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牛离体气管平滑肌细胞中钾离子通道活性的膜片钳研究

A patch-clamp study of K(+)-channel activity in bovine isolated tracheal smooth muscle cells.

作者信息

Green K A, Foster R W, Small R C

机构信息

Department of Physiological Sciences, University of Manchester.

出版信息

Br J Pharmacol. 1991 Apr;102(4):871-8. doi: 10.1111/j.1476-5381.1991.tb12269.x.

Abstract
  1. Single smooth muscle cells were isolated from bovine trachealis by enzymic digestion. The properties of large conductance plasmalemmal K(+)-channels in these cells were studied by the patch-clamp recording technique. 2. Recordings were made from inside-out plasmalemmal patches when [K+] was symmetrically high (140 mM) and when [Ca2+] on the cytosolic side of the patch was varied from nominally zero to 10 microM. Large unitary currents of both Ca(2+)-dependent and -independent types were observed. Measured between + 20 and + 40 mV, the slope conductances of the channels carrying these currents were 249 +/- 18 pS and 268 +/- 14 pS respectively. 3. Lowering [K+] on the cytosolic side of the patches from 140 to 6 mM, shifted the reversal potentials of the two types of unitary current from approximately zero to much greater than + 40 mV, suggesting that both currents were carried by K(+)-channels. 4. The Ca(2+)-dependent and -independent K(+)-channels detected in inside-out plasmalemmal patches could also be distinguished on the basis of their sensitivity to inhibitors (tetraethylammonium (TEA), 1-10 mM; Cs+, 10 mM; Ba2+, 1-10 mM; quinidine, 100 microM) applied to the cytosolic surface of the patches. 5. Recordings were made from outside-out plasmalemmal patches when [K+] was symmetrically high (140 mM) and when [Ca2+] on the cytosolic side of the patch was varied from nominally zero to 1 microM. Ca(2+)-dependent unitary currents were observed and the slope conductance of the channel carrying these currents was 229 +/- 5 pS. 6. Activity of the Ca2+-dependent K+-channel detected in outside-out patches could be inhibited by application of TEA (1 mM), Cs+ (10mM), Ba2(+210mM) or quinidine (100 microM) to the external surface of the patch. 4-Aminopyridine (4-AP; 1 mM) was ineffective as an inhibitor. 7. The activity of the Ca2+-dependent K+-channel recorded from outside-out patches was reversibly inhibited by charybdotoxin (100 nM). 8. When whole-cell recording was performed, the application of a depolarizing voltage ramp evoked outward current which was dependent on the [Ca2 +] in the recording pipette and which could be reversibly inhibited by charybdotoxin (50 nM-I microM) applied to the external surface of the cell.9. We conclude that bovine trachealis cells are richly endowed with charybdotoxin-sensitive, large conductance, Ca2 +-dependent K+-channels. These channels carry most of the outward current evoked by a depolarizing ramp and could play a major role in determining the outward rectifying properties of the trachealis cells. The role of the large Ca2 + -independent K+ -channels remains unclear.
摘要
  1. 通过酶消化从牛气管中分离出单个平滑肌细胞。采用膜片钳记录技术研究了这些细胞中大电导质膜钾离子通道的特性。2. 当[K⁺]对称地高(140 mM)且膜片胞质侧的[Ca²⁺]从名义上的零变化到10 μM时,从内向外的质膜片进行记录。观察到了钙依赖性和非依赖性两种类型的大的单通道电流。在+20至+40 mV之间测量,携带这些电流的通道的斜率电导分别为249±18 pS和268±14 pS。3. 将膜片胞质侧的[K⁺]从140 mM降低到6 mM,使两种类型的单通道电流的反转电位从大约零转移到远大于+40 mV,表明两种电流均由钾离子通道携带。4. 在内向外质膜片中检测到的钙依赖性和非依赖性钾离子通道也可以根据它们对应用于膜片胞质表面的抑制剂(四乙铵(TEA),1 - 10 mM;Cs⁺,10 mM;Ba²⁺,1 - 10 mM;奎尼丁,100 μM)的敏感性来区分。5. 当[K⁺]对称地高(140 mM)且膜片胞质侧的[Ca²⁺]从名义上的零变化到1 μM时,从外向内质膜片进行记录。观察到了钙依赖性单通道电流,携带这些电流的通道的斜率电导为229±5 pS。6. 应用于膜片外表面的TEA(1 mM)、Cs⁺(10 mM)、Ba²⁺(10 mM)或奎尼丁(100 μM)可抑制在向外质膜片中检测到的钙依赖性钾离子通道的活性。4 - 氨基吡啶(4 - AP;1 mM)作为抑制剂无效。7. 从外向内质膜片记录的钙依赖性钾离子通道的活性被蝎毒素(100 nM)可逆性抑制。8. 当进行全细胞记录时,施加去极化电压斜坡会诱发外向电流,该电流取决于记录电极中的[Ca²⁺],并且可被应用于细胞外表面的蝎毒素(50 nM - 1 μM)可逆性抑制。9. 我们得出结论,牛气管细胞富含对蝎毒素敏感的、大电导的、钙依赖性钾离子通道。这些通道携带去极化斜坡诱发的大部分外向电流,并且可能在决定气管细胞的外向整流特性中起主要作用。大的钙非依赖性钾离子通道的作用仍不清楚。

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