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犬结肠间质细胞和平滑肌细胞离子电流的比较。

Comparison of ionic currents from interstitial cells and smooth muscle cells of canine colon.

作者信息

Lee H K, Sanders K M

机构信息

Department of Physiology, University of Nevada School of Medicine, Reno 89557.

出版信息

J Physiol. 1993 Jan;460:135-52. doi: 10.1113/jphysiol.1993.sp019463.

Abstract
  1. Voltage-dependent ionic currents of isolated interstitial cells were characterized using the whole-cell voltage clamp technique, and compared with currents recorded from circular muscle cells. Both cell types were isolated from the submucosal pacemaking region in the canine distal colon. 2. Upon depolarization, interstitial cells and smooth muscle cells generated transient inward, followed by slowly inactivating outward, currents. 3. After blocking inward current and much of the Ca(2+)-dependent outward current, interstitial cells displayed voltage-dependent outward current that rapidly activated, reached a peak, and then inactivated. This current was resistant to 4-aminopyridine(4-AP; 1 mM). Smooth muscle cells expressed a similar current but it was reduced by about 40% at a test potential of +20 mV by 4-AP (1 mM). 4. The inactivation characteristics of the voltage-dependent outward currents of interstitial cells and smooth muscle cells were compared. The outward current of interstitial cells inactivated at more negative potentials; half-inactivation occurred at -53 mV, whereas half-inactivation occurred at -20 mV in smooth muscle cells. 5. Inward currents were not strikingly different in the two cell types when dialysing pipettes were used. When the perforated patch technique (using Amphotericin-B) was used, a negatively activating inward current was observed in interstitial cells that had a resolution threshold of -70 to -60 mV. This current peaked at -10 mV. Inward currents in smooth muscle cells were resolved at test potentials positive to -50 mV and peaked at 0 to +10 mV. 6. When interstitial cells were held at -40 mV, inward current could not be resolved with test depolarization negative to -30 mV. From this holding potential, peak amplitude was reduced by 85% with test depolarizations to -10 mV. Holding smooth muscle cells at -40 mV also reduced inward current, but the peak current in these cells was reduced by only 39% at 0 mV. 7. Ni2+ partially inhibited peak inward current in interstitial cells and abolished a 'hump' in the I-V curve that occurred at negative potentials. In dialysed cells where this 'hump' was not apparent, addition of nifedipine unmasked a 'hump'. The presence of both nifedipine and Ni2+ abolished inward current. 8. A portion of the inward current in smooth muscle cells was sustained and persisted for the duration of test pulses. Very little sustained inward current was observed in interstitial cells. 9. The time course of inactivation of inward current in interstitial cells was fitted with two exponentials.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 采用全细胞膜片钳技术对分离出的间质细胞的电压依赖性离子电流进行了特性分析,并与从环形肌细胞记录到的电流进行了比较。这两种细胞类型均从犬远端结肠的黏膜下起搏区域分离得到。2. 去极化时,间质细胞和平滑肌细胞产生短暂的内向电流,随后是缓慢失活的外向电流。3. 在阻断内向电流和大部分钙依赖性外向电流后,间质细胞呈现出电压依赖性外向电流,该电流迅速激活、达到峰值,然后失活。这种电流对4-氨基吡啶(4-AP;1 mM)具有抗性。平滑肌细胞表达类似的电流,但在+20 mV的测试电位下,1 mM的4-AP使其降低了约40%。4. 比较了间质细胞和平滑肌细胞电压依赖性外向电流的失活特性。间质细胞的外向电流在更负的电位下失活;半失活发生在-53 mV,而平滑肌细胞的半失活发生在-20 mV。5. 使用透析微电极时,两种细胞类型的内向电流没有显著差异。当使用穿孔膜片钳技术(使用两性霉素B)时,在间质细胞中观察到一种负向激活的内向电流,其分辨阈值为-70至-60 mV。该电流在-10 mV时达到峰值。平滑肌细胞中的内向电流在测试电位高于-50 mV时可分辨,在0至+10 mV时达到峰值。6. 当间质细胞保持在-40 mV时,测试去极化至-30 mV以下时无法分辨出内向电流。从这个保持电位开始,测试去极化至-10 mV时,峰值幅度降低了85%。将平滑肌细胞保持在-40 mV也会降低内向电流,但这些细胞在0 mV时的峰值电流仅降低了39%。7. Ni2+部分抑制间质细胞的内向电流峰值,并消除了I-V曲线在负电位处出现的一个“驼峰”。在透析细胞中,当这个“驼峰”不明显时,加入硝苯地平会揭示出一个“驼峰”。硝苯地平和Ni2+同时存在时会消除内向电流。8. 平滑肌细胞中的一部分内向电流持续存在,并在测试脉冲期间持续。在间质细胞中观察到的持续内向电流很少。9. 间质细胞内向电流的失活时间过程用两个指数函数拟合。(摘要截短至400字)

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