Abstract
Contrary to its effect on the gamma-aminobutyric acid type A and C receptors, picrotoxin antagonism of the alpha1 homomeric glycine receptors (GlyRs) has been shown to be non-use-dependent and nonselective between the picrotoxin components picrotoxinin and picrotin. Picrotoxin antagonism of the embryonic alpha2 homomeric GlyR is known to be use-dependent and reflects a channel-blocking mechanism, but the selectivity of picrotoxin antagonism of the embryonic alpha2 homomeric GlyRs between picrotoxinin and picrotin is unknown. Hence, we used the patch clamp recording technique in the outside-out configuration to investigate, at the single channel level, the mechanism of picrotin- and picrotoxinin-induced inhibition of currents, which were evoked by the activation of alpha2 homomeric GlyRs stably transfected into Chinese hamster ovary cells. Although both picrotoxinin and picrotin inhibited glycine-evoked outside-out currents, picrotin had a 30 times higher IC50 than picrotoxinin. Picrotin-evoked inhibition displayed voltage dependence, whereas picrotoxinin did not. Picrotoxinin and picrotin decreased the mean open time of the channel in a concentration-dependent manner, indicating that these picrotoxin components can bind to the receptor in its open state. When picrotin and glycine were co-applied, a large rebound current was observed at the end of the application. This rebound current was considerably smaller when picrotoxinin and glycine were co-applied. Both picrotin and picrotoxinin were unable to bind to the unbound conformation of the receptor, but both could be trapped at their binding site when the channel closed during glycine dissociation. Our data indicate that picrotoxinin and picrotin are not equivalent in blocking alpha2 homomeric GlyR.
Highlights
PTX is an equimolecular complex of picrotoxinin and picrotin (15), which differ only by a single group, with picrotin having a hydrophilic elongated end
Concentration-dependent Inhibition of ␣2 Homomeric glycine receptors (GlyRs) by Picrotoxinin and Picrotin—We first analyzed the relative potencies of picrotin and picrotoxinin in inhibiting GlyR activity in terms of the outside-out current evoked by glycine applications to outside-out patches containing ␣2 homomeric GlyR from Chinese hamster ovary (CHO) cells stably expressing the ␣2 GlyR subunit
We have proposed previously a simple model that well predicted the inhibitory mechanism of PTX on wild-type homomeric ␣2 GlyRs (9)
Summary
PTX is an equimolecular complex of picrotoxinin and picrotin (15), which differ only by a single group, with picrotin having a hydrophilic elongated end. Picrotin is inactive in inhibiting the GABAAR and GABACR, indicating that the inhibitory effect of PTX is related to picrotoxinin (15, 16) This is not the case for ␣1 homomeric GlyRs. Picrotoxinin and picrotin are potent in inhibiting ␣1 homomeric GlyR activation (17). We showed that picrotoxinin is considerably more potent than picrotin in inhibiting ␣2 homomeric GlyRs, indicating that the inhibitory effect of PTX we previously described (9) is mainly because of picrotoxinin. Picrotoxinin blocks homomeric ␣2 GlyR activation in a voltage-independent manner, picrotin-evoked inhibition appeared to be more voltagedependent Both picrotoxinin and picrotin can bind to the receptor in both the open channel conformation and the liganded closed state. A relatively simpler kinetic model better predicted the blocking mechanism for picrotin
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