Anomalous regulation of the Drosophila Na+-Ca2+ exchanger by Ca2+

The Na+-Ca2+ exchanger from Drosophila was expressed in Xenopus oocytes and characterized electrophysiologically using the giant excised patch technique. This protein, termed Calx, shares 49% amino acid identity to the canine cardiac Na+-Ca2+ exchanger, NCX1. Calx exhibits properties similar to previously characterized Na+-Ca2+ exchangers including intracellular Na+ affinities, current-voltage relationships, and sensitivity to the peptide inhibitor, XIP. However, the Drosophila Na+-Ca2+ exchanger shows a completely opposite response to cytoplasmic Ca2+. Previously cloned Na+-Ca2+ exchangers (NCX1 and NCX2) are stimulated by cytoplasmic Ca2+ in the micromolar range (0.1-10 mu M) This stimulation of exchange current is mediated by occupancy of a regulatory Ca2+ binding site separate from the Ca2+ transport site. In contrast, Calx is inhibited by cytoplasmic Ca2+ over this same concentration range. The inhibition of exchange current is evident for both forward and reverse modes of transport The characteristics of the inhibition are consistent with the binding of Ca2+ at a regulatory site distinct from the transport site. These data provide a rational basis for subsequent structure-function studies targeting the intracellular Ca2+ regulatory mechanism.