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免疫标记和计数年轻成年和老年沙鼠耳蜗中的带状突触。

Immunolabeling and Counting Ribbon Synapses in Young Adult and Aged Gerbil Cochleae.

机构信息

Cluster of Excellence "Hearing4all" and Research Centre Neurosensory Science, Department of Neuroscience, School of Medicine and Health Science, Carl von Ossietzky University Oldenburg.

Cluster of Excellence "Hearing4all" and Research Centre Neurosensory Science, Department of Neuroscience, School of Medicine and Health Science, Carl von Ossietzky University Oldenburg;

出版信息

J Vis Exp. 2022 Apr 21(182). doi: 10.3791/63874.

Abstract

The loss of ribbon synapses connecting inner hair cells and afferent auditory nerve fibers is assumed to be one cause of age-related hearing loss. The most common method for detecting the loss of ribbon synapses is immunolabeling because it allows for quantitative sampling from several tonotopic locations in an individual cochlea. However, the structures of interest are buried deep inside the bony cochlea. Gerbils are used as an animal model for age-related hearing loss. Here, routine protocols for fixation, immunolabeling gerbil cochlear whole mounts, confocal imaging, and quantifying ribbon synapse numbers and volumes are described. Furthermore, the particular challenges associated with obtaining good material from valuable aging individuals are highlighted. Gerbils are euthanized and either perfused cardiovascularly, or their tympanic bullae are carefully dissected out of the skull. The cochleae are opened at the apex and base and directly transferred to the fixative. Irrespective of the initial method, the cochleae are postfixed and subsequently decalcified. The tissue is then labeled with primary antibodies against pre- and postsynaptic structures and hair cells. Next, the cochleae are incubated with secondary fluorescence-tagged antibodies that are specific against their respective primary ones. The cochleae of aged gerbils are then treated with an autofluorescence quencher to reduce the typically substantial background fluorescence of older animals' tissues. Finally, cochleae are dissected into 6-11 segments. The entire cochlear length is reconstructed such that specific cochlear locations can be reliably determined between individuals. Confocal image stacks, acquired sequentially, help visualize hair cells and synapses at the chosen locations. The confocal stacks are deconvolved, and the synapses are either counted manually using ImageJ, or more extensive quantification of synaptic structures is carried out with image analysis procedures custom-written in Matlab.

摘要

内毛细胞和传入听觉神经纤维之间连接的 ribbon 突触的丧失被认为是与年龄相关的听力损失的一个原因。检测 ribbon 突触丧失的最常见方法是免疫标记,因为它允许从个体耳蜗的几个音调位置进行定量采样。然而,感兴趣的结构深埋在骨耳蜗内。沙鼠被用作与年龄相关的听力损失的动物模型。这里描述了固定、免疫标记沙鼠耳蜗全培养物、共焦成像以及量化 ribbon 突触数量和体积的常规方案。此外,还强调了从有价值的老年个体中获得良好材料所面临的特殊挑战。沙鼠被安乐死,要么通过心血管灌注,要么小心地将其鼓室泡从颅骨中分离出来。耳蜗在顶点和基部打开,并直接转移到固定剂中。无论初始方法如何,耳蜗都要后固定,然后脱钙。然后,组织用针对前突触和后突触结构以及毛细胞的初级抗体进行标记。接下来,耳蜗与针对各自初级抗体的二级荧光标记抗体孵育。然后,用自动荧光淬灭剂处理老年沙鼠的耳蜗,以减少老年动物组织中通常存在的大量背景荧光。最后,耳蜗被切成 6-11 个部分。整个耳蜗长度被重建,以便在个体之间可靠地确定特定的耳蜗位置。顺序获取的共焦图像堆栈有助于在选定位置可视化毛细胞和突触。共焦堆栈去卷积,然后使用 ImageJ 手动计数突触,或者使用在 Matlab 中编写的自定义图像分析程序对突触结构进行更广泛的定量分析。

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