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来自胚胎期绿色荧光蛋白表达小鼠的用于动眼神经生长延时成像的离体动眼神经切片培养

Ex Vivo Oculomotor Slice Culture from Embryonic GFP-Expressing Mice for Time-Lapse Imaging of Oculomotor Nerve Outgrowth.

作者信息

Whitman Mary C, Bell Jessica L, Nguyen Elaine H, Engle Elizabeth C

机构信息

Department of Ophthalmology, Boston Children's Hospital; Department of Ophthalmology, Harvard Medical School; F.M. Kirby Neurobiology Center, Boston Children's Hospital;

Department of Ophthalmology, Boston Children's Hospital; F.M. Kirby Neurobiology Center, Boston Children's Hospital.

出版信息

J Vis Exp. 2019 Jul 16(149). doi: 10.3791/59911.

Abstract

Accurate eye movements are crucial for vision, but the development of the ocular motor system, especially the molecular pathways controlling axon guidance, has not been fully elucidated. This is partly due to technical limitations of traditional axon guidance assays. To identify additional axon guidance cues influencing the oculomotor nerve, an ex vivo slice assay to image the oculomotor nerve in real-time as it grows towards the eye was developed. E10.5 Isl-GFP embryos are used to generate ex vivo slices by embedding them in agarose, slicing on a vibratome, then growing them in a microscope stage-top incubator with time-lapse photomicroscopy for 24-72 h. Control slices recapitulate the in vivo timing of outgrowth of axons from the nucleus to the orbit. Small molecule inhibitors or recombinant proteins can be added to the culture media to assess the role of different axon guidance pathways. This method has the advantages of maintaining more of the local microenvironment through which axons traverse, not axotomizing the growing axons, and assessing the axons at multiple points along their trajectory. It can also identify effects on specific subsets of axons. For example, inhibition of CXCR4 causes axons still within the midbrain to grow dorsally rather than ventrally, but axons that have already exited ventrally are not affected.

摘要

精确的眼球运动对于视觉至关重要,但眼动系统的发育,尤其是控制轴突导向的分子途径,尚未完全阐明。部分原因是传统轴突导向测定法存在技术局限性。为了识别影响动眼神经的其他轴突导向线索,开发了一种离体切片测定法,用于在动眼神经向眼睛生长时实时成像。利用E10.5期Isl-GFP胚胎,将其嵌入琼脂糖中,在振动切片机上切片,然后在显微镜载物台顶部培养箱中培养,并进行延时显微摄影24 - 72小时,以生成离体切片。对照切片重现了轴突从核向眼眶生长的体内时间进程。可以向培养基中添加小分子抑制剂或重组蛋白,以评估不同轴突导向途径的作用。该方法具有以下优点:能维持轴突穿越的更多局部微环境,不对生长中的轴突进行轴突切断,并在轴突轨迹的多个点评估轴突。它还可以识别对特定轴突亚群的影响。例如,抑制CXCR4会导致仍在中脑内的轴突背向而非腹向生长,但已经从腹侧穿出的轴突不受影响。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7d8a/6771922/7f3ac49252cb/nihms-1052047-f0001.jpg

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