Nitric Oxide Is Involved in Acetylcholinesterase Inhibitor-Induced Myopathy in Rats

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Vol. 295, Issue 1, 314-320, October 2000

Nitric Oxide Is Involved in Acetylcholinesterase Inhibitor-Induced Myopathy in Rats¹

Gayathri Jeyarasasingam², Michael Yeluashvili and Maryka Quik

The Parkinson's Institute, Sunnyvale, California

	Abstract

Top Abstract Introduction Experimental Procedures Results Discussion References

Excess activation of muscle nicotinic acetylcholine receptors due to genetic mutations, as seen in slow channel congenitalmyasthenic syndrome, or acetylcholinesterase (AChE) inhibitionresults in muscle cell degeneration. Our recent work showed thatnitric oxide synthase (NOS) inhibitors prevent nicotine-inducedmuscle cell death in culture. In the present study, we examinedthe effects of NOS inhibition on nicotinic receptor-mediated myopathyin vivo. Rats injected with the AChE inhibitor paraoxon demonstratea 90-fold increase in the number of dying muscle cells comparedwith control as evidenced histologically by centralized nucleiand the presence of degenerating profiles. Coadministration ofthe nonspecific NOS inhibitor nitro-L-arginine methyl ester orthe neuronal NOS-specific inhibitor 7-nitroindazole dramaticallyreduced the presence of such degenerating profiles to ~20% ofthat seen with paraoxon alone. These results show that inhibitionof NOS, as well as neuronal NOS, significantly reduces AChE inhibitor-inducedmuscle cell degeneration, suggesting that increased nitric oxideproduction mediates suchmyopathy.

	Introduction

Top Abstract Introduction Experimental Procedures Results Discussion References

Nicotinic acetylcholine receptors play a prominent role in synaptic transmission at the neuromuscular junction and have alsobeen implicated in cellular differentiation, maturation, and degeneration.In humans, the excess activation of nicotinic acetylcholine receptors,observed in slow channel congenital myasthenic disorder, resultsin severe myopathy that is associated with muscle fatigue andeventual paralysis (Engel et al., 1982). Similarly, chronic fatigueis a symptom of Gulf War syndrome, a disorder proposed to resultfrom exposure to acetylcholinesterase (AChE) inhibitors (Sapolsky,1998). Although the degree of muscle viability in these patientshas not been examined, it is well established that rodents exposedto AChE inhibitors demonstrate muscle fiber degeneration (Arienset al., 1969; Fenichel et al., 1972; Leonard and Salpeter, 1979).For example, injection of paraoxon, the active metabolite of theinsecticide parathion, results in marked muscle degeneration (Arienset al., 1969), the severity of which is correlated with the durationof cholinesterase inhibition (Wecker et al., 1978).

Several experimental approaches indicate that administration of AChE inhibitors leads to muscle degeneration by enhancingthe concentration of acetylcholine at the synaptic cleft. Priornerve transection or administration of the nicotinic receptorantagonist d-tubocurarine both prevented AChE inhibitor-inducedmyopathy (Ariens et al., 1969). As well, AChE inhibitor-mediateddegenerative effects were blocked by administration of the acetylcholinetransport blocker hemicholinium, which depletes nerve terminalacetylcholine (Fenichel et al., 1972). Furthermore, agents thatreactivate AchE activity, such as pyridine-2-aldoxime methochloride,attenuated myopathy (Wecker et al., 1978).

Although the majority of intracellular events that mediate nicotinic receptor-induced myopathy have not yet been identified,calcium may play a role. Evidence for this stems from studiesthat show that carbachol-induced muscle degeneration in cultureis prevented by removing calcium from the bathing solution (Leonardand Salpeter, 1979, 1982). Moreover, generation of the free radicalmessenger nitric oxide (NO) has been shown to play an intermediaryrole in nicotinic receptor-mediated muscle cell death in culture(El-Dada and Quik, 1997). Similarly, NO has been implicated incytotoxicity in the central nervous system (CNS) (Garthwaite andBoulton, 1995; Schulz et al., 1996; Brenman and Bredt, 1997).For example, NO mediates N-methyl-D-aspartate (NMDA) receptor-inducedexcitotoxicity (Dawson et al., 1991) where calcium influx resultingfrom receptor activation stimulates NO production and leads toneuronaldeath.

