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环磷酸腺苷对大鼠促黑素细胞中单一胞吐事件幅度的调节作用。

Modulation of the unitary exocytic event amplitude by cAMP in rat melanotrophs.

作者信息

Sikdar S K, Kreft M, Zorec R

机构信息

Molecular Biophysics Unit, Indian Institute of Science, Bangalore-560012, India.

出版信息

J Physiol. 1998 Sep 15;511 ( Pt 3)(Pt 3):851-9. doi: 10.1111/j.1469-7793.1998.851bg.x.

Abstract
  1. Secretory responses were measured in single rat pituitary melanotrophs as the relative increase in membrane capacitance (Cm) 8 min after the start of dialysis with solutions containing 0.45 microM Ca2+. In the added presence of cAMP (0.2 mM) in the patch pipette solution, capacitance responses increased 2- to 3-fold in comparison with controls. 2. To study whether cAMP-dependent mechanisms affect cytosolic calcium activity ([Ca2+]i), dibutyryl cyclic AMP (dbcAMP, 10 mM) was added to intact melanotrophs and [Ca2+]i was measured using fura-2 AM. Addition of dbcAMP caused a transient reduction in [Ca2+]i to 82 +/- 21 nM from a resting value of 100 +/- 19 nM (mean +/- S.E.M., n = 32, P < 0.002), indicating that the cAMP-induced increase in secretory activity was not the result of cAMP acting to increase [Ca2+]i, which then increased secretory activity. 3. To investigate whether cAMP affects the secretory apparatus directly, the interaction of a single secretory granule with the plasmalemma was monitored by measuring discrete femtofarad steps in Cm. The signal-to-noise ratio of recordings was increased by pre-incubating the cells with a hydrophobic anion, dipicrylamine. 4. Recordings of unitary exocytic events (discrete 'on' steps in Cm) showed that the amplitude of 'on' steps - a parameter correlated to the size of exocytosing secretory granules - increased from 4.2 +/- 0.2 fF (n = 356) in controls to 7.9 +/- 0.2 fF in the presence of cAMP (n = 329, P < 0.001), while the frequency of unitary exocytic events was similar in controls and in the presence of cAMP. 5. The results suggest that a cAMP-dependent mechanism mediates the fusion of larger granules with the plasmalemma.
摘要
  1. 在单个大鼠垂体黑素细胞中测量分泌反应,方法是在用含0.45微摩尔Ca2+的溶液开始透析8分钟后,测量膜电容(Cm)的相对增加。在膜片钳溶液中添加cAMP(0.2毫摩尔)后,与对照组相比,电容反应增加了2至3倍。2. 为了研究cAMP依赖性机制是否影响胞质钙活性([Ca2+]i),将二丁酰环磷腺苷(dbcAMP,10毫摩尔)添加到完整的黑素细胞中,并用fura-2 AM测量[Ca2+]i。添加dbcAMP导致[Ca2+]i从静息值100±19纳摩尔瞬时降至82±21纳摩尔(平均值±标准误,n = 32,P < 0.002),这表明cAMP诱导的分泌活性增加不是cAMP作用增加[Ca2+]i然后增加分泌活性的结果。3. 为了研究cAMP是否直接影响分泌装置,通过测量Cm中离散的飞法拉步骤来监测单个分泌颗粒与质膜的相互作用。通过用疏水性阴离子苦味胺预孵育细胞来提高记录的信噪比。4. 单细胞胞吐事件(Cm中的离散“开启”步骤)的记录显示,“开启”步骤的幅度——一个与胞吐分泌颗粒大小相关的参数——从对照组的4.2±0.2飞法拉(n = 356)增加到cAMP存在时的7.9±0.2飞法拉(n = 329,P < 0.001),而单细胞胞吐事件的频率在对照组和cAMP存在时相似。5. 结果表明,一种cAMP依赖性机制介导了较大颗粒与质膜的融合。

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