A young researcher’s guide to three-dimensional fluorescence microscopy of living cells

Pub Date : 2023-10-25 DOI:10.18054/pb.v125i1-2.25140
Vedrana Filić, Igor Weber
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Abstract

Three-dimensional imaging of fast intracellular processes by fluorescence microscopy should provide decent spatial and high temporal resolution while minimizing fluorophore bleaching and cytotoxicity. We give a condensed introductory overview of three contemporary methods mostly used for imaging of living cells in 3D and compare their performance in terms of temporal and spatial resolution, imaging flexibility and specimen photodamage: point-scanning confocal microscopy, spinning-disc confocal microscopy, and lattice light-sheet microscopy. While point-scanning instruments are unsurpassed in terms of confocal performance, flexibility and configurability of their optical path, spinning-disc and lattice light-sheet optical designs excel in acquisition speed and low levels of light-inflicted specimen deterioration.
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年轻研究者的活细胞三维荧光显微镜指南
通过荧光显微镜快速细胞内过程的三维成像应该提供体面的空间和高时间分辨率,同时最大限度地减少荧光团漂白和细胞毒性。我们简要介绍了三种主要用于活细胞三维成像的当代方法,并比较了它们在时间和空间分辨率、成像灵活性和标本光损伤方面的性能:点扫描共聚焦显微镜、旋转光盘共聚焦显微镜和晶格光片显微镜。虽然点扫描仪器在共聚焦性能、光路的灵活性和可配置性方面是无与伦比的,但旋转盘和点阵光片光学设计在采集速度和低水平的光致试样劣化方面表现出色。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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