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Resolution improvement in STED super-resolution microscopy at low power using a phasor plot approach

机译:分辨率、超分辨率的改善显微镜在低功率使用相量图方法

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摘要

Stimulated emission depletion (STED) microscopy is a powerful super-resolution microscopy technique that has achieved significant results in breaking the resolution limit and relevant applications. In principle, STED super resolution is obtained by stimulated emission partially inhibiting the spontaneous emission in the periphery of a diffraction-limited area. However, very high depletion laser power is generally necessary for the enhancement of imaging resolution, which is harmful to live biological specimens due to its high phototoxicity and photo-bleaching effects. Therefore, further improving the STED resolution at a lower depletion power level has recently attracted increasing interest from researchers in various fields. In this work, a phasor plot approach combined with fluorescence lifetime imaging microscopy (FLIM) is used to resolve the abovementioned problem based on a long- and short-lifetime criterion. Firstly, the time-resolved data obtained by STED-FLIM is converted to the frequency domain via a phasor approach. Next, partial data is extracted according to the information on the phase and amplitude for resolution improvement. Then, fluorescent microspheres (100 nm in diameter) are observed under different depletion powers, resulting in a series of improved resolution through phasor plots. Finally, this method is applied to image human Nup153 in fixed HeLa cells, providing a 86 nm higher resolution than that in traditional STED imaging at a depletion power of 20 mW.
机译:受激发射损耗(发生的)显微镜一个强大的超分辨率显微技术在打破取得了显著的成果分辨率的限制和相关应用程序。原则上,发生超分辨率通过受激发射部分抑制自发发射的边缘衍射极限。激光功率损耗通常是必要的是提高成像分辨率有害生物标本由于其生活高的光毒性和photo-bleaching效果。因此,进一步改善、解决低损耗功率最近吸引了越来越多的研究人员的兴趣各领域。方法结合荧光寿命成像显微镜(这部电影)用于解决基于一个长期和上述问题用于标准。时间分辨STED-FLIM获得的数据通过矢量转换为频域的方法。根据阶段和信息振幅解决改进。荧光微球直径(100海里)观察到在不同的损耗,导致一系列的改善解决通过相量图。应用于人类固定希拉Nup153形象细胞,提供一个比86纳米的分辨率也越高在传统的损耗、成像20兆瓦的力量。

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