| Abstract: | We usedsingle-channel recording techniques to identify and characterize alarge-conductance,Ca2+-independentK+ channel in the colonicsecretory cell line T84. In symmetric potassium gluconate, this channelhad a linear current-voltage relationship with a single-channelconductance of 161 pS. Channel open probability(Po) wasincreased at depolarizing potentials. Partial substitution of bathK+ withNa+ indicated a permeability ratioof K+ toNa+ of 25:1. ChannelPo was reduced byextracellular Ba2+. Event-durationanalysis suggested a linear kinetic model for channel gating having asingle open state and three closed states: C3  C2C1O.Arachidonic acid (AA) increased thePo of thechannel, with an apparent stimulatory constant(Ks)of 1.39 µM. Neither channel open time (O) nor the fast closed time(C1) was affected by AA. Incontrast, AA dramatically reduced mean closed time by decreasing bothC3 andC2. Thecis-unsaturated fatty acid linoleate increased Poalso, whereas the saturated fatty acid myristate and thetrans-unsaturated fatty acid elaidatedid not affectPo. This channelis activated also by negative pressure applied to the pipette duringinside-out recording. Thus we determined the effect of thestretch-activated channel blockers amiloride and Gd3+ on theK+ channel after activation by AA.Amiloride (2 mM) on the extracellular side reduced single-channelamplitude in a voltage-dependent manner, whereasGd3+ (100 µM) had no effect onchannel activity. Activation of this K+ channel may be important duringstimulation of Cl secretionby agonists that use AA as a second messenger (e.g., vasoactiveintestinal polypeptide, adenosine) or during the volume regulatoryresponse to cell swelling. |
