Inositol 1,4,5-trisphosphate (1,4,5-InsP₃) was perfused into rat dorsal root ganglion (DRG) neurons by whole-cell patch-clamp electrodes, while measuring the membrane potential. This operation evoked a transient (2–3 min) membrane hyperpolarization of about −15 mV (from −42 mV) followed by a depolarization. The membrane hyperpolarization was abolished when 30 mM EGTA was perfused together with 1,4,5-InsP₃ or when 0.2 mM quinine was added to the bath solution. The hyperpolarizing response was enhanced when a low-Ca²⁺ EGTA-free intracellular solution was used. Two InsP₂ isomers induced a different response. Our results suggest that the hyperpolarization is due to 1,4,5-InsP_3-induced Ca²⁺ release which may trigger Ca-sensitive K⁺ channels to open. Present results show that cultured DRG neurons are able to respond to 1,4,5-InsP₃ perfusion in the whole-cell configuration.