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牛蛙心房肌细胞中两种不同类型的内向整流钾通道。

Two distinct types of inwardly rectifying K+ channels in bull-frog atrial myocytes.

作者信息

Clark R B, Nakajima T, Giles W, Kanai K, Momose Y, Szabo G

机构信息

Department of Medical Physiology, University of Calgary, Alberta, Canada.

出版信息

J Physiol. 1990 May;424:229-51. doi: 10.1113/jphysiol.1990.sp018064.

Abstract
  1. Single atrial myocytes were enzymatically isolated from the bull-frog as previously described (Hume & Giles, 1981), and patch-clamp techniques were used in an attempt to identify and separate two inwardly rectifying K+ channels in this tissue. 2. Single-channel measurements consistently demonstrated the existence of two different resting K+ channels, which both exhibited strong inward rectification. The unitary conductances of these K+ channels were 34 +/- 4 and 22 +/- 3 pS (mean +/- S.D., at 22-24 degrees C) when measured with 110 mM-K+ in the pipette solution, and their mean open times were 0.87 +/- 0.33 and 129.9 +/- 49.4 ms, respectively. 3. In the absence of acetylcholine (ACh) in the pipette, openings of the larger channels with the shorter open times occurred at a very low frequency. When ACh was present in the patch pipette, the activity of this channel increased significantly, although the single-channel conductance and gating behaviour were very similar either with or without ACh in the pipette. 4. The zero-current voltage (extrapolated from the inward currents through these types of channels) depended on the extracellular K+ concentration. [K+]o, in the fashion expected for a predominantly K(+)-selective channel: it shifted by 58 mV for a tenfold change in [K+]o. Very similar results were obtained from whole-cell voltage-clamp measurements (53 mV for a tenfold change in [K+]o). 5. The conductance of both types of K+ channels depended on [K+]o. The single-channel conductances were 25 +/- 3 and 13 +/- 2 pS with 50 mM [K+]o, and 19 +/- 4 and 9 +/- 2 pS with 20 mM [K+]o, respectively. 6. These results demonstrate that two types of resting inwardly rectifying K+ channels can be identified in single atrial myocytes. One of these is an inwardly rectifying K+ channel (IK1) previously identified in whole-cell voltage-clamp experiments (Hume & Giles, 1983). The second channel is the muscarinic receptor-regulated K+ channel (IK(ACh) which was first described in mammalian nodal and atrial cells. 7. N-Ethylmaleimide (NEM), a reagent which alkylates sulphydryl groups, affects these two types of K+ channels differentially. In the cell-attached patch configuration, bath application of NEM (50 microM) completely abolished the activity of IK(ACh), without affecting the IK1 channel activity. 8. To obtain further evidence that these two currents, IK1 and IK(ACh), were different, the inside-out patch-clamp technique was used.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 如先前所述(休姆和贾尔斯,1981年),采用酶解法从牛蛙中分离出单个心房肌细胞,并运用膜片钳技术试图识别和分离该组织中的两种内向整流钾通道。2. 单通道测量结果始终表明存在两种不同的静息钾通道,二者均表现出强烈的内向整流特性。当移液管溶液中钾离子浓度为110 mM时,这些钾通道的单位电导分别为34±4和22±3 pS(平均值±标准差,22 - 24℃),其平均开放时间分别为0.87±0.33和129.9±49.4毫秒。3. 在移液管中不存在乙酰胆碱(ACh)时,开放时间较短的较大通道的开放频率非常低。当移液管中有ACh时,尽管移液管中有无ACh时单通道电导和门控行为非常相似,但该通道的活性显著增加。4. 零电流电压(通过这类通道的内向电流外推得出)取决于细胞外钾离子浓度。[K⁺]ₒ,对于主要为钾离子选择性的通道而言符合预期:[K⁺]ₒ每变化10倍,其偏移58 mV。全细胞电压钳测量也得到了非常相似的结果([K⁺]ₒ每变化10倍偏移53 mV)。5. 两种类型的钾通道电导均取决于[K⁺]ₒ。当[K⁺]ₒ为50 mM时,单通道电导分别为25±3和13±2 pS;当[K⁺]ₒ为20 mM时,分别为19±4和9±2 pS。6. 这些结果表明,在单个心房肌细胞中可识别出两种类型的静息内向整流钾通道。其中一种是先前在全细胞电压钳实验中已识别出的内向整流钾通道(IK1)(休姆和贾尔斯,1983年)。第二种通道是毒蕈碱受体调节的钾通道(IK(ACh)),该通道最早在哺乳动物的结区和心房细胞中被描述。7. N - 乙基马来酰亚胺(NEM),一种使巯基烷基化的试剂,对这两种类型的钾通道有不同影响。在细胞贴附式膜片钳配置中,将NEM(50 microM)应用于浴液可完全消除IK(ACh)的活性,而不影响IK1通道活性。8. 为了进一步证明这两种电流,即IK1和IK(ACh),是不同的,采用了内面向外膜片钳技术。(摘要截取自400字)

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