首页> 美国卫生研究院文献>Journal of Visualized Experiments : JoVE >High-resolution Volume Imaging of Neurons by the Use of Fluorescence eXclusion Method and Dedicated Microfluidic Devices
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High-resolution Volume Imaging of Neurons by the Use of Fluorescence eXclusion Method and Dedicated Microfluidic Devices

机译:使用荧光排除方法和专用微流控设备对神经元进行高分辨率体成像

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摘要

Volume is an important parameter regarding physiological and pathological characteristics of neurons at different time scales. Neurons are quite unique cells regarding their extended ramified morphologies and consequently raise several methodological challenges for volume measurement. In the particular case of in vitro neuronal growth, the chosen methodology should include sub-micrometric axial resolution combined with full-field observation on time scales from minutes to hours or days. Unlike other methods like cell shape reconstruction using confocal imaging, electrically-based measurements or Atomic Force Microscopy, the recently developed Fluorescence eXclusion method (FXm) has the potential to fulfill these challenges. However, although being simple in its principle, implementation of a high-resolution FXm for neurons requires multiple adjustments and a dedicated methodology. We present here a method based on the combination of fluorescence exclusion, low-roughness multi-compartments microfluidic devices, and finally micropatterning to achieve in vitro measurements of local neuronal volume. The high resolution provided by the device allowed us to measure the local volume of neuronal processes (neurites) and the volume of some specific structures involved in neuronal growth, such as growth cones (GCs).
机译:体积是有关不同时间尺度上神经元的生理和病理特征的重要参数。神经元在其扩展的分支形态方面是非常独特的细胞,因此对体积测量提出了一些方法上的挑战。在体外神经元生长的特殊情况下,选择的方法应包括亚微米级轴向分辨率以及从几分钟到几小时或几天的时间范围内的全场观察。与其他方法(例如使用共聚焦成像的细胞形状重建,基于电的测量或原子力显微镜)不同,最近开发的荧光排除法(FXm)具有解决这些挑战的潜力。但是,尽管原理很简单,但为神经元实现高分辨率FXm需要进行多次调整和专门的方法。我们在这里提出了一种基于荧光排斥,低粗糙度多室微流控设备以及最后进行微图案化以实现局部神经元体积体外测量的组合方法。该设备提供的高分辨率使我们能够测量神经元过程(神经突)的局部体积以及与神经元生长有关的某些特定结构(例如生长锥)的体积。

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