in fast than in slowmuscles (Groswald and Dettbarn, 1983; Sketelj et al., 1992b),probably because of the much higher transcript level of the AChEcatalytic subunit in fast muscles ( $C$ re $s$ nar et al., 1994; Michelet al., 1994).

Some differences in AChE regulation may be attributable to intrinsic properties of the two types of muscles (Sketelj et al.,1991; Dolenc et al., 1994). However, because the patterns of neuralactivation of motor units in fast and slow rat muscles are verydifferent (Navarrete and Vrbovà, 1983; Hennig and Lømo, 1985),we hypothesized that mRNA levels of AChE catalytic subunit andAChE synaptic activity in muscles depend on specific neural activationpatterns. Indeed, the AChE mRNA level in fast muscles was foundto decrease after 1 week of chronic low-frequency stimulationand became comparable to that in the slow soleus muscle. The activityof the asymmetric AChE forms in the motor endplates of chronicallystimulated fast muscles decreased too, revealing a dependenceof functional AChE activity in the synapse itself on the muscleactivation pattern. Low levels of AChE transcripts found in tonicallyactivated or completely inactive muscles are probably not causedby the increased AChE mRNA degradation rate that is characteristicof early stages of muscle development.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Animals. In accordance with national guidelines, the experiments on animals in Slovenia were approved by the Veterinary Administrationof the Ministry for Agriculture, Forestry and Food, permit 326-07-258/95,and in Germany by the Regierungspräsidium Freiburg, authorizationAz. 37/9185.815/733.

Experiments were performed on adult male Wistar rats. For surgical procedures, rats were anesthetized by a mixture of Ketalar(Parke-Davis, Vienna, Austria; 60 mg/kg), Rompun (Bayer, Leverkusen,Germany; 8 mg/kg), and atropine (Belupo, Koprivnica, Croatia;0.6 mg/kg), or by sodium pentobarbital (Werfft-Chemie, Wels, Austria;55 mg/kg), injected intraperitoneally. The animals were exsanguinatedunder ether anesthesia.

Low-frequency stimulation of EDL and tibialis anterior (TA) muscles. Stainless steel electrodes were implanted under anesthesiaon each side of the peroneal nerve of the left hindlimb (Simoneauand Pette, 1988). Stimulation was performed using a battery-operated,portable stimulator (Tyler and Wright, 1980). Square wave stimuli(10 Hz, single pulse duration 30 msec) were applied continuouslyfor 10 hr per day for either 7, 25, or 35 d. The amplitude ofstimulation was adjusted daily so that maximum contraction ofthe stimulated muscle group could be palpated and stimulationdid not cause apparent discomfort to the animals.

Muscle denervation. The sciatic nerve in one leg was exposed and transected in a midthigh region. A piece of the nerve wasexcised to prevent reinnervation.

Noninnervated regenerating muscle. One leg was denervated as described above, and the EDL muscle was exposed in that leg.The muscle was thereafter injected with the myotoxic local anestheticMarcaine (0.5% bupivacaine; Astra, Södertälje, Sweden) as described(Hall-Craggs, 1974). The wound was closed, the animals were leftto recover, and the muscles were allowed to regenerate for 3 or8 d.

Cycloheximide treatment. Rats were injected intraperitoneally with 20 mg/kg of cycloheximide in PBS. Four hours later, theywere given another 10 mg/kg of cycloheximide. Controls were injectedwith saline. The animals were killed 8 hr after the first injection,and muscles to be used for further analysis were immediately isolatedand frozen.

Velocity sedimentation analysis of AChE. The EDL and soleus muscles of both hindlimbs were isolated (muscles from the nontreatedleg served as controls). Regions containing NMJs (junctional regions)were separated from regions without them (extrajunctional regions)(Koenig and Rieger, 1981; Sketelj et al., 1993). The samples wereweighed, frozen in liquid nitrogen, and kept at $-$ 80°C until theywere analyzed. Frozen muscle samples were crushed and pulverizedin a mortar chilled in liquid nitrogen and then immediately homogenized.An ice-cold high-salt-detergent medium with a set of proteaseinhibitors was used to extract AChE, which was then subjectedto velocity sedimentation analysis in 5-20% linear sucrose gradientsas described (Sketelj et al., 1993). The activity pertaining toan individual molecular form of AChE was calculated by measuringthe area under its peak of activity in the velocity sedimentationpattern, using our own computer program (Ribari $c$ et al., 1996).

Northern blot analysis. EDL, TA, diaphragm, or soleus muscles were isolated rapidly under antiseptic conditions and frozenimmediately in liquid nitrogen. Frozen muscles were pulverizedin a mortar chilled by liquid nitrogen and briefly homogenizedin denaturing solution by an Ultra-Turrax homogenizer. Total RNAwas isolated by a slightly modified single-step procedure (Chomczynskiand Sacchi, 1987), subjected to electrophoresis in 1.2% denaturingformaldehyde-agarose gel (30-50 µg of RNA per lane), and transferredto nylon membranes by capillary blotting (Hybond N, Amersham,Arlington Heights, IL). Specific DNA probe corresponding to afragment of the cDNA of the rat AChE catalytic subunit (commoncatalytic domain, nucleotides 920-1683; a gift by Dr. C. Legayand Dr. J. Massoulié, Paris, France) was used for hybridization.Random prime kit components (Boehringer Mannheim, Mannheim, Germany)were used for labeling the probe with $alpha$ ³²P dCTP (DuPont de Nemours, Brussels, Belgium). A specific syntheticoligonucleotide complementary to the 3' end of the probe (RansomHill Bioscience, Ramona, CA) was used as the primer instead ofrandom oligonucleotides. The membranes were prehybridized for1 hr at 42°C in a buffer solution containing 5× SSPE, 50% formamide,5× Denhardt's solution, 0.5% SDS, and 20 µg/ml salmon sperm DNA(Sigma, St. Louis, MO). Hybridization was performed at 42°C overnightin the same solution with the addition of the radioactive probeto ~10⁶ cpm/ml. The blots were washed in 2× SSPE at room temperature,then twice for 15 min in 2× SSPE and 0.1% SDS at 42°C, then for30 min in 1× SSPE and 0.1% SDS at 42°C, and finally two timesfor 15 min in 0.1× SSPE and 0.1% SDS at room temperature. Themembranes were exposed to x-ray films using intensifying screenfor 1-4 d. The AChE probe was then stripped off the membranes,and they were rehybridized by radioactive $beta$ -actin probe as describedabove. The autoradiograms were quantified densitometrically usingMCID M4 image analyzer by Imaging Research, and the values forAChE mRNA were normalized in regard to the intensity of the corresponding $beta$ -actin signal.

