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饱和激发显微镜与优化激发调制。

Saturated excitation microscopy with optimized excitation modulation.

机构信息

Department of Applied Physics, Osaka University, 2-1 Yamadaoka, Suita, Osaka 565-0871 (Japan).

出版信息

Chemphyschem. 2014 Mar 17;15(4):743-9. doi: 10.1002/cphc.201300879. Epub 2014 Feb 2.

Abstract

Saturated excitation (SAX) microscopy utilizes the nonlinear relation between fluorescence emission and excitation under saturated excitation to improve the spatial resolution of confocal microscopy. In this study, we theoretically and experimentally investigate the saturation of fluorescence excitation under modulated excitation to optimize the excitation conditions for SAX microscopy. Calculation of the relationships between fluorescence and excitation intensity with different modulation frequencies reveals that the lifetime of the triplet state of the fluorescent probe strongly affects the strength of the demodulated fluorescence signals. We also find that photobleaching shows little dependence on the modulation frequency. These investigations allow us to determine the optimum excitation conditions, that is, the conditions providing sufficient fluorescence saturation without strong photobleaching. For a sample stained with ATTO Rho6G phalloidin, we estimate the optimal excitation conditions, which are produced with 50 kHz excitation modulation and a 50 μsec pixel dwell time, and successfully perform three-dimensional imaging with sub-diffraction resolution.

摘要

饱和激发(SAX)显微镜利用饱和激发下荧光发射与激发之间的非线性关系来提高共焦显微镜的空间分辨率。在这项研究中,我们从理论和实验上研究了调制激发下荧光激发的饱和情况,以优化 SAX 显微镜的激发条件。计算不同调制频率下荧光与激发强度之间的关系表明,荧光探针的三重态寿命强烈影响解调荧光信号的强度。我们还发现光漂白几乎不依赖于调制频率。这些研究使我们能够确定最佳的激发条件,即在没有强烈光漂白的情况下提供足够荧光饱和的条件。对于用 ATTO Rho6G 鬼笔环肽染色的样品,我们估计最佳激发条件为 50 kHz 激发调制和 50 μs 像素停留时间,并成功地进行了具有亚衍射分辨率的三维成像。

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