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Spatiotemporal control of degenerate multiphoton fluorescence microscopy with delay-tunable femtosecond pulse pairs

机译:时延可调飞秒脉冲对对简并多光子荧光显微镜的时空控制

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摘要

Selective excitation of a particular fluorophore in an ensemble of different fluorophores with overlapping fluorescence spectra is shown to be dependent on the time delay of femtosecond pulse pairs in multiphoton fluorescence microscopy. In particular, the two-photon fluorescence behavior of the Texas Red and DAPI dye pair inside Bovine Pulmonary Artery Endothelial (BPAE) cells depends strongly on the center wavelength of the laser, as well as the delay between two identical laser pulses in one-color femtosecond pulse-pair excitation scheme. Thus, we present a novel design concept using pairs of femtosecond pulses at different central wavelengths and tunable pulse separations for controlling the image contrast between two spatially and spectrally overlapping fluorophores. This femtosecond pulse-pair technique is unique in utilizing the variation of dye dynamics inside biological cells as a contrast mode in microscopy of different fluorophores. (C) 2016 Elsevier B.V. All rights reserved.
机译:在多光子荧光显微镜中,不同荧光团的重叠荧光光谱中特定荧光团的选择性激发显示取决于飞秒脉冲对的时间延迟。特别是,牛肺动脉内皮(BPAE)细胞内部的德州红和DAPI染料对的双光子荧光行为在很大程度上取决于激光的中心波长,以及两个相同的激光脉冲在一种颜色中的延迟飞秒脉冲对激励方案。因此,我们提出了一种新颖的设计概念,使用不同中心波长的飞秒脉冲对和可调节的脉冲间隔来控制两个空间和光谱重叠的荧光团之间的图像对比度。飞秒脉冲对技术在利用生物细胞内部染料动力学的变化作为不同荧光团显微镜的对比模式方面具有独特性。 (C)2016 Elsevier B.V.保留所有权利。

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