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Enhanced Desensitization Followed by Unusual Resensitization in Gaba(A) Receptors in Phospholipase C-Related Catalytically Inactive Protein-1/2 Double-Knockout Mice

Pflügers Archiv für die gesamte Physiologie des Menschen und der Tiere/Pflügers Archiv(2014)

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Abstract
Phospholipase C-related catalytically inactive proteins (PRIP-1/2) are previously reported to be involved in the membrane trafficking of GABA(A) receptor (GABA(A)R) and the regulation of intracellular Ca2+ stores. GABA(A)R-mediated currents can be regulated by the intracellular Ca2+. However, in PRIP-1/2 double-knockout (PRIP-DKO) mice, it remains unclear whether the kinetic properties of GABA(A)Rs are modulated by the altered regulation of intracellular Ca2+ stores. Here, we investigated whether GABA(A)R currents (I-GABA) evoked by GABA puff in layer 3 (L3) pyramidal cells (PCs) of the barrel cortex are altered in PRIP-DKO mice. The deletion of PRIP-1/2 enhanced the desensitization of I-GABA but induced a hump-like tail current (tail-I) at the GABA puff offset. I-GABA and the hump-like tail-I were suppressed by GABA(A)R antagonists. The enhanced desensitization of I-GABA and the hump-like tail-I in PRIP-DKO PCs were mediated by increases in the intracellular Ca2+ concentration and were largely abolished by a calcineurin inhibitor and ruthenium red. Calcium imaging revealed that Ca2+-induced Ca2+ release (CICR) and subsequent store-operated Ca2+ entry (SOCE) are more potent in PRIP-DKO PCs than in wild-type PCs. A mathematical model revealed that a slowdown of GABA-unbinding rate and an acceleration of fast desensitization rate by enhancing its GABA concentration dependency are involved in the generation of hump-like tail-Is. These results suggest that in L3 PCs of the barrel cortex in PRIP-DKO mice, the increased calcineurin activity due to the potentiated CICR and SOCE enhances the desensitization of GABA(A)Rs and slows the GABA-unbinding rate, resulting in their unusual resensitization following removal of GABA.
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Key words
PRIP,GABA(A) receptor,Desensitization,Calcineurin,Ca2+-induced Ca2+ release,Store-operated Ca2+ entry
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