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Molecular Pharmacology, Vol 12, 999-1006, Copyright © 1976 by the American Society for Pharmacology and Experimental Therapeutics
-Bungarotoxin with Aplysia Acetylcholine Receptors
1 Neurobiology Department, Armed Forces Radiobiology Research Institute, and Laboratory of Biochemical
Genetics, National Heart and Lung Institute, Bethesda, Maryland 20014, and Bermuda Biological Station,
Bermuda
Binding of [125I]
-bungarotoxin to acetylcholine receptors of ganglionic homogenate of
the marine mollusc Aplysia is blocked by the anticholinesterases eserine (I50 = 4 µM)
and neostigmine (I50 = 0.2 mM). The classical acetylcholine antagonist d-tubocurarine
blocks with an I50 of 2 µM. Eserine (I50 = 3.2 µM) and neostigmine (I50 > 1 mM) also
block toxin binding to a solubilized receptor preparation. In contrast to their relative
potency in blocking toxin binding, neostigmine is a more potent inhibitor of Aplysia
acetylcholinesterase (I50 = 14 nM) than is eserine (I50 = 250 nM). -Bungarotoxin does
not affect esterase activity or interfere with the ability of eserine to block the esterase.
The response to acetylcholine recorded through intracellular microelectrodes is blocked
by -bungarotoxin. Neither eserine nor neostigmine blocks the acetylcholine response;
rather, they prolong and increase it, as expected from their effects on the esterase.
Eserine (0.1 mM) blocks the -bungarotoxin inhibition of the physiological acetylcholine
response. These results indicate that eserine and neostigmine block the binding of -bungarotoxin by interacting with a site which is different from both the esterase and the
cholinergic sites of the acetylcholine receptor.
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