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胰腺腺泡细胞:钙在刺激-分泌偶联中的作用。

Pancreatic acinar cells: the role of calcium in stimulus-secretion coupling.

作者信息

Petersen O H, Ueda N

出版信息

J Physiol. 1976 Jan;254(3):583-606. doi: 10.1113/jphysiol.1976.sp011248.

Abstract
  1. Segments of mouse or rat pancreas were placed in a flow cell through which physiological salt solutions of varying composition were pumped at a constant rate. Intracellular recordings of membrane potential, resistance and electrical time constant were made from the acini using fine glass micro-electrodes. In some experiments two micro-electrodes were inserted into two acinar cells within the same acinus to assess directly cell to cell coupling. The concentration of amylase in the effluent was measured continuously. 2. Electrical coupling between two acinar cells was observed when the tips of the two micro-electrodes were less than 50 mum from each other. The coupling ratio was close to 1. Acetylcholine (ACh) always evoked depolarization of exactly the same amplitude in two coupled cells and reduced the amplitude of current-pulse induced membrane potential changes in both cell simultaneously. 3. Stimulation with ACh caused an immediate increase in amylase output. Replacement of superfusion fluid Na by Tris or Cl by sulphate abolished ACh-evoked increase in amylase release, but the subsequent reintroduction of Na or Cl caused an increase in amylase release of a magnitude similar to what was normally observed following stimulation. 4. Omitting Ca from the superfusion fluid and adding EGTA rapidly depolarized the acinar cell membrane, reduced the input resistance and caused a marked reduction in amylase secretion. During exposure to a Ca-free, EGTA containing solution a marked increase in amylase release occurred following maximal ACh stimulation. 5. Addition of small amounts of Mg, Ca or Mn to a Ca-, Mg-free solution caused an increase in membrane potential, input resistance and electrical time constant and markedly increased amylase release. The effect on the electrical parameters was reversed in the absence of extracellular Na while extracellular Na was of no importance for the effect on amylase release. 6. The effect of ACh on amylase was enhanced during superfusion with a fluid containing 20 mM-Ca. The presence of Mn (5 mM) in an otherwise normal control had no effect on ACh-evoked release. 7. These results show that ACh acts on the acinus by reducing the surface cell membrane resistance. It is suggested that the ACh-receptor interaction causes a release of Ca from the surface cell membrane and that the concentration of Ca in the surface cell membrane determines the specific membrane resistance particularly for Na. The release of Ca to the cytosol activates exocytosis while the Na influx is of importance for acinar fluid secretion. The effect of ACh on amylase secretion can be mimicked by agents displacing membrane-bound Ca (Mg, Ca, Mn).
摘要
  1. 将小鼠或大鼠的胰腺组织块置于流动小室中,以恒定速率泵入不同成分的生理盐溶液。使用精细玻璃微电极对腺泡进行膜电位、电阻和电时间常数的细胞内记录。在一些实验中,将两个微电极插入同一腺泡内的两个腺泡细胞中,以直接评估细胞间的耦合。连续测量流出液中淀粉酶的浓度。2. 当两个微电极尖端彼此距离小于50微米时,观察到两个腺泡细胞之间存在电耦合。耦合比率接近1。乙酰胆碱(ACh)总是在两个耦合细胞中引起完全相同幅度的去极化,并同时降低两个细胞中电流脉冲诱导的膜电位变化幅度。3. 用ACh刺激导致淀粉酶输出立即增加。用Tris替代灌流液中的Na或用硫酸盐替代Cl可消除ACh引起的淀粉酶释放增加,但随后重新引入Na或Cl会导致淀粉酶释放增加,其幅度与刺激后通常观察到的相似。4. 从灌流液中省略Ca并添加EGTA会使腺泡细胞膜迅速去极化,降低输入电阻,并导致淀粉酶分泌显著减少。在暴露于不含Ca、含有EGTA的溶液期间,最大ACh刺激后淀粉酶释放显著增加。5. 向不含Ca、Mg的溶液中添加少量Mg、Ca或Mn会导致膜电位、输入电阻和电时间常数增加,并显著增加淀粉酶释放。在没有细胞外Na的情况下,对电参数的影响会逆转,而细胞外Na对淀粉酶释放的影响并不重要。6. 在含有20 mM - Ca的溶液灌流期间,ACh对淀粉酶的作用增强。在其他方面正常的对照中存在Mn(5 mM)对ACh诱导的释放没有影响。7. 这些结果表明,ACh通过降低表面细胞膜电阻作用于腺泡。有人提出,ACh - 受体相互作用导致从表面细胞膜释放Ca,并且表面细胞膜中Ca的浓度决定了特定的膜电阻,特别是对于Na。Ca释放到细胞质中激活胞吐作用,而Na内流对腺泡液分泌很重要。ACh对淀粉酶分泌的作用可以被置换膜结合Ca的试剂(Mg、Ca、Mn)模拟。

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