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使用传统紫外激光共聚焦显微镜引发细胞应激与死亡

Triggering Cell Stress and Death Using Conventional UV Laser Confocal Microscopy.

作者信息

Morsch Marco, Radford Rowan A W, Don Emily K, Lee Albert, Hortle Elinor, Cole Nicholas J, Chung Roger S

机构信息

Department of Biomedical Sciences, Faculty of Medicine and Health Sciences, Macquarie University;

Department of Biomedical Sciences, Faculty of Medicine and Health Sciences, Macquarie University.

出版信息

J Vis Exp. 2017 Feb 3(120):54983. doi: 10.3791/54983.

DOI:10.3791/54983
PMID:28190072
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5409196/
Abstract

Using a standard confocal setup, a UV ablation method can be utilized to selectively induce cellular injury and to visualize single-cell responses and cell-cell interactions in the CNS in real-time. Previously, studying these cell-specific responses after injury often required complicated setups or the transfer of cells or animals into different, non-physiological environments, confounding immediate and short-term analysis. For example, drug-mediated ablation approaches often lack the specificity that is required to study single-cell responses and immediate cell-cell interactions. Similarly, while high-power pulsed laser ablation approaches provide very good control and tissue penetration, they require specialized equipment that can complicate real-time visualization of cellular responses. The refined UV laser ablation approach described here allows researchers to stress or kill an individual cell in a dose- and time-dependent manner using a conventional confocal microscope equipped with a 405-nm laser. The method was applied to selectively ablate a single neuron within a dense network of surrounding cells in the zebrafish spinal cord. This approach revealed a dose-dependent response of the ablated neurons, causing the fragmentation of cellular bodies and anterograde degeneration along the axon within minutes to hours. This method allows researchers to study the fate of an individual dying cell and, importantly, the instant response of cells-such as microglia and astrocytes-surrounding the ablation site.

摘要

使用标准共聚焦装置,紫外线消融方法可用于选择性诱导细胞损伤,并实时观察中枢神经系统中的单细胞反应和细胞间相互作用。以前,研究损伤后的这些细胞特异性反应通常需要复杂的装置,或者将细胞或动物转移到不同的、非生理环境中,这会混淆即时和短期分析。例如,药物介导的消融方法往往缺乏研究单细胞反应和即时细胞间相互作用所需的特异性。同样,虽然高功率脉冲激光消融方法能提供很好的控制和组织穿透性,但它们需要专门的设备,这可能会使细胞反应的实时可视化变得复杂。这里描述的改进的紫外线激光消融方法使研究人员能够使用配备405纳米激光的传统共聚焦显微镜,以剂量和时间依赖性方式对单个细胞进行应激或杀伤。该方法被应用于选择性消融斑马鱼脊髓中周围细胞密集网络内的单个神经元。这种方法揭示了被消融神经元的剂量依赖性反应,导致细胞体在数分钟到数小时内碎片化,并沿轴突进行顺行性变性。这种方法使研究人员能够研究单个垂死细胞的命运,重要的是,还能研究消融部位周围细胞(如小胶质细胞和星形胶质细胞)的即时反应。

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