Biochemical properties of the sensitivity to GABAAergic ligands, Cl-/HCO3--ATPase isolated from fish (Cyprinus carpio) olfactory mucosa and brain.

Abstract

This paper presents a comparative study of the roles of Cl- and HCO3- in the functioning of the GABAAR-associated Cl-/HCO3--ATPase of the plasma membranes of the olfactory sensory neurons (OSNs) and mature brain neurons (MBNs) of fish. The ATPase activity of OSNs and its dephosphorylation were increased twofold by Cl-(15-30mmoll-1), whereas the enzyme from MBNs was not significantly affected by Cl-. By contrast, HCO3-(15-30mmoll-1) significantly activated the MBN enzyme and its dephosphorylation, but had no effect on the OSN ATPase. The maximum ATPase activity and protein dephosphorylation was observed in the presence of both Cl-(15mmoll-1)/HCO3-(27mmoll-1) and these activities were inhibited in the presence of picrotoxin (100μmoll-1), bumetanide (150μmoll-1), and DIDS (1000μmoll-1). SDS-PAGE revealed that ATPases purified from the neuronal membrane have a subunit with molecular mass of ~ 56kDa that binds [3H]muscimol and [3H]flunitrazepam. Direct phosphorylation of the enzymes in the presence of ATP-γ-32P and Mg2+, as well as Cl-/HCO3- sensitive dephosphorylation, is also associated with this 56kDa peptide. Both preparations also showed one subunit with molecular mass 56kDa that was immunoreactive with GABAAR β3 subunit. The use of a fluorescent dye for Cl- demonstrated that HCO3-(27mmoll-1) causes a twofold increase in Cl- influx into proteoliposomes containing reconstituted ATPases from MBNs, but HCO3- had no effect on the reconstituted enzyme from OSNs. These data are the first to demonstrate a differential effect of Cl- and HCO3- in the regulation of the Cl-/HCO3--ATPases functioning in neurons with different specializations.