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Vol. 292, Issue 2, 692-697, February 2000
Douglas Hospital Research Centre (D.S.A., J.C.D., F.M., R.Q.),
Departments of Neurology and Neurosurgery (D.S.A., R.Q.), Pharmacology
and Therapeutics (R.Q.), and Psychiatry (R.Q.), Faculty of Medicine,
McGill University, Montreal, Quebec, Canada.
A detailed investigation of endogenous acetylcholine (ACh) release from
primary embryonic septal cultures is described in this study.
Applications of veratridine (25 µM) or increasing extracellular
concentrations of K+ (6-100 mM) induced robust increases
of endogenous ACh release (~500-15,000 fmol/well/10 min). Release
stimulated with K+ (25 mM) was sustainable and did not
differ significantly over 180 min. ACh release was dependent on
extracellular choline and decreased proportionally to choline
concentrations (0-10 µM). For example, after 30 min of stimulation
with K+ (25 mM), release in the absence of extracellular
choline was ~25% of that associated with 10 µM choline. The
vesicular transport blocker vesamicol (0-5 µM) almost completely
prevented stimulated and basal ACh release at the highest concentration
evaluated, which suggests a mostly vesicular mode of release in this
model. The M2-like muscarinic receptor antagonist AF-DX 384 (0-10 µM) enhanced stimulated ACh release (~150% at the highest
concentration evaluated), whereas the nonspecific muscarinic receptor
agonist oxotremorine (0-10 µM) decreased stimulated release (~60%
at the highest concentration evaluated), suggesting that functional
muscarinic autoreceptors exist in primary embryonic septal cultures.
Novel findings concerning ACh release from primary embryonic septal cultures are reported herein, and the demonstration of ACh release gives further credit to the use of these cultures for studying cholinergic system functioning and in relation to physiology and pathology.
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