EMG recording. The rats were anesthetized as described and kept on a warm blanket to prevent hypothermia. Skin and musclefascia on the frontal side of the calf were incised, and the EDLmuscle (control, denervated, or regenerating) was carefully exposed.A disposable concentric needle electrode (No. 53155, recordingarea 0.07 mm²) was inserted into the muscle at several sites consecutively.Spontaneous electromyographic activity followed and was recordedseveral times during the next 10-30 min by a Mystro electromyograph(Medelec, Old Woking, UK). The frequency bandwidth used was 0.2-2.0kHz.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Levels of AChE mRNA and molecular forms of AChE in different rat muscles

Gene transcript levels of AChE catalytic subunit were determined in several rat muscles differing in regard to their speedof contraction, fiber type composition, and expression of myosinheavy chain (MHC) isoforms. AChE mRNA levels were found to behigher in fast muscles such as EDL and TA than in slower onessuch as the diaphragm and soleus (Fig. 1B). We used densitometricevaluation and assigned a value of 100 to the mRNA level in theEDL muscle, and the average mRNA levels in the TA were ~70, inthe diaphragm ~50, and in the soleus ~15 (Fig. 1C). The relativelevels of AChE mRNA in the examined muscles were roughly proportionalto activities of the monomeric 4 S molecular form of AChE in theextrajunctional regions of these muscles (Fig. 1A,C).

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Figure 1. AChE expression in four different rat muscles: soleus (SOL, lane 1), extensor digitorum longus (EDL, lane 2), tibialis anterior(TA, lane 3), and the diaphragm (DIA, lane 4). A, Velocity sedimentationpatterns of AChE molecular forms, identified by their sedimentationcoefficients, in the extrajunctional muscle regions; AChE activityis expressed in arbitrary units per unit of wet weight. B, Northernblot analysis of AChE mRNA levels in muscles. $beta$ -actin mRNA wasused to control uniformity of sample loading. C, Relative levelsof the 4 S AChE form activity (blank bars) and AChE mRNA (hatchedbars) in rat muscles (mean + SE; the number of determinationsis given in parentheses).

The asymmetric A₁₂ molecular forms of AChE are highly concentrated in NMJs of rat muscles and contribute most of the junctionalAChE activity (Hall, 1973). We analyzed the patterns of molecularforms of AChE separately in the muscle region containing all ofthe NMJs (junctional region) and in muscle regions without NMJs(extrajunctional regions). By deducting the specific activityof the A₁₂ AChE form in the extrajunctional region from that inthe junctional region, the activity of the synaptic A₁₂ form properin the junctional region was calculated, both in the fast EDLmuscle and in the slow soleus muscle. The number of muscle fibers(and therefore, of motor endplates) in the two muscles was determinedin stained histological cross-sections (EDL, 3120 ± 20 fibers;soleus, 1790 ± 60 fibers; mean ± SE; n = 3), and A₁₂ AChE activityper NMJ in the two muscles was calculated. The activity of theA₁₂ AChE per endplate in the soleus muscles was ~60% of that inthe EDL (4.5 ± 0.5 fmol ACh/min vs 7.3 ± 0.3 fmol ACh/min; mean± SD; n = 4); the difference was statistically significant (p< 0.01).

The effect of chronic low-frequency stimulation on AChE mRNA levels and its synaptic activity in fast muscles

In rats, fast muscles are normally activated by rare, short-lasting high-frequency bursts of nerve impulses (Navarrete andVrbovà, 1983; Hennig and Lømo, 1985). Chronic low-frequency electricalstimulation of fast EDL and TA muscles via their nerves subjectedthe two muscles to an activation pattern similar to that in theslow soleus muscle. We found that after only 1 week AChE mRNAlevels in both stimulated fast muscles fell to low values comparableto those in the soleus muscle (~10-20% of the AChE mRNA levelsin control fast muscles). Low levels of AChE mRNA in chronicallystimulated EDL muscle also persisted after 25 d of stimulation(Fig. 2).

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Figure 2. The effect of chronic low-frequency stimulation on AChE mRNA levels in fast muscles tibialis anterior (TA) and extensor digitorumlongus (EDL). A, Northern blot analysis of control (c) and stimulated(s) muscles, stimulation lasting 7 d (7d) or 25 d (25d). Normalsoleus muscle (SOL) is included for comparison; $beta$ -actin mRNA wasused to control uniformity of sample loading. B, Histogram ofrelative levels of AChE mRNA in control (contr) and stimulated(stim) EDL muscles in comparison to soleus (SOL) muscle (mean+ SE of several determinations; the number of determinations isgiven in parentheses).

