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青蛙神经肌肉接头处递质释放和突触小泡循环的光学监测。

Optical monitoring of transmitter release and synaptic vesicle recycling at the frog neuromuscular junction.

作者信息

Betz W J, Bewick G S

机构信息

Department of Physiology, University of Colorado School of Medicine, Denver 80220.

出版信息

J Physiol. 1993 Jan;460:287-309. doi: 10.1113/jphysiol.1993.sp019472.

DOI:10.1113/jphysiol.1993.sp019472
PMID:8387585
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1175214/
Abstract
  1. Frog cutaneous pectoris motor nerve terminals were loaded with the fluorescent dye FM1-43, which produced a series of discrete spots along the length of terminals, each spot evidently marking a cluster of synaptic vesicles. Terminals were imaged for 2-10 min as they destained during repetitive nerve stimulation. Endplate potentials (EPPs) were recorded simultaneously from the muscle fibres innervated by these terminals; their summed amplitudes provided a measure of cumulative transmitter release. 2. Individual fluorescent spots in any one terminal varied in initial brightness but destained at similar fractional rates. 3. The rates of cumulative transmitter release and destaining increased with stimulus frequency in the range 2-30 Hz. At 40 Hz, however, both transmitter release and destaining were slower than at 30 Hz. 4. In twenty-six experiments, rates of dye loss and transmitter release were compared quantitatively. When the time course of summed EPPs was scaled to fit the time course of dye loss during the first 30-60 s of destaining, the two curves usually diverged at later times, the dye loss curve falling below the summed EPP curve. Thus, assuming that dye loss and transmitter release are proportional at early times, at later times the rate of dye loss decreases relative to the rate of transmitter release. 5. At stimulus frequencies from 2 to 30 Hz, the results could be fitted by a simple model in which vesicles lose their dye during exocytosis and, after a fixed recycle 'dead time', they re-enter the vesicle pool, mixing randomly with other vesicles. 6. Unlike stimulation at lower frequencies, at 40 Hz dye loss and summed EPP amplitude curves did not significantly diverge. Stimulation periods lasted up to about 2 min. Interpreted according to the model of vesicle recycling, this suggests that vesicle recycling is inhibited at 40 Hz. 7. The model led to predictions about the relative number, N, of vesicles (labelled and unlabelled) in the terminal at any time during stimulation. The calculated value of N decreased at times less than the recycle 'dead time', and then increased, reflecting the appearance of recycled vesicles in the vesicle pool. 8. From estimates of N and recorded EPP amplitudes, the fraction of vesicles released per shock, F, could be calculated during the entire stimulation period. At low stimulus frequencies (2-5 Hz), after an initial rapid fall, F decreased slowly and monotonically by about 50% in 6 min. At higher stimulus frequencies, a different process was observed.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 用荧光染料FM1-43标记青蛙胸皮运动神经末梢,该染料沿神经末梢长度产生一系列离散的斑点,每个斑点明显标记着一群突触小泡。在重复神经刺激过程中,当神经末梢褪色时,对其进行2至10分钟的成像。同时记录这些神经末梢所支配的肌肉纤维的终板电位(EPPs);它们的总振幅提供了累积递质释放的一种度量。2. 任何一个神经末梢中的单个荧光斑点初始亮度不同,但以相似的分数速率褪色。3. 在2至30赫兹的范围内,累积递质释放速率和褪色速率随刺激频率增加。然而,在40赫兹时,递质释放和褪色都比30赫兹时慢。4. 在26次实验中,对染料损失速率和递质释放速率进行了定量比较。当将总EPPs的时间进程按比例缩放以拟合褪色最初30至60秒内染料损失的时间进程时,两条曲线通常在后期发散,染料损失曲线低于总EPP曲线。因此,假设在早期染料损失和递质释放成比例,在后期染料损失速率相对于递质释放速率下降。5. 在2至30赫兹的刺激频率下,结果可以用一个简单模型拟合,在该模型中,小泡在胞吐过程中失去染料,经过固定的再循环“停滞时间”后,它们重新进入小泡池,与其他小泡随机混合。6. 与较低频率的刺激不同,在40赫兹时,染料损失和总EPP振幅曲线没有明显发散。刺激期持续长达约2分钟。根据小泡再循环模型解释,这表明在40赫兹时小泡再循环受到抑制。7. 该模型对刺激期间任何时刻神经末梢中(标记和未标记的)小泡的相对数量N做出了预测。计算出的N值在小于再循环“停滞时间”时下降,然后上升,反映了再循环小泡在小泡池中的出现。8. 根据N的估计值和记录的EPP振幅,可以在整个刺激期计算每次刺激释放的小泡分数F。在低刺激频率(2至5赫兹)下,最初快速下降后,F在6分钟内缓慢且单调下降约50%。在较高刺激频率下,观察到不同的过程。(摘要截断于400字)
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d357/1175214/3e83dc748ad8/jphysiol00422-0303-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d357/1175214/3e83dc748ad8/jphysiol00422-0303-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d357/1175214/3e83dc748ad8/jphysiol00422-0303-a.jpg

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