NO is synthesized from L-arginine via the enzyme nitric oxide synthase (NOS). Three different NOS isoforms have been identified:two constitutive, calcium/calmodulin-dependent forms, endothelial(eNOS) and neuronal NOS (nNOS), and an inducible form. Both nNOSand eNOS have been localized to skeletal muscle (Kobzik et al.,1994, 1995; Silvagno et al., 1996) and have been demonstratedto affect muscle contractility (Kobzik et al., 1994). In addition,nNOS is concentrated at the synaptic junction of motor end platesof skeletal muscle, colocalizing with nicotinic receptors (Brenmanet al., 1995, 1996).

Chronic muscle stimulation increases nNOS protein expression and NOS activity (Reiser et al., 1997). Although enhanced NOSactivity under physiological conditions may be essential for normalmuscle function, it is plausible that excessive receptor stimulationincreases NO production to pathological levels. Such a hypothesisis consistent with our earlier studies that implicate NO in receptor-mediatedmuscle cell death in culture (El-Dada and Quik, 1997). The purposeof the present study was to investigate whether NOS inhibitorsprevent myopathy induced by the AChE inhibitor paraoxon invivo.

	Experimental Procedures

Top Abstract Introduction Experimental Procedures Results Discussion References

Materials. Paraoxon, nitro-L-arginine methyl ester (L-NAME), 7-nitroindazole (7-NI), hematoxylin, eosin, leupeptin, aprotinin, pepstatin,calmodulin, EDTA, phenylmethylsulfonyl fluoride, NADPH, and $beta$ -mercaptoethanolwere purchased from Sigma Chemical Co. (St. Louis, MO), [³H]arginine from New England Nuclear (Boston, MA), and Dowex 50W-X8resin from Bio-Rad Laboratories (Mississauga, Ontario, Canada).All other chemicals were purchased from standard commercialsources.

Animals. All experiments were carried out in accordance with the National Institutes of Health Guide for the Care and Use of LaboratoryAnimals and were approved by the Institutional Animal Care andUse Committee. Adult male Sprague-Dawley rats weighing 180 to200 g were used. Paraoxon or saline was injected i.p. once dailyfor 4 days, unless indicated otherwise, at doses of 0.25 or 0.4mg/kg. The rats showed few adverse effects with the i.p. routeof administration. These doses were selected based on the resultsof previous studies that 1) demonstrated the occurrence of myopathywith such treatments (Fenichel et al., 1972; Laskowski et al.,1975, 1977; Wecker et al., 1978). Furthermore, 2) they showedan almost complete decline in AChE activity immediately afterthe administration of paraoxon that returned to about 20 to 50%of control after 24 h, depending on the specific skeletal musclegroup studied; these levels of inhibition persisted with repeatedadministration (Wecker and Dettbarn, 1976; Wecker et al., 1978).

L-NAME (5-20 mg/kg) or saline was injected i.p. 1 h before and 6 h after each paraoxon injection. This scheduling regimenwas selected because previous studies had shown that two systemicinjections of L-NAME given 8 h apart produced an inhibition thatwas rapid in onset and lasted for at least 24 h (Connop et al.,1995

). 7-NI (5-20 mg/kg), dissolved in peanut oil, or vehiclewas injected i.p. 1 h before and 4 h after each paraoxon injection.7-NI was administered 4 h rather than 6 h after paraoxon administrationbecause of the shorter duration of action of this NOS inhibitorcompared with L-NAME. Previous reports had shown that maximalinhibition of NOS activity was obtained 30 to 60 min after injectionof 7-NI, with a 30% inhibition remaining after 4 h (Connop etal., 1996

