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Vasopressin Preferentially Depresses Excitatory Over Inhibitory Synaptic Transmission in the Rat Supraoptic Nucleus In Vitro
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Endogenous arginine‐vasopressin (AVP) in the supraoptic nucleus is known to decrease the firing rate of some supraoptic nucleus neurones. To determine a possible mechanism by which this locally released AVP produces this change in neuronal excitability, we investigated the effects of AVP on evoked excitatory (e.p.s.c.) and inhibitory post‐synaptic (i.p.s.c.) responses recorded in magnocellular neurones in a hypothalamic slice preparation, using the perforated‐patch recording technique. Our data show that AVP produces a dose‐dependent decrease in the evoked e.p.s.c. in about 80% of magnocellular neurones tested with an estimated EC50 of about 0.9 μM. The maximum decrease in e.p.s.c. amplitude was about 31% of control and was obtained with an AVP concentration of 2 μM. The AVP‐induced synaptic depression was blocked by Manning Compound (MC), a non‐selective antagonist of oxytocin (OXT) and vasopressin (AVP) receptors, but not by a selective OXT receptor antagonist. It was not mimicked by desmopressin (ddAVP), a V2‐receptor subtype agonist. By contrast, AVP used at the same concentration (2 μM), had no global effect on pharmacologically isolated i.p.s.c.s in the majority of magnocellular neurones tested. These results show that AVP acts in the supraoptic nucleus to reduce excitatory synaptic transmission to magnocellular neurones by activating a non‐OXT receptor, presumably the V1 receptor subtype.
Title: Vasopressin Preferentially Depresses Excitatory Over Inhibitory Synaptic Transmission in the Rat Supraoptic Nucleus In Vitro
Description:
Endogenous arginine‐vasopressin (AVP) in the supraoptic nucleus is known to decrease the firing rate of some supraoptic nucleus neurones.
To determine a possible mechanism by which this locally released AVP produces this change in neuronal excitability, we investigated the effects of AVP on evoked excitatory (e.
p.
s.
c.
) and inhibitory post‐synaptic (i.
p.
s.
c.
) responses recorded in magnocellular neurones in a hypothalamic slice preparation, using the perforated‐patch recording technique.
Our data show that AVP produces a dose‐dependent decrease in the evoked e.
p.
s.
c.
in about 80% of magnocellular neurones tested with an estimated EC50 of about 0.
9 μM.
The maximum decrease in e.
p.
s.
c.
amplitude was about 31% of control and was obtained with an AVP concentration of 2 μM.
The AVP‐induced synaptic depression was blocked by Manning Compound (MC), a non‐selective antagonist of oxytocin (OXT) and vasopressin (AVP) receptors, but not by a selective OXT receptor antagonist.
It was not mimicked by desmopressin (ddAVP), a V2‐receptor subtype agonist.
By contrast, AVP used at the same concentration (2 μM), had no global effect on pharmacologically isolated i.
p.
s.
c.
s in the majority of magnocellular neurones tested.
These results show that AVP acts in the supraoptic nucleus to reduce excitatory synaptic transmission to magnocellular neurones by activating a non‐OXT receptor, presumably the V1 receptor subtype.
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