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通过共聚焦荧光显微镜对神经肌肉接头进行成像:在完整肌肉中观察到的单个终板,神经末梢进行了活细胞内染色。

Imaging neuromuscular junctions by confocal fluorescence microscopy: individual endplates seen in whole muscles with vital intracellular staining of the nerve terminals.

作者信息

Marques M J, Santo Neto H

机构信息

Department of Anatomy, Institute of Biology, UNICAMP, São Paulo, Brazil.

出版信息

J Anat. 1998 Apr;192 ( Pt 3)(Pt 3):425-30. doi: 10.1046/j.1469-7580.1998.19230425.x.

DOI:10.1046/j.1469-7580.1998.19230425.x
PMID:9688508
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1467786/
Abstract

The mammalian neuromuscular junction has been extensively studied by different methods to understand better the biological aspects of its normal development, ageing and pathological conditions, such as disorders of neuromuscular transmission. In the present report, a new technique is described that combines confocal microscopy with the use of a vital nerve terminal dye (4-Di-2-ASP) and rhodamine-alpha-bungarotoxin to stain postsynaptic acetylcholine receptors in the same endplate. Nerve terminals in the sternomastoid muscles of living adult mice were stained with 4-Di-2-ASP, which labels intracellular compartments of the nerve terminal containing mitochondria. Slides of these muscles were viewed by confocal microscopy and images were stored on magnetic optical discs. This procedure was compatible with subsequent acetylcholine receptor staining with rhodamine-alpha-bungarotoxin and observation under the confocal microscope. Classical features of the adult neuromuscular junction were displayed, such as the branched-pattern distribution of the nerve terminals and receptors and their complete colocalisation. In addition, nerve fibres from intramuscular nerve branches with their neighbouring cells, nuclei and muscle fibre striations could also be visualised. We conclude that the present technique can complement existing methods of investigation of nerve terminal anatomy and pathology, particularly where preservation of 3-dimensional relationships is required and intracellular disturbances involving mitochondrial organisation, such as ageing or other degenerative disorders, may be present.

摘要

为了更好地理解哺乳动物神经肌肉接头正常发育、衰老及病理状况(如神经肌肉传递障碍)的生物学特性,人们已采用不同方法对其进行了广泛研究。在本报告中,我们描述了一种新技术,该技术将共聚焦显微镜与一种活性神经末梢染料(4-Di-2-ASP)及罗丹明-α-银环蛇毒素相结合,用于在同一终板中对突触后乙酰胆碱受体进行染色。用4-Di-2-ASP对成年活体小鼠胸锁乳突肌中的神经末梢进行染色,该染料可标记含有线粒体的神经末梢细胞内区室。通过共聚焦显微镜观察这些肌肉的切片,并将图像存储在磁光盘上。此程序与随后用罗丹明-α-银环蛇毒素进行乙酰胆碱受体染色及在共聚焦显微镜下观察兼容。展示了成年神经肌肉接头的典型特征,如神经末梢和受体的分支模式分布及其完全共定位。此外,来自肌内神经分支的神经纤维及其相邻的细胞、细胞核和肌纤维条纹也清晰可见。我们得出结论,本技术可补充现有的神经末梢解剖学和病理学研究方法,特别是在需要保留三维关系且可能存在涉及线粒体组织的细胞内紊乱(如衰老或其他退行性疾病)的情况下。

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