使用DiI, NeuroVue和高尔基方法进行频率映射的耳蜗神经元追踪。

Yayoi S Kikkawa, Karen S Pawlowski
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引用次数: 2

摘要

结论:使用NeuroVue Red染料的标记实验使我们能够展示耳蜗中从Corti器官内毛细胞突触区到Rosenthal管螺旋神经节的单个传入纤维轨迹。为了获得根尖区域的三维神经分布,需要进一步优化以进行频率映射。目的:我们打算开发一种方法,通过螺旋神经节(SG)的径向纤维可以单独可视化和三维跟踪从耳蜗基部到顶点。然后可以计算每个耳蜗纤维的组合轨迹,用于人工耳蜗研究中OC和SG的三维关系建模,以帮助优化人工耳蜗在噪声中对音乐和语言的感知。材料和方法:我们测试了三种不同的方法来可视化耳蜗神经纤维从OC到SG。用DiI染色、改良高尔基-考克斯染色或NeuroVue染色对成年大鼠和小鼠耳进行染色,切片或整片,共聚焦显微镜或标准光学显微镜下观察。结果:在DiI染色中,空间分辨率和待染色神经元的数量太低,无法利用该方法创建耳蜗的特征频率图。高尔基法主要染色传出神经纤维,对耳蜗神经分布的信息较少。当与DAPI反染色相结合时,NeuroVue Red染料可以清晰地跟踪单个纤维。
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Cochlear neuronal tracing for frequency mapping with DiI, NeuroVue, and Golgi methods.

Conclusions: Labeling experiments using NeuroVue Red dye allowed us to demonstrate individual afferent fiber tracks in the cochlea from the synaptic region of the inner hair cell in the organ of Corti (OC) to the spiral ganglion in Rosenthal's canal. Further optimization is necessary to obtain 3-dimensional (3D) neural distribution in the apical region for frequency mapping.

Objectives: We intend to develop a method by which the radial fibers of the spiral ganglion (SG) can be individually visualized and tracked in 3D from the base to the apex of the cochlea. The combined trajectories of fibers from each cochlea could then be calculated for modeling of the 3D relationship of OC and SG in cochlear implant studies to assist in the optimization of cochlear implants for music and speech perception in noise.

Materials and methods: We tested three different methods to visualize cochlear nerve fibers from OC to SG. Adult rat and mouse ears were stained with DiI dye, modified Golgi-Cox method or NeuroVue dye, sectioned or whole-mounted, and viewed with confocal or standard light microscope.

Results: In DiI staining, spacial resolution and the number of neurons to be stained are too low to utilize this method to create a characteristic frequency map of the cochlea. The Golgi method mainly stained efferent nerve fibers, resulting in less information on cochlear nerve distribution. NeuroVue Red dye allowed clear tracking of individual fibers when combined with DAPI counterstaining.

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