In addition, the patterns of AChE molecular forms in the junctional regions of 35 d stimulated and control EDL muscles wereanalyzed (Fig. 3A). Specific activity of the monomeric G₁ formwas heavily reduced in the stimulated muscles. Activity of thejunctional A₁₂ AChE form calculated per NMJ in the stimulatedEDL was only ~56% of that in the control EDL muscle (p < 0.05)and was about the same as that in the NMJs of normal soleus muscles(Fig. 3B).

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Figure 3. The effect of chronic low-frequency stimulation on the junctional 16 S (A₁₂) AChE form in fast extensor digitorum longus (EDL)muscles. A, Velocity sedimentation pattern of AChE molecular formsin the junctional region of control and 35 d stimulated EDL muscles;the peak corresponding to the 16 S form is hatched. AChE activityis expressed in arbitrary units per neuromuscular junction. B,Activities of the 16 S AChE form per neuromuscular junction insoleus (SOL) muscles, control EDL muscles (EDL), and 35 d stimulatedEDL muscles (EDL stim) (mean + SE; the number of determinationsis given in parentheses).

The effect of muscle inactivity caused by denervation on the levels of AChE mRNA in fast muscles

We focused our attention on an early period after denervation that was characterized by complete muscle inactivity. Northernblot analysis of denervated EDL muscles revealed that mRNA levelsof AChE started to decrease during the first 24 hr after denervation(Fig. 4A,B). At that time, AChE mRNA levels were already reducedto ~30% of control levels. AChE mRNA levels in the denervatedEDL muscles were further reduced to just a small percentage ofcontrol levels after 48 hr of inactivity.

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Figure 4. The effect of denervation on AChE mRNA levels in mature and regenerating EDL muscles. A, Northern blot analysis of AChE mRNAlevels in control EDL (con), EDL denervated (den) for 24 hr (1d),48 hr (2d), or 8 d (8d), and in noninnervated 8-d-old regeneratingEDL muscle (reg 8d). $beta$ -Actin mRNA was used to control uniformityof sample loading. B, Histogram of relative AChE mRNA levels incontrol (contr) and different kinds of denervated EDL muscles(mean + SE; the number of determinations is given in parentheses).

AChE mRNA levels also were examined in noninnervated muscles that regenerated after injury. We let muscle regeneration takeplace in the absence of innervation to be able to compare denervatedimmature regenerating muscles with denervated mature muscles.In contrast to mature 8 d denervated muscles, AChE mRNA levelsin noninnervated 8-d-old regenerating fast muscles were fairlyhigh, i.e., ~80% of those in control mature innervated muscles(Fig. 4).

Electromyographic recording of spontaneous muscle activity in denervated mature and regenerating muscles was performed toexamine the hypothesis that possible differences in spontaneousactivity might be responsible for different AChE mRNA levels inmature versus immature denervated muscles (Fig. 5). In denervatedmature muscles, we were able to record spontaneous fibrillationsat 10 of 18 recording sites in three 8 d denervated EDL muscles,using standard concentric needle electrodes. Action potentialsoriginating from one or a few muscle fibers were observed at recordingsites with activity. Individual muscle fibers fibrillated withfrequencies ranging from ~0.5 to 5 Hz. In the noninnervated regeneratingmuscles, however, profuse spontaneous fibrillatory activity couldalways be recorded at each impalement by the same EMG electrode.The number of active fibers within the reach of the electrodewas too great to allow more detailed analysis of the firing rateof individual muscle fibers.

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Figure 5. Representative examples of electromyographic recordings of spontaneous electrical activity in denervated EDL muscles. A, Threemuscle fibers firing in the neighborhood of the electrode in an8 d denervated mature EDL muscle. B, Profuse fibrillatory activityin an 8-d-old noninnervated regenerating EDL muscle. C, Electricalsilence in a normal EDL muscle, showing the level of noise.

The effect of cycloheximide treatment on AChE mRNA levels in very immature regenerating muscle and various mature muscles

Inhibition of protein synthesis in myoblasts in vitro by cycloheximide for 6 hr caused a great increase of AChE mRNA levelsin these cells, probably because of inhibited synthesis of short-livedproteins responsible for the fast degradation rate of AChE mRNAin myoblasts (Fuentes and Taylor, 1993). We found that the levelof AChE mRNA in 3-d-old regenerating EDL muscles was <50% of thatin more mature 8-d-old regenerating muscles (Fig. 6). In accordancewith the results obtained in vitro, we found an 1.8-fold increaseof AChE mRNA levels in early regenerating EDL muscles 8 hr afterwe treated the rats with a high dose of cycloheximide. It is possiblethat low AChE mRNA levels observed in either inactive musclesor tonically activated muscles are caused by an accelerated AChEmRNA degradation rate, as in immature muscle cells. However, inthe rats treated with a high dose of cycloheximide, no major increaseof AChE mRNA levels could be detected after 8 hr of cycloheximidetreatment either in denervated fast muscles or in normal innervatedslow soleus muscles (Fig. 6).

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Figure 6. The effect of cycloheximide on AChE mRNA levels in different muscles 8 hr after the rats received the drug. A, Northern blotanalysis of AChE mRNA levels in 3-d-old regenerating EDL muscles(reg 3d) in control (c) and cycloheximide-treated (chx) rats,with an 8-d-old control regenerating muscle (reg 8d) shown forcomparison. B, Northern blot analysis of AChE mRNA levels in normalEDL, 3 d denervated mature EDL (EDL den) and normal soleus (SOL)muscles from control (c) or cycloheximide-treated (chx) rats. $beta$ -actin mRNA was used for control of uniformity of sample loading.C, Relative levels of AChE mRNA in control EDL (EDL c), 3-d-oldnoninnervated regenerating EDL (EDL reg 3d), 3 d denervated matureEDL (EDL den 3d), and normal soleus (SOL) muscles in control (blankbars) or cycloheximide-treated animals (hatched bars) (mean +SE; the number of determinations is given in parentheses).