; Kalisch et al., 1996

; Przedborski et al., 1996

). Theconcentration range for L-NAME and 7-NI used in these experimentswas within that reported in the literature (Connop et al., 1995

,1996

; Kalisch et al., 1996

; Przedborski et al., 1996

; Taraskaand Finnegan, 1997

Tissue Preparation. Twenty-four hours after the last injection, animals were euthanized with CO₂, and the diaphragm and leg muscles, includingsoleus, gastrocnemius, and plantaris, were dissected. Muscle tissuewas washed in 0.9% saline, mounted in histoprep mounting medium,snap frozen in liquid N₂-cooled isopentane, and sectioned at 10µm on a cryostat. Sections were fixed in 100% ethanol for 10 min,and washed in running tap water for 5 min before staining. Sectionswere then incubated in Harris' hematoxylin for 15 to 20 min, washedin tap water, incubated in acid alcohol, and rinsed in tap water,followed by incubation in ammonia water. Sections were rinsedagain before being stained in eosin for 5 min, washed and dehydratedin graded series of ethanol, cleared in xylene, and coverslippedusingDepex.

Cell Counts. A minimum of 10 grids from each tissue section was counted at a final magnification of 100×. A cell was considered degeneratingif it had centralized nuclei, macrophage infiltration, or eosinophilia(Ariens et al., 1969). The number of degenerating profiles isexpressed as the number of lesions per 1000 totalcells.

NOS Assay. NOS activity was determined by monitoring the conversion of [³H]arginine to [³H]citrulline as previously described by Kobzik et al. (1995) withminor modifications. Rat skeletal muscle tissue was homogenizedin 4 volumes of 50 mM HEPES (pH 7.5) containing 5 mM KCl, 120mM NaCl, 10 mM glucose, 1 mM EDTA, 10 µg/ml pepstatin A, 10 µg/mlleupeptin, 10 µg/ml aprotinin, 100 µg/ml phenylmethylsulfonylfluoride, and 5 mM $beta$ -mercaptoethanol. Homogenate was then incubatedin 50 mM HEPES (pH 7.5) containing 5 mM KCl, 120 mM NaCl, 10 mMglucose, 20 µg/ml calmodulin, 2 mM NADPH, 2.5 mM CaCl₂, and 1µCi/ml [³H]arginine for 45 min at 37°C. The reaction was terminated byaddition of 1 ml of 20 mM HEPES (pH 5.5) containing 2 mM EDTA.The samples were applied to 1-ml columns of Bio-Rad AG 50W-X8resin and eluted with 2 × 1.0 ml of distilled water. [³H]Citrulline was quantified by liquid scintillation spectroscopyof the 3 × 1 ml flowthrough.

Data Analysis. All values are expressed as the mean ± S.E. Results of cell counts were analyzed using a one-way ANOVA followed by a Fisher'sprotected least-significant difference test. Results of the NOSassay were analyzed using a Student's ttest.

	Results

Top Abstract Introduction Experimental Procedures Results Discussion References

Paraoxon Induces Muscle Cell Degeneration in a Time- and Dose-Dependent Manner. Adult rats were injected once daily with 0.25 or 0.4 mg/kg of the AChE inhibitor paraoxon for 2, 4, or 8 days. Such a treatmentwas selected because previous studies by Wecker and Dettbarn (1976)had shown that paraoxon at somewhat lower doses had resulted inan almost complete inhibition of AChE activity 30 min after administrationwith 20 to 50% declines 24 h after the initial injection. Degeneratingmuscle fibers were identified based on the presence of centralizednuclei, eosinophilia, and macrophage infiltration (Ariens et al.,1969). There was no significant increase in the number of degeneratingmuscle cells with either dose of paraoxon after 2 days of treatmentin diaphragm or leg muscle (Fig. 1). However, the number of degeneratingfibers was significantly enhanced over control after administrationof 0.4 mg/kg paraoxon for 4 days in muscle sections from bothdiaphragm and leg (Figs. 1-3). Considerably less degeneration wasobserved in leg muscle compared with diaphragm as has been reportedpreviously (Ariens et al., 1969; Wecker and Dettbarn, 1976). Similarto 4 days of treatment, injection of 0.4 mg/kg paraoxon for 8days resulted in a significant increase in the number of degeneratingprofiles compared with control, although this was not significantlydifferent from the 4-day time point (Fig. 1). We, therefore, usedan injection regimen of 0.4 mg/kg daily for 4 days for all subsequentexperiments to produce a significant level of degeneration.

