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Vol. 11, Issue 7, 2213-2219, July 2000
Departments of Pharmacology and Cellular and Molecular Physiology,
Yale University, New Haven, Connecticut 06520
Channel activity of the calcium release channel from skeletal
muscle, ryanodine receptor type 1, was measured in the presence and
absence of protamine sulfate on the cytoplasmic side of the channel.
Single-channel activity was measured after incorporating channels into
planar lipid bilayers. Optimally and suboptimally calcium-activated
calcium release channels were inactivated by the application of
protamine to the cytoplasmic side of the channel. Recovery of channel
activity was not observed while protamine was present. The addition of
protamine bound to agarose beads did not change channel activity,
implying that the mechanism of action involves an interaction with the
ryanodine receptor rather than changes in the bulk calcium
concentration of the medium. The block of channel activity by protamine
could be reversed either by removal by perfusion with buffer or by the
addition of heparin to the cytoplasmic side of the channel.
Microinjection of protamine into differentiated
C2C12 mouse muscle cells prevented
caffeine-induced intracellular calcium release. The results suggest
that protamine acts on the ryanodine receptor in a similar but opposite
manner from heparin and that protamine can be used as a potent,
reversible inhibitor of ryanodine receptor activity.
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