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

AChE mRNA levels in rat muscles depend on the muscle activation pattern

AChE expression was examined in four rat muscles displaying different patterns of MHC isoforms: EDL: 60-65% MHCIIb, 25-35%MHCIId/x, 10-12% MHCIIa, 1% MHCI; TA: 60-77% MHCIIb, 19-25% MHCIId/x,4-14% MHCIIa, 0-4% MHCI; diaphragm: 1% MHCIIb, 53% MHCIId/x, 32%MHCIIa, 14% MHCI; and soleus: 0% MHCIIb, 0% MHCIId/x, 10-20% MHCIIa,80-90% MHCI (Bär and Pette, 1988; Kirschbaum et al., 1990; Petteand Staron, 1990; Snoj-Cvetko et al., 1996; Sketelj et al., 1997).We found that high cumulative percentages of the fastest MHC isoformsMHCIIb and IId/x and low percentages of the isoform MHCIIa andslow isoform MHCI were associated with high levels of AChE transcriptsin a muscle, and vice versa. Activity of the monomeric 4 S AChEform (G₁), reflecting the concentration of the basic catalyticsubunit of AChE, roughly parallelled the levels of AChE mRNA inthe examined muscles. Because the most important factor determiningthe MHC profile of a muscle, although not the only one, is a specificpattern of neural activation of muscle fibers (Pette and Staron,1997), the above results indirectly support the hypothesis thatthe AChE mRNA level in muscles also depends on the neural activationpattern. However, although the MHC profiles of EDL and TA musclesare fairly similar, the AChE transcript level and activity ofthe G₁ AChE form were consistently higher, whereas the activityof the G₄ form was lower in the EDL compared with the TA. Thelatter observation indicates that this may be attributable toa greater work load imposed on the TA than on the EDL muscle (Fernandezand Hodges-Savola, 1992; Gisiger et al., 1994; Boudreaularviereet al., 1997). Some mechanisms seem to modify AChE expressionto a certain extent independently of MHC regulation.

Fast motor units in rat muscles such as EDL are activated phasically, with short high-frequency bursts interspersed with longperiods of inactivity (Fischbach and Robbins, 1969; Navaretteand Vrbovà, 1983; Hennig and Lømo, 1985). We demonstrated thatby imposing a chronic low-frequency stimulation, which roughlymimics the tonic activation pattern in slow muscle fibers, onfast muscles such as EDL or TA, high levels of AChE mRNA in thesemuscles became reduced to a low level characteristic of the soleusmuscle after 1 week, and they persisted for at least a few weeksthereafter. Conversely, AChE activity and the transcript levelsin the soleus muscle were reported to increase after its disuse(Dettbarn et al., 1985; Sketelj and $C$ re $s$ nar, 1995), which changedits pattern of activation from tonic to phasic and greatly reducedthe aggregate number of nerve impulses per day (Fischbach andRobbins, 1969). Therefore, the AChE mRNA level in a rat muscledepends on specific neural activation patterns: rare phasic burstsof high-frequency activity enhance and continuous tonic low-frequencymuscle activation reduces AChE mRNA levels.

Activity of the junctional asymmetric AChE forms is affected by the pattern of muscle activation

We found earlier that activity of the globular molecular forms of AChE in the extrajunctional muscle regions decreased aftercontinuous muscle stimulation (Sketelj et al., 1997). In addition,we show here that activity of the functionally most importantpart of muscle AChE, i.e., activity of the multimeric asymmetricAChE forms in the neuromuscular junction itself, parallels theavailable amount of catalytic subunits and the level of AChE mRNA:activity of the synaptic A₁₂ AChE form in control EDL was nearlytwo times higher than in the stimulated EDL or in the normal soleusmuscles. Accordingly, transgenically overexpressed AChE in embryonicmuscles caused an increase in the size of their NMJs (Shapiraet al., 1994). However, the amount of A₁₂ AChE forms assembledfrom the catalytic subunits and the noncatalytic tail subunitis also determined by the expression of the collagen-like tailsubunit (collagen Q) (Krejci et al., 1991; Duval et al., 1992;Bon and Massoulié, 1997; Krejci et al., 1997). At present, therefore,it is not possible to decide whether changes in expression ofeither catalytic or tail subunits, or both, are responsible forthe observed changes in junctional A₁₂ AChE activity in chronicallyactive muscles. Our data agree well with earlier indirect estimationsof junctional AChE activity in slow and fast rat muscles usingelectrophysiological experiments (Magazanik et al., 1984). Higherjunctional AChE activity in fast muscles, as compared with slowones, may be an advantage when very rapid acetylcholine hydrolysisis required for transmission of nerve impulses at very high frequenciesin fast muscles.