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Fig. 1. Effect of varying dose and time of paraoxon treatment on diaphragm and leg muscle degeneration. Rats were injected with either vehicle, 0.25 or 0.4 mg/kg paraoxon for 2, 4, or 8 days. The number of degenerating fibers per 1000 cells was counted. The columns represent mean ± S.E. of the number of animals indicated in parentheses. Significance of difference from control: *P < .05, **P < .01, ***P < .001.

L-NAME Decreases Paraoxon-Induced Degeneration. To determine whether NO mediates paraoxon-induced myopathy, rats were treated with the reversible NOS inhibitor L-NAME 1 hbefore and 6 h after paraoxon treatment. L-NAME injections (20mg/kg) alone produced no effect on muscle cell morphology comparedwith control (Table 1). However, L-NAME at a dose of 10 mg/kgsignificantly decreased paraoxon-induced muscle fiber degenerationin sections from both diaphragm (Figs. 2 and 4) and leg (Figs.3 and 4). Higher concentrations of L-NAME did not further reduceparaoxon-induced damage. In fact, there appears to be somewhatless of a protective effect at 20 mg/kg L-NAME.

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TABLE 1
Effect of NOS inhibitor administration on muscle cell morphology
Each animal received saline injections daily for 4 days and either vehicle or the indicated NOS inhibitor at the dose specified 1 h before and 6 h (L-NAME), or 4 h (7-NI) after saline injection. Animals were sacrificed 24 h after the last injection, and the tissue was sectioned, stained, and counted for the presence of degenerating profiles. Each value represents the mean ± S.E. of the number of animals (n) indicated in parentheses.

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Fig. 2. Photomicrographs of diaphragm muscle sections treated with vehicle, paraoxon (0.4 mg/kg), and paraoxon + L-NAME (10 mg/kg). Arrows indicate degenerating fibers. Scale bar, 100 µm.

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Fig. 3. Photomicrographs of leg muscle sections treated with vehicle, paraoxon (0.4 mg/kg), and paraoxon + L-NAME (10 mg/kg). Arrows indicate degenerating fibers. Scale bar, 200 µm.

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Fig. 4. Effect of L-NAME on paraoxon-induced muscle degeneration. Rats were injected with L-NAME (doses in mg/kg listed below each column) 1 h before and 6 h after paraoxon treatment (0.4 mg/kg). Note that 10 mg/kg L-NAME significantly reduced paraoxon-induced myopathy in both diaphragm and leg. The columns represent mean ± S.E. of the number of animals indicated in parentheses. Significance of difference from control: *P < .05. Significance of difference from paraoxon in the absence of L-NAME: ^#P < .05, ^##P < .01.

Neuronal NOS Mediates AChE Inhibitor-Induced Myopathy. The results with L-NAME suggest that NO mediates AChE inhibitor-induced myopathy, at least in part. Because the neuronal isoformhas been shown to colocalize with nicotinic receptors (Brenmanet al., 1995, 1996), we sought to determine whether activationof nNOS may mediate paraoxon-induced muscle degeneration. Ratswere treated with 7-NI, an NOS inhibitor specific for the neuronalisoform, 1 h before and 4 h after paraoxon treatment every dayfor 4 days. As seen with L-NAME, 7-NI administration (20 mg/kg)alone had no effect on muscle tissue degeneration (Table 1).The ability of 7-NI to attenuate paraoxon-induced myopathy wassimilar to that observed with L-NAME. At concentrations of 7-NIlower than 10 mg/kg, there was no significant reversal of paraoxon-inducedmyopathy. However, 7-NI at a dose of 10 mg/kg significantly reducedparaoxon-induced muscle cell death in both diaphragm and leg sections(Fig. 5). A dose of 20 mg/kg 7-NI also significantly reduced theincidence of degenerating profiles in diaphragm compared withparaoxon treatment alone, although to a lesser degree than the10-mg/kg dose. This, however, was not the case for leg musclesections, where the extent of muscle degeneration observed aftertreatment with 20 mg/kg 7-NI was not significantly different fromparaoxon treatment alone, although it was also not significantlydifferent from control. The maximal protective effect of 7-NIis comparable with that produced by L-NAME, suggesting that paraoxon-inducedmuscle cell degeneration is due to the activation of nNOS.

