Characteristics of transient outward currents in single smooth muscle cells from the ureter of the guinea‐pig.
- 1 August 1990
- journal article
- research article
- Published by Wiley in The Journal of Physiology
- Vol. 427 (1) , 301-324
- https://doi.org/10.1113/jphysiol.1990.sp018173
Abstract
1. Two kinds of transient outward currents were observed upon depolarization of single smooth muscle cells isolated from guinea-pig ureter. The major transient outward current was through Ca2+-activated K+ channels (IK(Ca)) which had a large conductance (130 pS; 126 mM [K]i/5.9 mM [K+]o). 2. The smaller transient outward current (ITO) was pharmacologically separated from other membrane currents in the presence of 1 mM-Cd2+ and 2 mM-tetraethylammonium(TEA+) and was selectively blocked by 3 mM-4-aminopyridine. It peaked (approximately 200 pA) wihtin 10 ms upon depolarization from -80 to +20 mV and its half-inactivation time was approximately 50 ms at +20 mV. Half-maximum voltages (V1/2 for activation and inactivation were about -8 and -50 mV, respectively, in the presence of 1 mM-Cd2+ and 2 mM-TEA+. The time course of recovery from inactivation of ITO was fitted with a single-exponential function (.tau. = 100 ms at -80 mV). A tenfold change of [K+]o resulted in a 53 mV change in the reversal potential of the tail of ITO. 3. Cadmium reduced peak ITO and shifted the voltage dependence of activation and inactivation in the positive direction in a concentration-dependent manner. The V1/2 for inactivation in the absence of Cd2+ was estimated to be approximately -64 mV. 4. Single-channel outward currents which appeared only in the initial part of a depolarizing pulse from about -100 mV were recorded using the cell-attached patch clamp. The decay of the ensemble average of the current was similar to the macroscopic ITO under whole-cell clamp. When the holding potential was less negative, the opening probability of the channel greatly decreased. The channel conductance in normal extracellular medium was 14 pS. 5. In ureter cells ITO resembles A-type current. ITO does not contribute significantly to the repolarization of the action potential but it may regulate membrane excitability by opposing Ca2+ current activated around the threshold of the action potential.This publication has 55 references indexed in Scilit:
- Membrane currents that govern smooth muscle contraction in a ctenophoreNature, 1988
- Sodium current in single cells from bullfrog atrium: voltage dependence and ion transfer properties.The Journal of Physiology, 1987
- Quinidine-induced inhibition of transient outward current in cardiac muscleAmerican Journal of Physiology-Heart and Circulatory Physiology, 1987
- Features of 4-aminopyridine sensitive outward current observed in single smooth muscle cells from the rabbit pulmonary arteryPflügers Archiv - European Journal of Physiology, 1987
- Selectivity and patch measurements of A‐current channels in Helix aspersa neurones.The Journal of Physiology, 1987
- Single-Channel and Genetic Analyses Reveal Two Distinct A-Type Potassium Channels in DrosophilaScience, 1987
- Inactivating and non-inactivating outward current channels in cell-attached patches ofHelix neuronsBrain Research, 1987
- Characterization of calcium-activated potassium channels in single smooth muscle cells using the patch-clamp techniquePflügers Archiv - European Journal of Physiology, 1987
- Identification and characterization of major ionic currents in isolated smooth muscle cells using the voltage-clamp techniquePflügers Archiv - European Journal of Physiology, 1987
- Mechanism of increased amplitude and duration of the plateau with sudden shortening of diastolic intervals in rabbit ventricular cells.Circulation Research, 1987