The idea that NMJ development is regulated by "trophic" factors released by the nerve ending has gained new support recently(Bowe and Fallon, 1995). Thus, expression of acetylcholine receptorin the subjunctional nuclei might be enhanced by calcitonin gene-relatedpeptide (CGRP) (Fontaine et al., 1986; New and Mudge, 1986) andacetylcholine receptor-inducing activity (ARIA)-neuregulin (Harriset al., 1988; Falls et al., 1993; Chu et al., 1995). AChE transcriptsare approximately 10 times more concentrated under the motor endplatethan elsewhere in muscle fibers in different vertebrate species(Jasmin et al., 1993; Michel et al., 1994; Legay et al., 1995).Different sensitivity of AChE transcript levels to either denervationor tetrodotoxin paralysis of rat muscles suggested that trophicfactors also regulated AChE expression in subjunctional nuclei(Michel et al., 1994). Indeed, CGRP had an innervation-like effecton the junctional G₄ AChE form in rat muscles (Hodges-Savola andFernandez, 1995). It increased AChE mRNA levels in cultured chickmuscles approximately threefold (Choi et al., 1996), but ARIA-neuregulinhad no effect (Pun and Tsim, 1995). In addition to this, our resultssuggest that junctional muscle nuclei, like the extrajunctionalones, still possess the ability to respond to different neuralstimulation patterns as far as the regulation of junctional AChEis concerned.

Either muscle inactivity or continuous muscle activation decreases AChE expression in muscles

It has been shown before that the levels of AChE mRNA become very low in 5 to 10 d denervated rat muscles ( $C$ re $s$ nar et al.,1994; Michel et al., 1994). In light of the present results, itwas not clear whether this was attributable to muscle inactivityor chronic spontaneous low-frequency activity, called fibrillations,which appear in denervated rat muscles ~2-3 d after denervation(Hník and $S$ korpil, 1962; Salafski et al., 1968). We thereforeexamined the AChE mRNA level in the denervated EDL muscle beforeit starts fibrillating. The immediate decrease of AChE mRNA indicatesthat muscle inactivity itself is primarily responsible. Fibrillatoryactivity that appears later is insufficient to maintain the AChEmRNA levels, just as it is unable to prevent the extrajunctionalappearance of acetylcholine receptors in denervated muscle fibers(Fambrough, 1970; Purves and Sakmann, 1974). Namely, periods offibrillatory activity in individual denervated rat muscle fiberslast on average <1 day and are interspersed with 2- to 3-d-longperiods of electromechanical inactivity (Purves and Sakmann, 1974).

However, immature noninnervated rat muscle fibers express fairly high AChE activity either in culture or during regenerationin vivo (Sugiyama, 1977; Sketelj et al., 1987). We showed herethat high AChE activity in noninnervated regenerating EDL muscleswas caused by fairly high levels of AChE mRNA (~80% of controlfast muscles). Because profuse spontaneous fibrillatory activitywas recorded by EMG at each impalement of regenerating EDL muscles,it seems that spontaneous fibrillatory activity in noninnervatedimmature muscle fibers is sufficiently intense to sustain highAChE mRNA levels yet not too persistent to suppress it. Accordingly,a dramatic increase of AChE activity occurs in cultured rat myotubesafter the onset of fibrillations but can be prevented if fibrillationsare blocked by tetrodotoxin (Brockman et al., 1984; De La Porteet al., 1984; Rubin et al., 1985).

Regarding the mechanisms of AChE mRNA level dependence on muscle activation pattern, it is surprising that both inactivityand continuous muscle activation should have similar suppressiveeffects on AChE transcript levels. Either a decreased transcriptionrate or an enhanced mRNA degradation rate might be responsiblefor these effects. It has been shown that increased AChE expressionafter fusion of myoblasts into myotubes is attributable to a decreaseof the AChE mRNA degradation rate, whereas its transcription ratedoes not change appreciably (Fuentes and Taylor, 1993). When culturedmyoblasts were treated by the protein synthesis inhibitor cycloheximide,a prompt increase of AChE mRNA levels was noted. This "superinduction"was thought to be attributable to the suppressed synthesis ofproteins responsible for destabilization of AChE mRNA (Fuentesand Taylor, 1993). We treated the rats with a dose of cycloheximide10-fold higher than that which produced 80% inhibition of proteinsynthesis (Dupret et al., 1986). Accordingly, 8 hr later AChEmRNA levels in the early regenerating muscles, still containingmyoblasts (Carlson, 1976; Hansen-Smith and Carlson, 1979), becameapproximately twofold higher than in the untreated controls. However,after we applied the same dose of cycloheximide, we could findno substantial increase of AChE mRNA levels either in normal slowsoleus muscles or in denervated fast EDL muscles. This arguesagainst the possibility that either denervated fast muscles ortonically activated muscles display low levels of AChE mRNA becauseof relapsing to a very immature state in which an increased AChEmRNA degradation rate would reduce its steady-state levels. Accordingly,immature myotubes in vitro, although noninnervated, have alreadyachieved AChE mRNA stabilization (Fuentes and Taylor, 1993). Theseresults favor the view that AChE mRNA stabilization is a veryearly, and possibly irreversible, event during muscle cell differentiation.We propose that at later stages, regulation of AChE mRNA levelsby muscle activation pattern is based on regulation of the AChEmRNA transcription rate. Our results support this assumption,although they do not prove it.

  FOOTNOTES

Received Oct. 9, 1997; revised Dec. 15, 1997; accepted Dec. 29, 1997.

This study was supported by a grant from the Ministry of Science and Technology of the Republic of Slovenia (J.S.) and DeutscheForschungsgemeinschaft, Sonderforschungsbereich 156, TP/B3 (D.P.).The skillful technical assistance of Mr. Boris Pe $c$ enko and Mrs.Elmi Leisner is gratefully acknowledged. We thank Dr. M. Mihelinfor help with EMG recording.
Correspondence should be addressed to Dr. Janez Sketelj, Institute of Pathophysiology, Zalo $s$ ka 4, 1000 Ljubljana, Slovenia.