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Fig. 5. Effect of 7-NI on paraoxon-induced muscle degeneration. Rats were injected with 7-NI (doses in mg/kg listed below each column) 1 h before and 4 h after paraoxon treatment (0.4 mg/kg). Note that 10 mg/kg 7-NI significantly reduces paraoxon-induced myopathy in both diaphragm and leg, and 20 mg/kg 7-NI decreases myopathy in diaphragm. The columns represent mean ± S.E. of the number of animals indicated in parentheses. Significance of difference from control: **P < .01. Significance of difference from paraoxon in the absence of 7-NI: ^#P < .05, ^##P < .01.

NOS Activity in Control and Paraoxon-Treated Muscle Tissue. To determine whether paraoxon treatment resulted in an increase in muscle NOS activity, we assessed the calcium-dependentNOS-mediated conversion of [³H]arginine to [³H]citrulline in homogenized muscle tissue from control and paraoxon-treatedanimals. Rats were injected i.p. once daily with paraoxon (0.4mg/kg) for 4 days, a similar regimen in which myopathy was observed(Fig. 1). There was a small (13%) although not statistically significantincrease in muscle NOS activity in paraoxon-treated rats (1.96± 0.1 fmol/mg of tissue, n = 5) compared with control (1.74 ±0.2 fmol/mg of tissue, n =4).

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

The present study demonstrates that paraoxon-induced muscle cell degeneration is decreased by exposure to the nonspecificNOS inhibitor L-NAME. Moreover, the nNOS-specific inhibitor 7-NIproduces an equivalent level of protection as L-NAME against AChEinhibitor-induced myopathy, suggesting that activation of nNOSis involved. These experiments extend our previous results withmuscle cells in culture (El-Dada and Quik, 1997) to the in vivosituation, and may suggest that excess stimulation of nicotinicreceptors after AChE inhibitor administration results in increasednNOS activity to induce muscledegeneration.

As an approach to directly test this possibility, we measured NOS activity in muscle tissue from control and paraoxon-treatedanimals. There was a small increase in enzyme activity after paraoxontreatment, although it was not significantly different from control.Our data with the nNOS-specific inhibitor 7-NI suggest that nNOSis the primary NOS isoform involved in AchE-induced myopathy.Because muscle tissue contains both the eNOS and nNOS isoforms(Kobzik et al., 1995), the present results may suggest that anincrease in muscle nNOS activity in paraoxon-treated tissue ismasked by high basal levels of eNOS, as well as nNOS. Experimentswith nNOS knockout mice may prove useful in evaluating the involvementof nNOS in AchE-induced myopathy, although there is the possibilityof compensatory changes by other NOSisoforms.

Indirect evidence from other in vivo studies has also implicated NO in both cardiac and skeletal muscle injury. One majorpathway through which NO induces cellular injury is through itsreaction with superoxide anion and the formation of peroxynitrite,a highly reactive free radical species that is known to mediateoxidative injury. Consistent with this role of NO, peroxynitritelevels are elevated in cardiac muscle after ischemia-reperfusioninjury (Wang and Zweier, 1996). Moreover, exposure to the NOSinhibitor L-NAME prevents such reperfusion-induced injury to cardiacmyocytes (Wang and Zweier, 1996). Pretreatment with L-NAME alsoincreases cell viability in gastrocnemius muscle after limb ischemia-reperfusioninjury (Knight et al., 1997). NO has been implicated in othermodels of muscle injury as well. For example, L-NAME has beenshown to rescue muscle cells from mechanical crush injury (Rubinsteinet al., 1998). Similarly, in a mouse model of cachexia, a conditioncharacterized by weight loss primarily due to muscle wasting,administration of the NOS inhibitor nitro-arginine prevented myopathy(Buck and Chojkier, 1996).

