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培养中发育的神经肌肉突触的结构与生理学

Structure and physiology of developing neuromuscular synapses in culture.

作者信息

Takahashi T, Nakajima Y, Hirosawa K, Nakajima S, Onodera K

出版信息

J Neurosci. 1987 Feb;7(2):473-81. doi: 10.1523/JNEUROSCI.07-02-00473.1987.

DOI:10.1523/JNEUROSCI.07-02-00473.1987
PMID:3029342
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6568910/
Abstract

The structure and function of developing neuromuscular synapses in culture have been investigated. We used neuromuscular junctions formed by coculturing dissociated muscle cells and dissociated neurons obtained from Xenopus embryos. After recording nerve-evoked endplate potentials (e.p.p.s) and spontaneously occurring miniature endplate potentials (m.e.p.p.s) from a given junction, the same specimen was investigated for electron-microscopic histology. We surveyed almost the total area of the junctional region by making serial sections. Even in preparations cocultured for only a short time (4-11 hr), both e.p.p.s and m.e.p.p.s could be obtained. The junctional region of these early synapses revealed a simple structure. The presynaptic terminals contained smooth-surfaced clear vesicles, but there were no presynaptic specializations such as active zones. The width of the synaptic cleft was variable, with predominance of narrow regions (10-30 nm), and there was no basal lamina inside the cleft. When the coculture time was 1 d or longer, the junctional area started to show structural features resembling a mature neuromuscular synapse. In the presynaptic terminal there were active zones, consisting of the presynaptic density and an accumulation of vesicles near the density. In many junctions, the postsynaptic membrane showed densities and thickenings, with a widened synaptic cleft, that contained basal lamina. It is known that growth cones, prior to making neuromuscular junctions, can release the transmitter substance with a very long latency if stimulated repetitively. In contrast, e.p.p.s with short latencies can be evoked by single stimuli soon after the growth cones attach to muscle cells. However, our data did not reveal any structural changes to account for such functional changes.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

对培养中发育的神经肌肉突触的结构和功能进行了研究。我们使用从非洲爪蟾胚胎获得的解离肌肉细胞与解离神经元共培养形成的神经肌肉接头。在记录给定接头的神经诱发终板电位(e.p.p.s)和自发出现的微小终板电位(m.e.p.p.s)后,对同一标本进行电子显微镜组织学研究。我们通过制作连续切片来观察几乎整个接头区域。即使在仅共培养短时间(4 - 11小时)的标本中,也能获得e.p.p.s和m.e.p.p.s。这些早期突触的接头区域显示出简单的结构。突触前终末含有表面光滑的清亮小泡,但没有诸如活性区之类的突触前特化结构。突触间隙的宽度可变,以狭窄区域(10 - 30纳米)为主,间隙内没有基膜。当共培养时间为1天或更长时,接头区域开始呈现出类似于成熟神经肌肉突触的结构特征。在突触前终末有活性区,由突触前致密物和致密物附近的小泡聚集组成。在许多接头中,突触后膜显示出致密物和增厚,突触间隙变宽,其中含有基膜。已知生长锥在形成神经肌肉接头之前,如果反复受到刺激,能够以非常长的潜伏期释放递质。相反,在生长锥附着于肌肉细胞后不久,单次刺激就能诱发潜伏期短的e.p.p.s。然而,我们的数据并未揭示任何能够解释这种功能变化的结构变化。(摘要截断于250字)

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