(A and B) Confluent monolayers of GCaMP-transfected HAECs were exposed to laminar shear stress (20 dynes/cm²) for 48 hours before live cell imaging. (A) Representative GCaMP intensity trace showing Ca²⁺ activity at the downstream end after the addition of EGTA (1.6 μM) to chelate calcium ions in culture medium. (B) Representative GCaMP intensity trace showing Ca²⁺ activity at the downstream end after the addition of the TRPV4 antagonist GSK205 (20 μM). (C and D) HAECs were seeded on Y-shaped slides and exposed to unidirectional laminar flow for 48 hours. Immunofluorescence was compared for cells in low-flow (~5 dynes/cm²) and high-flow regions (~20 dynes/cm²). (C) TRPV4 protein staining showed no difference for low-flow versus high-flow regions. Representative images from n = 3 biological replicates; statistics calculated by 2-tailed, unpaired t test show no significance (NS) of difference between regions. Quantifying the subcellular distribution of expression indicated that TRPV4 was not polarized under flow. Shown are means ± SD from 44 low-flow and 57 high-flow cells across 4 biological replicates. Scale bars: 20 μm. (D) Representative images of proximity ligation assay (PLA) to detect TRPV4 and caveolin-1 association (magenta puncta) in low-flow and high-flow regions for n = 4 replicates. Shown are puncta per cell with means ± SD and statistics calculated using unpaired, 2-tailed t test. ***P < 0.001. Additional segmentation analysis showed that TRPV4/caveolin-1 PLA puncta preferentially occurred in the downstream end only for cells exposed to high flow. Thirty-eight cells were analyzed for the low-flow region and 93 cells for the high-flow region from n = 4 biological replicates. Data were analyzed by 1-way ANOVA and post hoc Tukey’s multiple-comparison test. *P < 0.05, ***P < 0.001. Scale bars: 10 μm.