A single amino acid change in Ca_V1.2 channels eliminates the permeation and gating differences between Ca²⁺ and Ba²⁺

Glutamate scanning mutagenesis was used to assess the role of the calcicludine binding segment in regulating channel permeation and gating using both Ca²⁺ and Ba²⁺ as charge carriers. As expected, wild-type Ca_V1.2 channels had a Ba²⁺ conductance ~2× that in Ca²⁺ (G_Ba/G_Ca = 2) and activation was ~10 mV more positive in Ca²⁺ vs. Ba²⁺. Of the 11 mutants tested, F1126E was the only one that showed unique permeation and gating properties compared to the wild type. F1126E equalized the Ca_V1.2 channel conductance (G_Ba/G_Ca = 1) and activation voltage dependence between Ca²⁺ and Ba²⁺. Ba²⁺ permeation was reduced because the interactions among multiple Ba²⁺ ions and the pore were specifically altered for F1126E, which resulted in Ca²⁺-like ionic conductance and unitary current. However, the high-affinity block of monovalent cation flux was not altered for either Ca ²⁺ or Ba²⁺. The half-activation voltage of F1126E in Ba²⁺ was depolarized to match that in Ca²⁺, which was unchanged from that in the wild type. As a result, the voltages for half-activation and half-inactivation of F1126E in Ba²⁺ and Ca ²⁺ were similar to those of wild-type in Ca²⁺. This effect was specific to F1126E since F1126A did not affect the half-activation voltage in either Ca²⁺ or Ba²⁺. These results indicate that residues in the outer vestibule of the Ca_V1.2 channel pore are major determinants of channel gating, selectivity, and permeation.