Reduced deep-tissue image degradation in three-dimensional multiphoton microscopy with concentric two-color two-photon fluorescence excitation

Chen Wang; Lingling Qiao; Zhengle Mao; Ya Cheng; Zhizhan Xu

doi:10.1364/JOSAB.25.000976

Reduced deep-tissue image degradation in three-dimensional multiphoton microscopy with concentric two-color two-photon fluorescence excitation

Chen Wang^*
, Lingling Qiao
, Zhengle Mao
, Ya Cheng
, Zhizhan Xu

^*此作品的通讯作者

CAS - Shanghai Institute of Optics and Fine Mechanics

科研成果: 期刊稿件 › 文章 › 同行评审

20 引用（Scopus）

摘要

We theoretically demonstrate that enhanced penetration depth in three-dimensional multiphoton microscopy can be achieved using concentric two-color two-photon (C2C2P) fluorescence excitation in which the two excitation beams are separated in space before reaching their common focal spot. Monte Carlo simulation shows that, in comparison with the one-color two-photon excitation scheme, the C2C2P fluorescence microscopy provides a significantly greater penetration depth for imaging into a highly scattering medium.

源语言	英语
页（从-至）	976-982
页数	7
期刊	Journal of the Optical Society of America B: Optical Physics
卷	25
期	6
DOI	https://doi.org/10.1364/JOSAB.25.000976
出版状态	已出版 - 6月 2008
已对外发布	是

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abstract = "We theoretically demonstrate that enhanced penetration depth in three-dimensional multiphoton microscopy can be achieved using concentric two-color two-photon (C2C2P) fluorescence excitation in which the two excitation beams are separated in space before reaching their common focal spot. Monte Carlo simulation shows that, in comparison with the one-color two-photon excitation scheme, the C2C2P fluorescence microscopy provides a significantly greater penetration depth for imaging into a highly scattering medium.",

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T1 - Reduced deep-tissue image degradation in three-dimensional multiphoton microscopy with concentric two-color two-photon fluorescence excitation

AU - Wang, Chen

AU - Qiao, Lingling

AU - Mao, Zhengle

AU - Cheng, Ya

AU - Xu, Zhizhan

PY - 2008/6

Y1 - 2008/6

N2 - We theoretically demonstrate that enhanced penetration depth in three-dimensional multiphoton microscopy can be achieved using concentric two-color two-photon (C2C2P) fluorescence excitation in which the two excitation beams are separated in space before reaching their common focal spot. Monte Carlo simulation shows that, in comparison with the one-color two-photon excitation scheme, the C2C2P fluorescence microscopy provides a significantly greater penetration depth for imaging into a highly scattering medium.

AB - We theoretically demonstrate that enhanced penetration depth in three-dimensional multiphoton microscopy can be achieved using concentric two-color two-photon (C2C2P) fluorescence excitation in which the two excitation beams are separated in space before reaching their common focal spot. Monte Carlo simulation shows that, in comparison with the one-color two-photon excitation scheme, the C2C2P fluorescence microscopy provides a significantly greater penetration depth for imaging into a highly scattering medium.

UR - https://www.scopus.com/pages/publications/50449106496

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DO - 10.1364/JOSAB.25.000976

M3 - 文章

AN - SCOPUS:50449106496

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JO - Journal of the Optical Society of America B: Optical Physics

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ER -

Reduced deep-tissue image degradation in three-dimensional multiphoton microscopy with concentric two-color two-photon fluorescence excitation

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