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Optical recordings of Ca2+ signaling activities from identified inner ear cells in cochlear slices and hemicochleae.

机译:Ca2 +信号活性的光学记录,来自耳蜗切片和半裸片中已鉴定的内耳细胞。

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One of the major obstacles hindering the progress of studies on mammalian cochlear physiology is the inaccessibility of inner ear cells located in a complex structure of the bony labyrinth. We describe here a technique to record cellular fluorescent signals from any identified inner ear cells in cochlear slices and hemicochleae. Cochlear slices were obtained from postnatal rats (P0-P7) before the cochlea completely ossify, and hemicochleae were cut from older animals (P7-adult). Individual inner ear cells were visually identified using infrared differential interference contrast or oblique illumination optics. Techniques were developed for either bulk-loading cells or loading selected single cells with Ca(2+) indicator dyes, and for maintaining functional viability of cochlear slices/hemicochleae for recordings. Robust and reliable responses of ligand-gated receptors were recorded from individual inner ear cells (e.g. hair cells, spiral ganglion neurons etc.) for at least 24 h after slices/hemicochleaewere cut by an oscillating tissue slicer. The technique described here allowed direct observations of [Ca(2+)](i) activities from multiple cells simultaneously in situ, thus providing a feasible way to study the intercellular communication or networking activities from identified cells in the inner ear.
机译:阻碍哺乳动物耳蜗生理学研究进展的主要障碍之一是无法进入位于骨迷宫复杂结构中的内耳细胞。我们在这里描述一种技术来记录来自任何已识别的内耳细胞的耳蜗切片和半裸细胞的细胞荧光信号。在耳蜗完全骨化之前,从产后大鼠(P0-P7)获得耳蜗切片,并从年长的动物(P7-成年动物)切下半线虫。使用红外微分干涉对比或倾斜照明光学元件在视觉上识别单个内耳细胞。开发了用于批量加载细胞或使用Ca(2+)指示剂染料加载选定的单个细胞,并保持用于记录的耳蜗片/半功能性功能的技术。在振荡的组织切片机切下切片/半鞭毛后至少24小时内,从各个内耳细胞(例如毛细胞,螺旋神经节神经元等)记录到配体门控受体的鲁棒而可靠的响应。这里描述的技术允许直接从原位同时观察多个细胞的[Ca(2 +)](i)活动,从而提供了一种可行的方法来研究内耳中已识别细胞的细胞间通讯或网络活动。

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