In addition to a destructive role in the periphery, NO has been implicated in many neurodegenerative processes in the CNSsuch as those involved in Parkinson's disease, Alzheimer's disease,Huntington's disease, amyotrophic lateral sclerosis, and cerebralischemia (Dawson et al., 1991; Lipton and Rosenberg, 1994; Schulzet al., 1996). There is significant support for the idea thatNMDA receptor-mediated neurotoxicity, which is thought to contributeto ischemic damage, occurs via NO. For example, NOS inhibitorsprevent glutamate neurotoxicity in primary cortical cultures (Dawsonet al., 1991). Moreover, administration of NOS inhibitors decreasedthe severity of NMDA-mediated excitotoxic lesions in mouse striatum(Ayata et al., 1997). Our data demonstrating that excess nicotinicreceptor stimulation is attenuated by NOS inhibitors are consistentwith the results from these models of CNSexcitotoxicity.

AChE inhibitors such as paraoxon have been reported to have several actions in relation to nicotinic acetylcholine receptors.First, cholinesterase inhibitors enhance muscle responses to nervestimulation due to the prolonged action of acetylcholine withinthe synaptic cleft (Clark and Hobbiger, 1983). In addition, suchcompounds act as weak noncompetitive agonists on acetylcholinereceptors at low concentrations (Rao et al., 1987; Storch et al.,1995) unrelated to their actions as cholinesterase inhibitors.Although AChE inhibitors have low efficacy at activating the receptor,they do potentiate receptor responses to acetylcholine (Storchet al., 1995). Therefore, in addition, to the excess presenceof acetylcholine in the synaptic cleft, the cholinesterase inhibitoritself may further increase the response of the receptor, resultingin excessive stimulation and thereby leading to calcium entryand ultimately muscle celldegeneration.

In contrast to the above-mentioned effects, there have also been reports that AChE inhibitors block nicotinic receptor-mediatedactivity, particularly at high concentrations. Katz et al. (1997)showed that paraoxon bound to and desensitized muscle-type nicotinicreceptors in membrane preparations with an IC₅₀ of 300 µM, whereasVan Den Beukel et al. (1998) showed that paraoxon reduced nicotinicreceptor-mediated currents in neuronal cell cultures with an IC₅₀value of 100 µM. If we assume a uniform distribution of paraoxonafter injection of our standard dose of 0.4 mg/kg i.p., we estimatea tissue concentration of approximately 1 to 2 µM. Thus, a directinhibitory action of paraoxon at the level of the receptor appearsunlikely in the presentexperiments.

Previous studies have demonstrated that nicotinic acetylcholine receptor activation results in a calcium influx, which mayactivate numerous intracellular calcium-dependent processes. Althoughthe maximum calcium entry through nicotinic receptors only accountsfor 2% of the total current, receptor stimulation may also activatevoltage-gated calcium channels, resulting in a greater calciuminflux (Decker and Dani, 1990). It is well known that calciumhomeostasis is critical for maintaining cellular viability. Eitherlowering or raising intracellular calcium concentrations can resultin cellular degeneration (McBurney and Neering, 1987). Therefore,excess activation of these receptors, as is seen after exposureto AChE inhibitors in vivo, may raise the intracellular calciumconcentration to pathological levels. Such an interpretation issupported by the work of Leonard and Salpeter (1979, 1982) whoshowed that removal of calcium prevented nicotinic receptor-inducedmyopathy in vitro. The present results, as well as others, maynow suggest that alterations in intracellular calcium subsequentlytrigger the activation of NOS.

