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通过双光子激发的4Pi共聚焦荧光显微镜提高轴向分辨率。

Axial resolution enhancement by 4Pi confocal fluorescence microscopy with two-photon excitation.

作者信息

Glaschick Sylvia, Röcker Carlheinz, Deuschle Karen, Wiedenmann Jörg, Oswald Franz, Mailänder Volker, Nienhaus G Ulrich

机构信息

Institute of Biophysics, University of Ulm, 89069 Ulm, Germany.

出版信息

J Biol Phys. 2007 Dec;33(5-6):433-43. doi: 10.1007/s10867-008-9084-1. Epub 2008 Jun 19.

Abstract

Confocal fluorescence microscopy and two-photon microscopy have become important techniques for the three-dimensional imaging of intact cells. Their lateral resolution is about 200-300 nm for visible light, whereas their axial resolution is significantly worse. By superimposing the spherical wave fronts from two opposing objective lenses in a coherent fashion in 4Pi microscopy, the axial resolution is greatly improved to approximately 100 nm. In combination with specific tagging of proteins or other cellular structures, 4Pi microscopy enables a multitude of molecular interactions in cell biology to be studied. Here, we discuss the choice of appropriate fluorescent tags for dual-color 4Pi microscopy and present applications of this technique in cellular biophysics. We employ two-color fluorescence detection of actin and tubulin networks stained with fluorescent organic dyes; mitochondrial networks are imaged using the photoactivatable fluorescent protein EosFP. A further example concerns the interaction of nanoparticles with mammalian cells.

摘要

共聚焦荧光显微镜和双光子显微镜已成为对完整细胞进行三维成像的重要技术。对于可见光,它们的横向分辨率约为200 - 300纳米,而轴向分辨率则明显较差。在4Pi显微镜中,通过以相干方式叠加来自两个相对物镜的球面波前,轴向分辨率可大幅提高至约100纳米。结合蛋白质或其他细胞结构的特异性标记,4Pi显微镜能够研究细胞生物学中的多种分子相互作用。在此,我们讨论双色4Pi显微镜合适荧光标记的选择,并展示该技术在细胞生物物理学中的应用。我们采用荧光有机染料对肌动蛋白和微管蛋白网络进行双色荧光检测;使用光激活荧光蛋白EosFP对线粒体网络进行成像。另一个例子涉及纳米颗粒与哺乳动物细胞的相互作用。

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