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Vol. 296, Issue 3, 704-711, March 2001
Department of Pharmacology and Experimental Therapeutics, School of
Pharmacy, Faculty of Medicine (E.B.-S., S.A.-R., P.L.), and Department
of Biological Chemistry, Life Sciences Institute (M.L.), The Hebrew
University of Jerusalem, Jerusalem, Israel; William T. Gossett
Neurology Laboratories, Henry Ford Health Sciences Center, and John D. Dingell Veterans Affairs Medical Center, Detroit, Michigan (H.J.)
Pardaxin (PX), an ionophore-peptide neurotoxin isolated from the fish
Pardachirus marmoratus, induces neurotransmitter release from neuronal preparations by both calcium-dependent and
calcium-independent mechanisms. The aim of the present study was to
investigate the role of extracellular signal-regulated kinase
(ERK)/mitogen-activated protein kinase (MAPK) in pardaxin-induced
dopamine (DA) release. The experiments were performed on variants of
the PC12 cell line, an established cellular model for investigating DA
release. Time course experiments indicated that PX, at nontoxic
concentrations, stimulated ERK1 and ERK2 within 5 to 15 min, measured
with a dual phospho-ERK antibody. PX stimulation of ERK activity was
calcium (Ca2+)-dependent and followed by ERK translocation
to the nucleus. This effect was temporally related to PX-induced
exocytosis, and measured by [3H]dopamine release as well
as by a vesicle fusion-based enzyme-linked immunosorbent assay.
Blocking ERK activity with the specific mitogen-activated protein
kinase kinase inhibitors PD98059 (50 µM for 45 min) and UO126 (30 µM for 30 min) inhibited PX-induced exocytosis in the presence but
not in the absence of extracellular Ca2+. These results
suggest the essential role of ERKs in PX-induced DA release under
physiological conditions and support the hypothesis that ERKs are
involved in regulating exocytosis.
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