The results show that a lower dose (10 mg/kg) of L-NAME reversed the toxic effects of paraoxon on muscle, whereas a higherdose (20 mg/kg) did not significantly reduce paraoxon-inducedmyopathy, although an approximate 50% decline in muscle degenerationwas still observed. With 7-NI, on the other hand, there was stilla significant decline in myopathy at the higher concentration,at least in diaphragm, albeit of a slightly smaller magnitude.NOS inhibitors on their own did not result in myopathy at anydose tested. These observations may suggest that the higher dosesof the NOS inhibitors decrease NO production to levels below thatnecessary for optimal function only when the system is compromisedas in the presence of an AChE inhibitor. Such an interpretationis consistent with studies that show that NO is involved in diversebiological functions ranging from development and homeostasisto degenerative effects (Garthwaite and Boulton, 1995; Brenmanand Bredt, 1997). Another or alternate possibility may relateto the fact that L-NAME inhibits both nNOS and eNOS, whereas 7-NIpreferentially inhibits nNOS. A reduction in nNOS activity mayprevent myopathy; however, inhibition of eNOS may block vasodilationto enhance neurodegenerative effects (Brenman and Bredt, 1997).

A question that arises is the time requirements for AChE-induced degenerative effects. This is important because it may provideinsight into the molecular mechanisms that mediate myopathy. Inthe CNS, it has been shown that an initial brief insult can generatea series of events to result in a delayed toxicity. For instance,a 5-min exposure to glutamate results in marked neurodegenerativeeffects 24 h later (Dawson et al., 1991). A similar mechanismmay also apply in the current studies, especially in view of anextensive literature that shows that nicotinic receptor activationresults in an initial excitatory response followed by a rapiddesensitization, which may persist in the presence of continuedAChE inhibition (Edmonds et al., 1995). As the effect of the AChEinhibitor diminishes over time, there may be a resensitizationof receptor-mediated responses. Experiments with different treatmentregimens will be necessary to determine whether exposure to shortpulses of acetylcholine or chronic exposure to high levels ofacetylcholine produce a more severe myopathy. However, because1) paraoxon-induced myopathy is more robust than that which occursin the presence of the more reversible AChE inhibitors such asneostigmine and physostigmine (Wecker et al., 1978), and 2) prolongedexposure to carbachol induces more severe degenerative effectsin muscle cells in culture than a brief exposure period (Leonardand Salpeter, 1979), the extent of myopathy may represent a complexinterplay between receptor stimulation, desensitization, andresensitization.

In summary, these studies show that NOS inhibition decreases paraoxon-induced muscle cell degeneration in rodents and supporta role for nNOS in mediating this effect. These findings are thefirst to suggest that increased NO levels downstream of nicotinicreceptor activation mediate agonist-induced myopathy in vivo.The current work may suggest that NOS inhibitors have the potentialto provide therapeutic benefit in slow channel congenital myasthenicdisorder.

	Footnotes

Accepted for publication June 9, 2000.

Received for publication April 6, 2000.

¹ This study was supported by the Muscular Dystrophy Association, USA #2421, and the California Tobacco Related Disease Program#7FT-0010.

² Present address: Extramural Review Branch, National Institute of Mental Health, 6001 Executive Blvd., Room 6154, MSC 9609,Bethesda, MD 20892-9609 [Rockville, MD 20852 (for express/courierservice)].

Send reprint requests to: Dr. Maryka Quik, The Parkinson's Institute, 1170 Morse Ave., Sunnyvale, CA 94089-1605. E-mail: mquik{at}parkinsonsinstitute.org

	Abbreviations

AChE, acetylcholinesterase; NO, nitric oxide; CNS, central nervous system; NMDA, N-methyl-D-aspartate; NOS, nitric oxide synthase; eNOS, endothelial nitric oxide synthase; nNOS, neuronal nitric oxide synthase; L-NAME, nitro-L-arginine methyl ester; 7-NI, 7-nitroindazole.

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