  REFERENCES

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Bacou F, Vigneron P, Massoulié J (1982) Acetylcholinesteraseforms in fast and slow rabbit muscle. Nature 296:661-664[Medline].
Bär A, Pette D (1988) Threefast myosin heavy chains in adult rat skeletal muscle. FEBSLett 235:153-155[ISI][Medline].
Bon S, Massoulié J (1997) Quaternaryassociations of acetylcholinesterase. JBiol Chem 272:3007-3015[Abstract/Free Full Text].
Boudreaularviere C, Gisiger V, Michel RN, Hubatsch DA, Jasmin BJ (1997) Fastand slow skeletal muscles express a common basic profile of acetylcholinesterasemolecular forms. Am J Physiol 41:C68-C76.
Bowe MA, Fallon JR (1995) Therole of agrin in synapse formation. AnnuRev Neurosci 18:443-462[ISI][Medline].
Brockman SM, Younkin LH, Younkin SG (1984) Theeffect of spontaneous electromechanical activity on the metabolismof acetylcholinesterase in cultured embryonic rat myotubes. JNeurosci 4:131-140[Abstract].
Carlson BM (1976) A quantitative study of muscle fibersurvival and regeneration in normal, predenervated, and Marcaine-treatedfree muscle grafts in the rat. ExpNeurol 52:421-432[ISI][Medline].
Choi RCY, Leung PWY, Dong TTX, Wan DCC, Tsim KWK (1996) Calcitoningene-related peptide increases the expression of acetylcholinesterasein cultured chick myotubes. NeurosciLett 217:165-168[ISI][Medline].
Chomczynski P, Sacchi N (1987) Single-stepmethod of RNA isolation by acid guanidinium thiocyanate-phenol-chloroformextraction. Anal Biochem 162:156-159[ISI][Medline].
Chu GC, Moscoso LM, Sliwkowski MX, Merlie JP (1995) Regulationof the acetylcholine receptor $epsilon$ subunit gene by recombinant ARIA:an in vitro model for transynaptic gene regulation. Neuron 14:329-339[ISI][Medline].
$C$ re $s$ nar B, $C$ rne-Finderle N, Breskvar K, Sketelj J (1994) Neuralregulation of muscle acetylcholinesterase is exerted on the levelof its mRNA. J Neurosci Res 38:294-299[ISI][Medline].
De La Porte S, Vigny M, Massoulié J, Koenig J (1984) Actionof veratridine on acetylcholinesterase in cultures of rat musclecells. Dev Biol 106:450-456[ISI][Medline].
Dettbarn W-D, Groswald D, Gupta RC, Misulis KE (1985) Useand disuse and the control of acetylcholinesterase activity infast and slow twitch muscle of rat. In: Molecularbasis of nerve activity (Changeux J-P, Hucho F, Maelicke A, Neumann E, eds), pp 567-588. Berlin: Walterde Gruyter.
Dolenc I, $C$ rne-Finderle N, Er $z$ en I, Sketelj J (1994) Satellitecells in slow and fast rat muscles differ in respect to acetylcholinesteraseregulation mechanisms they convey to their myofibers during regeneration. JNeurosci Res 37:236-246[ISI][Medline].
Dupret JM, Brun P, Thomasset M (1986) Invivo effects of transcriptional and translational inhibitors onduodenal vitamin D-dependent calcium-binding protein messengerribonucleic acid stimulation by 1,25-dihydroxycholecalciferol. Endocrinology 119:2476-2483[Abstract].
Duval N, Krejci E, Grassi J, Coussen F, Massoulié J, Bon S (1992) Moleculararchitecture of acetylcholinesterase collagen-tailed forms; constructionof a glycolipid-tailed tetramer. EMBOJ 11:3255-3261[ISI][Medline].
Eccles JC, Katz B, Kuffler SW (1942) Effectof eserine on neuromuscular transmission. JNeurophysiol 5:211-230[Free Full Text].
Falls DL, Rosen KM, Corfas G, Lane WS, Fischbach GD (1993) ARIA,a protein that stimulates acetylcholine receptor synthesis, isa member of the Neu ligand family. Cell 72:801-815[ISI][Medline].
Fambrough DM (1970) Acetylcholine sensitivity of musclefiber membranes: mechanism of regulation by motoneurons. Science 163:372-373.
Fernandez HL, Hodges-Savola CA (1992) Trophicregulation of acetylcholinesterase isoenzymes in adult mammalianskeletal muscles. NeurochemRes 17:115-124[ISI][Medline].
Fernandez HL, Inestrosa NC, Stiles JR (1984) Subcellularlocalization of acetylcholinesterase molecular forms in endplateregions of adult mammalian skeletal muscle. NeurochemRes 9:1211-1230[ISI][Medline].
Fischbach GD, Robbins N (1969) Changesin contractile properties of disused soleus muscles. JPhysiol (Lond) 201:305-320[Abstract/Free Full Text].
Fontaine B, Klarsfeld A, Hokfelt T, Changeux J-P (1986) Calcitoningene-related peptide, a peptide present in spinal cord motoneurons,increases the number of acetylcholine receptors in primary culturesof chick embryo myotubes. NeurosciLett 711:59-65.
Fuentes MA, Taylor P (1993) Controlof acetylcholinesterase gene expression during myogenesis. Neuron 10:679-687[ISI][Medline].
Gisiger V, Belisle M, Gardiner PF (1994) Acetylcholinesteraseadaptation to voluntary wheel running is proportional to the volumeof activity in fast, but not slow, rat hindlimb muscles. EurJ Neurosci 6:673-680[ISI][Medline].
Groswald DE, Dettbarn W-D (1983) Characterizationof acetylcholinesterase molecular forms in slow and fast muscleof rat. Neurochem Res 8:983-995[ISI][Medline].
