A voltage-dependent K+ current contributes to membrane potential of acutely isolated canine articular chondrocytes

The electrophysiological properties of acutely isolated canine articular chondrocytes have been characterized using patch-clamp methods. The ‘steady-state’ current–voltage relationship ( I–V ) of single chondrocytes over the range of potentials from −100 to +40 mV was highly non-linear, sh...

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Veröffentlicht in:The Journal of physiology 2004-05, Vol.557 (1), p.93-104
Hauptverfasser: Wilson, Jim R., Duncan, Neil A., Giles, Wayne R., Clark, Robert B.
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Sprache:eng
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Zusammenfassung:The electrophysiological properties of acutely isolated canine articular chondrocytes have been characterized using patch-clamp methods. The ‘steady-state’ current–voltage relationship ( I–V ) of single chondrocytes over the range of potentials from −100 to +40 mV was highly non-linear, showing strong outward rectification positive to the zero-current potential. Currents activated at membrane potentials negative to −50 mV were time independent, and the I–V from −100 to −60 mV was linear, corresponding to an apparent input resistance of 9.3 ± 1.4 GΩ ( n = 23). The outwardly rectifying current was sensitive to the K + channel blocking ion tetraethylammonium (TEA), which had a 50% blocking concentration of 0.66 m m (at +50 mV). The ‘TEA-sensitive’ component of the outwardly rectifying current had time- and membrane potential-dependent properties, activated near −45 mV and was half-activated at −25 mV. The reversal potential of the ‘TEA-sensitive’ current with external K + concentration of 5 m m and internal concentration of 145 m m , was −84 mV, indicating that the current was primarily carried by K + ions. The resting membrane potential of isolated chondrocytes (−38.1 ± 1.4 mV; n = 19) was depolarized by 14.8 ± 0.9 mV by 25 m m TEA, which completely blocked the K + current of these cells. These data suggest that this voltage-sensitive K + channel has an important role in regulating the membrane potential of canine articular chondrocytes.
ISSN:0022-3751
1469-7793
DOI:10.1113/jphysiol.2003.058883