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토끼 단일 심근세포에서 대사억제시 Inward Rectifier(IK1)의 변화 Effect of Metabolic Inhibition on Inward Rectifier K Current in Single Rabbit Ventricular Myocytes
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  • 토끼 단일 심근세포에서 대사억제시 Inward Rectifier(IK1)의 변화 Effect of Metabolic Inhibition on Inward Rectifier K Current in Single Rabbit Ventricular Myocytes
저자명
정유정,호원경,엄융의,YuJeongChung,Won-KyungHo,YungEEarm
간행물명
The Korean Journal of Physiology & PharmacologyKCI,SCI,SCOPUS
권/호정보
1997년|1권 6호(통권6호)|pp.741-748 (8 pages)
발행정보
대한생리학회-대한약리학회|한국
파일정보
정기간행물|KOR|
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국문초록

In the present study, we have investigated the effect of metabolic inhibition on the inward rectifier K current (IK1). Using whole cell patch clamp technique we applied voltage ramp from ⁢80 mV to ⁣140 mV at a holding potential of ⁣30 mV and recorded the whole cell current in single ventricular myocytes isolated from the rabbit heart. The current-voltage relationship showed N-shape (a large inward current and little outward current with a negative slope) which is a characteristic of IK1. Application of 0.2 mM dinitrophenol (DNP, an uncoupler of oxidative phosphorylation as a tool for chemical hypoxia) to the bathing solution with the pipette solution containing 5 mM ATP, produced a gradual increase of outward current followed by a gradual decrease of inward current with little change in the reversal potential (⁣80 mV). The increase of outward current was reversed by glibenclamide (10 ㄍM), suggesting that it is caused by the activation of KATP. When DNP and glibenclamide were applied at the same time or glibenclamide was pretreated, DNP produced same degree of reduction in the magnitude of the inward current. These results show that metabolic inhibition induces not only the increase of KATP channel but also the decrease of IK1. Perfusing the cell with ATP-free pipette solution induced the changes very similar to those observed using DNP. Long exposure of DNP (30 min) or ATP-free pipette solution produced a marked decrease of both inward and outward current with a significant change in the reversal potential. Above results suggest that the decrease of IK1 may contribute to the depolarisation of membrane potential during metabolic inhibition.

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