Hall ZW (1973) Multiple forms of acetylcholinesteraseand their distribution in endplate and non-endplate regions ofrat diaphragm muscle. J Neurobiol 4:343-361[ISI][Medline].
Hall-Craggs ECB (1974) Rapid degeneration and regenerationof a whole skeletal muscle following treatment with bupivacaine(Marcaine). Exp Neurol 43:349-354[ISI][Medline].
Hansen-Smith FM, Carlson BM (1979) Cellularresponses to free grafting of the extensor digitorum longus muscleof the rat. J Neurol Sci 41:149-173[ISI][Medline].
Harris DA, Falls DL, Dill-Devor RM, Fischbach GD (1988) Acetylcholinereceptor-inducing factor from chicken brain increases the levelof mRNA encoding the receptor $alpha$ subunit. ProcNatl Acad Sci USA 85:1983-1987[Abstract/Free Full Text].
Hennig R, Lømo T (1985) Firingpattern of motor units in normal rats. Nature 314:164-166[Medline].
Hník P, $S$ korpil V (1962) Fibrillationactivity in denervated muscle. In: Thedenervated muscle (Gutmann E, ed), pp 135-150. Prague: CzechoslovakAcademy of Sciences.
Hodges-Savola CA, Fernandez HL (1995) Arole for calcitonin gene-related peptide in the regulation ofrat skeletal muscle G₄ acetylcholinesterase. NeurosciLett 190:117-120[ISI][Medline].
Inestrosa NC, Parelman A (1990) Associationof acetylcholinesterase with the cell surface. JMembr Biol 118:1-9[ISI][Medline].
Jasmin BJ, Lee RK, Rotundo RL (1993) Compartmentalizationof acetylcholinesterase mRNA and enzyme at the vertebrate neuromuscularjunction. Neuron 11:467-477[ISI][Medline].
Kirschbaum BJ, Kucher H-B, Termin A, Kelly AM, Pette D (1990) Antagonisticeffects of chronic low frequency stimulation and thyroid hormoneon myosin expression in rat fast-twitch muscle. JBiol Chem 265:13974-13980[Abstract/Free Full Text].
Koenig J, Rieger F (1981) Biochemicalstability of the AChE molecular forms after cytochemical staining:postnatal focalization of the 16 S AChE in rat muscle. DevNeurosci 4:249-257[ISI][Medline].
Krejci E, Coussen F, Duval N, Chatel J-M, Legay C, Puype M, Vandekerckhove J, Cartaud J, Bon S, Massoulié J (1991) Primarystructure of a collagenic tail peptide of Torpedo acetylcholinesterase:co-expression with catalytic subunit induces the production ofcollagen-tailed forms in transfected cells. EMBOJ 10:1285-1293[ISI][Medline].
Krejci E, Thomine S, Boschetti N, Legay C, Sketelj J, Massoulie J (1997) Themammalian gene of acetylcholinesterase-associated collagen. JBiol Chem 272:22840-22847[Abstract/Free Full Text].
Lai J, Jedrzejczyk J, Pizzey JA, Green D, Barnard EA (1986) Neuralcontrol of the forms of acetylcholinesterase in slow mammalianmuscles. Nature 321:72-74[Medline].
Legay C, Huchet M, Massoulié J, Changeux J-P (1995) Developmentalregulation of acetylcholinesterase transcripts in the mouse diaphragm:alternative splicing and focalization. EurJ Neurosci 7:1803-1809[ISI][Medline].
Lømo T, Massoulié J, Vigny M (1985) Stimulationof denervated rat soleus muscle with fast and slow activity patternsinduces different expression of acetylcholinesterase molecularforms. J Neurosci 5:1180-1187[Abstract].
Magazanik LG, Fedorov VV, Giniatullin RA, Nikolsky EE (1984) Functionalrole of cholinesterase in different types of neuro-muscular junction. In: Cholinesterases:fundamental and applied aspects (Brzin M, Barnard EA, Sket D, eds), pp 229-242. Berlin: Walterde Gruyter.
Marnay A, Nachmansohn D (1938) Cholineesterase in voluntary muscle. JPhysiol (Lond) 92:37-47.
Massoulié J, Bon S (1982) Themolecular forms of cholinesterase and acetylcholinesterase invertebrates. Annu Rev Neurosci 5:57-106[ISI][Medline].
Michel RN, Vu CQ, Tetzlaff W, Jasmin BJ (1994) Neuralregulation of acetylcholinesterase mRNAs at mammalian neuromuscularsynapses. J Cell Biol 127:1061-1069[Abstract/Free Full Text].
Navarrete R, Vrbovà G (1983) Changesof activity patterns in slow and fast muscles during postnataldevelopment. Dev Brain Res 8:11-19.
New HV, Mudge AW (1986) Calcitoningene-related peptide regulates muscle acetylcholine receptor synthesis. Nature 323:809-811[Medline].
Pette D, Staron RS (1990) Cellularand molecular diversities of mammalian skeletal muscle fibers. RevPhysiol Biochem Pharmacol 116:1-76[Medline].
Pette D, Staron RS (1997) Mammalianskeletal muscle fiber type transitions. IntRev Cytol 170:143-223[Medline].
Pette D, Vrbovà G (1992) Adaptationof mammalian skeletal muscle fibers to chronic electrical stimulation. RevPhysiol Biochem Pharmacol 120:115-220[ISI][Medline].
Pette D, Vrbovà G (1994) Transformationof skeletal muscle induced by electrical stimulation. AnnCard Surg 7:14-21.
Pun S, Tsim KW (1995) Truncatedform of pro-acetylcholine receptor-inducing activity (ARIA) inducesAChR $alpha$ -subunit but not AChE transcripts in cultured chick myotubes. NeurosciLett 198:107-110[ISI][Medline].
