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Confocal microscopy for astrocyte in vivo imaging: Recycle and reuse in microscopy

机译:共聚焦显微镜用于星形胶质细胞体内成像:显微镜中的回收和再利用

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摘要

In vivo imaging is one of the ultimate and fundamental approaches for the study of the brain. Two-photon laser scanning microscopy (2PLSM) constitutes the state-of-the-art technique in current neuroscience to address questions regarding brain cell structure, development and function, blood flow regulation and metabolism. This technique evolved from laser scanning confocal microscopy (LSCM), which impacted the field with a major improvement in image resolution of live tissues in the 1980s compared to widefield microscopy. While nowadays some of the unparalleled features of 2PLSM make it the tool of choice for brain studies in vivo, such as the possibility to image deep within a tissue, LSCM can still be useful in this matter. Here we discuss the validity and limitations of LSCM and provide a guide to perform high-resolution in vivo imaging of the brain of live rodents with minimal mechanical disruption employing LSCM. We describe the surgical procedure and experimental setup that allowed us to record intracellular calcium variations in astrocytes evoked by sensory stimulation, and to monitor intact neuronal dendritic spines and astrocytic processes as well as blood vessel dynamics. Therefore, in spite of certain limitations that need to be carefully considered, LSCM constitutes a useful, convenient, and affordable tool for brain studies in vivo.
机译:体内成像是研究大脑的最终方法和基本方法之一。两光子激光扫描显微镜(2PLSM)构成了当前神经科学领域的最新技术,旨在解决有关脑细胞结构,发育和功能,血流调节和代谢的问题。这项技术是从激光扫描共聚焦显微镜(LSCM)演变而来的,与宽视野显微镜相比,激光扫描共聚焦显微镜(LSCM)在1980年代对活组织的图像分辨率产生了重大影响。如今,尽管2PLSM的一些无与伦比的功能使其成为体内大脑研究的首选工具,例如可以在组织内部进行深层成像,但LSCM在此问题上仍然有用。在这里,我们讨论了LSCM的有效性和局限性,并为使用LSCM进行最小程度的机械破坏的活啮齿动物的大脑进行高分辨率的体内成像提供了指导。我们描述了外科手术程序和实验设置,使我们能够记录由感觉刺激诱发的星形胶质细胞中的细胞内钙变化,并监测完整的神经元树突棘和星形胶质细胞以及血管动态。因此,尽管有一些局限性需要仔细考虑,但LSCM仍然是用于体内脑研究的有用,方便且负担得起的工具。

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