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采用全内反射荧光受激发射损耗显微镜的荧光相关光谱法(TIRF-STED-FCS)。

Fluorescence correlation spectroscopy with a total internal reflection fluorescence STED microscope (TIRF-STED-FCS).

作者信息

Leutenegger Marcel, Ringemann Christian, Lasser Theo, Hell Stefan W, Eggeling Christian

机构信息

Department of NanoBiophotonics, Max Planck Institute for Biophysical Chemistry, Am Fassberg 11, 37077 Göttingen, Germany.

出版信息

Opt Express. 2012 Feb 27;20(5):5243-63. doi: 10.1364/OE.20.005243.

DOI:10.1364/OE.20.005243
PMID:22418331
Abstract

We characterize a novel fluorescence microscope which combines the high spatial discrimination of a total internal reflection epi-fluorescence (epi-TIRF) microscope with that of stimulated emission depletion (STED) nanoscopy. This combination of high axial confinement and dynamic-active lateral spatial discrimination of the detected fluorescence emission promises imaging and spectroscopy of the structure and function of cell membranes at the macro-molecular scale. Following a full theoretical description of the sampling volume and the recording of images of fluorescent beads, we exemplify the performance and limitations of the TIRF-STED nanoscope with particular attention to the polarization state of the laser excitation light. We demonstrate fluorescence correlation spectroscopy (FCS) with the TIRF-STED nanoscope by observing the diffusion of dye molecules in aqueous solutions and of fluorescent lipid analogs in supported lipid bilayers in the presence of background signal. The nanoscope reduced the out-of-focus background signal. A lateral resolution down to 40-50 nm was attained which was ultimately limited by the low lateral signal-to-background ratio inherent to the confocal epi-TIRF scheme. Together with the estimated axial confinement of about 55 nm, our TIRF-STED nanoscope achieved an almost isotropic and less than 1 attoliter small all-optically induced measurement volume.

摘要

我们描述了一种新型荧光显微镜,它将全内反射落射荧光(epi-TIRF)显微镜的高空间分辨率与受激发射损耗(STED)纳米显微镜的高空间分辨率结合在一起。这种对检测到的荧光发射的高轴向限制和动态主动横向空间分辨能力的结合,有望在大分子尺度上对细胞膜的结构和功能进行成像和光谱分析。在对采样体积和荧光珠图像记录进行完整的理论描述之后,我们举例说明了TIRF-STED纳米显微镜的性能和局限性,特别关注激光激发光的偏振态。我们通过观察染料分子在水溶液中的扩散以及荧光脂质类似物在有背景信号存在的支撑脂质双层中的扩散,展示了TIRF-STED纳米显微镜的荧光相关光谱(FCS)。该纳米显微镜降低了离焦背景信号。实现了低至40 - 50 nm的横向分辨率,这最终受到共焦epi-TIRF方案固有的低横向信背比的限制。结合估计约55 nm的轴向限制,我们的TIRF-STED纳米显微镜实现了几乎各向同性且小于1阿托升的全光诱导测量体积。

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