Purves D, Sakmann B (1974) Theeffect of contractile activity on fibrillation and extrajunctionalacetylcholine-sensitivity in rat muscle maintained in organ culture. JPhysiol (Lond) 237:157-182[Abstract/Free Full Text].
Ribari $c$ S, Peterec D, Sketelj J (1996) Computeraided data acquisition and analysis of acetylcholinesterase velocitysedimentation profiles. ComputMethods Programs Biomed 49:149-156[ISI][Medline].
Rossi SG, Rotundo RL (1996) Transientinteractions between collagen-tailed acetylcholinesterase andsulfated proteoglycans prior to immobilization on the extracellularmatrix. J Biol Chem 271:1979-1987[Abstract/Free Full Text].
Rotundo RL, Rossi SG, Anglister L (1997) Transplantationof quail collagen-tailed acetylcholinesterase molecules onto thefrog neuromuscular synapse. JCell Biol 136:367-374[Abstract/Free Full Text].
Rubin LL, Chalfin NA, Adamo A, Klymkovsky MW (1985) Cellularand secreted forms of acetylcholinesterase in mouse muscle culture. JNeurochem 45:1932-1940[ISI][Medline].
Salafsky B, Bell J, Prewitt MA (1968) Developmentof fibrillation potentials in denervated fast and slow skeletalmuscle. Am J Physiol 215:637-643[Free Full Text].
Schiaffino S, Gorza L, Aussoni S, Botinelli R, Reggiani C, Larson L, Edström L, Gundersen K, Lømo T (1990) Musclefiber types expressing different myosin heavy chain isoforms:the functional properties and adaptive capacity. In: Thedynamic state of muscle fibers (Pette D, ed), pp 329-341. Berlin: Walterde Gruyter.
Shapira M, Seidman S, Sternfeld M, Timberg R, Kaufer D, Patrick J, Soreq H (1994) Transgenicengineering of neuromuscular junctions in Xenopus laevis embryostransiently overexpressing key cholinergic proteins. ProcNatl Acad Sci USA 91:9072-9076[Abstract/Free Full Text].
Simoneau J-A, Pette D (1988) Speciesspecific effects of chronic nerve stimulation upon tibialis anteriormuscle in mouse, rat, guinea pig, and rabbit. PflügersArch 412:86-92[ISI][Medline].
Sketelj J (1994) Neural regulation of acetylcholinesterasein skeletal muscles. BAM 4:281-291.
Sketelj J, Brzin M (1985) Asymmetricmolecular forms of acetylcholinesterase in mammalian skeletalmuscle. J Neurosci Res 14:95-103[ISI][Medline].
Sketelj J, $C$ re $s$ nar B (1995) Neuralregulation of acetylcholinesterase expression in slow and fastmuscles of the rat. In: Enzymesof the cholinesterase family (Quinn DM, Balasubramanian AS, Doctor BP, Taylor P, eds), pp 253-260. NewYork: Plenum.
Sketelj J, $C$ rne N, Brzin M (1987) Molecularforms and localization of acetylcholinesterase and nonspecificcholinesterase in regenerating skeletal muscles. NeurochemRes 12:159-165[ISI][Medline].
Sketelj J, $C$ rne N, Ribari $c$ S, Brzin M (1991) Interactionsbetween intrinsic regulation and neural modulation of acetylcholinesterasein fast and slow skeletal muscle. CellMol Neurobiol 11:35-54[ISI][Medline].
Sketelj J, $C$ rne-Finderle N, Brzin M (1992a) Influenceof denervation on the molecular forms of junctional and extrajunctionalacetylcholinesterase in fast and slow muscles of the rat. NeurochemInt 21:415-421[ISI][Medline].
Sketelj J, $C$ rne-Finderle N, Dolenc I (1992b) Factorsinfluencing acetylcholinesterase regulation in slow and fast skeletalmuscles. In: Multidisciplinaryapproaches to cholinesterase functions (Shafferman A, Velan B, eds), pp 209-216. NewYork: Plenum.
Sketelj J, $C$ rne-Finderle N, Sket D, Dettbarn W-D, Brzin M (1993) Comparisonbetween the effects of botulinum toxin-induced paralysis and denervationon molecular forms of acetylcholinesterase in muscles. JNeurochem 61:501-508[ISI][Medline].
Sketelj J, Leisner E, Gohlsch B, $S$ korjanc D, Pette D (1997) Specificimpulse patterns regulate acetylcholinesterase activity in skeletalmuscles of rats and rabbits. JNeurosci Res 47:49-57[ISI][Medline].
Snoj-Cvetko E, Smerdu V, Sketelj J, Dolenc I, d'Albis A, Janmot C, Er $z$ en I (1996) Adaptiverange of myosin heavy chain expression in regenerating soleusis broader than in mature muscle. JMuscle Res Cell Motil 17:401-409[ISI][Medline].
Sugiyama H (1977) Multiple forms of acetylcholinesterasein clonal muscle cells. FEBSLett 84:257-260[ISI][Medline].
Termin A, Staron RS, Pette D (1989) Changesin myosin heavy chain isoforms during chronic low-frequency stimulationsof rat fast hind limb muscles: a single fiber study. EurJ Biochem 186:749-754[ISI][Medline].
Tyler KR, Wright AJA (1980) Lightweight portable stimulators for stimulation of skeletal musclesat different frequencies and for cardiac pacing. JPhysiol (Lond) 307:6P-7P.
Westgaard RH, Lømo T (1988) Controlof contractile properties within adaptive ranges by patterns ofimpulse activity in the rat. JNeurosci 8:4415-4426[Abstract].

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