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离子和第二信使对鸟类睫状神经节化学传递长时程增强的影响。

The effect of ions and second messengers on long-term potentiation of chemical transmission in avian ciliary ganglia.

作者信息

Scott T R, Bennett M R

机构信息

Department of Physiology, University of Sydney, N.S.W., Australia.

出版信息

Br J Pharmacol. 1993 Sep;110(1):461-9. doi: 10.1111/j.1476-5381.1993.tb13833.x.

Abstract
  1. The effects of tetanic stimulation of the oculomotor nerve on transmission through the avian ciliary ganglion have been determined by use of the amplitude of the compound action potential recorded in the ciliary nerve, in the presence of hexamethonium (300 microM), as a measure of synaptic efficacy. 2. Tetanic stimulation for 20 s at 30 Hz potentiated the chemical phase of the compound action potential by at least 100% of its control level. This potentiation, reflecting an increase in synaptic efficacy, decayed over two distinct time courses: firstly, a rapid decay with a time constant in the order of minutes, and secondly, a slower decay, representing a smaller potentiation, with a time constant in the order of an hour. The large increase in synaptic efficacy is attributed to post-tetanic potentiation (PTP) whereas the smaller but longer lasting increase is attributed to long-term potentiation (LTP). 3. Higher frequencies of tetanic stimulation gave increased PTP and LTP. 4. In order to test whether the influx of calcium ions into the nerve terminal during the tetanus is likely to be involved in potentiation, facilitation was measured during PTP and LTP. Facilitation was reduced to approximately zero during PTP but recovered to normal values about 15 min into LTP. A requirement for the induction of LTP was shown to be the presence of calcium in the bathing solution. However, blocking synaptic transmission with a high concentration of hexamethonium (3 mM) during the tetanic stimulation did not block the induction of LTP. 5. Application of the muscarinic inhibitor, atropine (2 microM), did not affect the magnitude of PTP or LTP. 5. Application of the muscarinic inhibitor, atropine (2 tM), did not affect the magnitude of PTP or LTP.6. The activator of protein kinase C, phorbol 12,13-dibutyrate (2 microM) potentiated synaptic transmission and reduced the potentiation due to PTP although it did not affect that due to LTP, but the inhibitor of this kinase, staurosporine (0.5 microM), partially blocked the appearance of LTP without affecting PTP after the tetanus.7. An inhibitor of calmodulin, W-7 (5 microM), reversibly blocked the appearance of LTP significantly after a tetanus although the size of PTP was not affected.8. The results presented here suggest that the initiation of LTP in the ciliary ganglion is due to an influx of calcium ions into the calyciform nerve terminal during the tetanus and that the mechanism for LTP involves a calcium-calmodulin-dependent process.
摘要
  1. 通过在六甲铵(300微摩尔)存在的情况下,使用睫状神经中记录的复合动作电位的幅度,来确定动眼神经强直刺激对通过禽睫状神经节传递的影响,以此作为突触效能的一种度量。2. 以30赫兹进行20秒的强直刺激使复合动作电位的化学相增强至其对照水平的至少100%。这种增强反映了突触效能的增加,其衰减过程分为两个不同的时间进程:首先,快速衰减,时间常数约为几分钟;其次,较慢的衰减,代表较小的增强,时间常数约为一小时。突触效能的大幅增加归因于强直后增强(PTP),而较小但持续时间更长的增加归因于长期增强(LTP)。3. 更高频率的强直刺激会使PTP和LTP增加。4. 为了测试强直期间钙离子流入神经末梢是否可能参与增强作用,在PTP和LTP期间测量了易化作用。在PTP期间易化作用降至约零,但在LTP开始约15分钟后恢复到正常值。已表明诱导LTP的一个必要条件是浴液中存在钙离子。然而,在强直刺激期间用高浓度的六甲铵(3毫摩尔)阻断突触传递并不会阻断LTP的诱导。5. 应用毒蕈碱抑制剂阿托品(2微摩尔)不会影响PTP或LTP的幅度。6. 蛋白激酶C的激活剂佛波醇12,13 - 二丁酸酯(2微摩尔)增强了突触传递,并降低了由PTP引起的增强作用,尽管它不影响由LTP引起的增强作用,但是这种激酶的抑制剂星形孢菌素(0.5微摩尔)在强直后部分阻断了LTP的出现,而不影响PTP。7. 钙调蛋白抑制剂W - 7(5微摩尔)在强直后显著且可逆地阻断了LTP的出现,尽管PTP的大小不受影响。8. 此处呈现的结果表明,睫状神经节中LTP的起始是由于强直期间钙离子流入花萼状神经末梢,并且LTP的机制涉及钙 - 钙调蛋白依赖性过程。

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