Prostate cancer is often treated by perturbing androgen receptor signalling. CACNA1D, encoding Ca V1.3 ion channels is upregulated in prostate cancer. Here we show how hormone therapy affects CACNA1D expression and Ca V1.3 function. Human prostate cells (LNCaP, VCaP, C4-2B, normal RWPE-1) and a tissue microarray were used. Cells were treated with anti-androgen drug, Enzalutamide (ENZ) or androgen-removal from media, mimicking androgen-deprivation therapy (ADT). Proliferation assays, qPCR, Western blot, immunofluorescence, Ca 2+-imaging and patch-clamp electrophysiology were performed. Nifedipine, Bay K 8644 (Ca V1.3 inhibitor, activator), mibefradil, Ni 2+ (Ca V3.2 inhibitors) and high K + depolarising solution were employed. CACNA1D and Ca V1.3 protein are overexpressed in prostate tumours and CACNA1D was overexpressed in androgen-sensitive prostate cancer cells. In LNCaP, ADT or ENZ increased CACNA1D time-dependently whereas total protein showed little change. Untreated LNCaP were unresponsive to depolarising high K +/Bay K (to activate Ca V1.3); moreover, currents were rarely detected. ADT or ENZ-treated LNCaP exhibited nifedipine-sensitive Ca 2+-transients; ADT-treated LNCaP exhibited mibefradil-sensitive or, occasionally, nifedipine-sensitive inward currents. CACNA1D knockdown reduced the subpopulation of treated-LNCaP with Ca V1.3 activity. VCaP displayed nifedipine-sensitive high K +/Bay K transients (responding subpopulation was increased by ENZ), and Ni 2+-sensitive currents. Hormone therapy enables depolarization/Bay K-evoked Ca 2+-transients and detection of Ca V1.3 and Ca V3.2 currents. Physiological and genomic CACNA1D/Ca V1.3 mechanisms are likely active during hormone therapy—their modulation may offer therapeutic advantage.