(A) Left: Images of a voltage-clamped primary cilia in the on-cilia configuration. Primary cilium of PKD1^null:PKD2^null HEK293 cells expressing PKD2 channels are illuminated by ARL13B-GFP under 475 nm laser excitation. Scale bar: 12 μm. (B) Example single-channel recordings from cilia membranes activated by depolarizing voltage steps. Note, no open-channel events were observed in cilia patch recordings from cells expressing R654X channels. (C) Unitary conductance was estimated from the slope (γ) of a linear fit of the single-channel current magnitudes. (D) Open probability (Po)–voltage relationships were fit to a Boltzmann equation to estimate half-activation voltage (V_1/2). (E) Left: Images of a voltage-clamped primary cilia membrane in the inside-out configuration. Note that the cilium is separated from the cell body, exposing the inner side of the membrane where internal calcium concentration ([Ca²⁺]_in) was modulated through bath conditions, as previously described (46). (F) Exemplar continuous inside-out PKD2 single-channel recording where initial stimulatory calcium-dependent modulation (CDM) and subsequent desensitization (CDM) effects are initiated by increasing [Ca²⁺]_in from 100 nM to 30 μM. Note: Fewer simultaneous channel openings are stimulated from R803X cilia membrane patch (2 channels, O₂) compared with WT PKD2 (6 channels, O₆). Scale bar: 5 μm. (G) CDM of WT and R803X single channels as demonstrated by robust shifts in the V_1/2. (H) Violin plots of the maximum number of simultaneous open-channel events before and after calcium stimulation. The number of cilia records for each data set is indicated within the parenthesis. P values indicate results from 2-tailed, unpaired Student’s t tests comparing WT and variant channel data sets.