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采用长波长照明对深部小鼠脑进行无标记共聚焦成像。

label-free confocal imaging of the deep mouse brain with long-wavelength illumination.

作者信息

Xia Fei, Wu Chunyan, Sinefeld David, Li Bo, Qin Yifan, Xu Chris

机构信息

School of Applied and Engineering Physics, Cornell University, Ithaca, NY 14853, USA.

Meinig School of Biomedical Engineering, Cornell University, Ithaca, NY 14853, USA.

出版信息

Biomed Opt Express. 2018 Nov 29;9(12):6545-6555. doi: 10.1364/BOE.9.006545. eCollection 2018 Dec 1.

Abstract

Optical microscopy is a valuable tool for monitoring of biological structures and functions because of its non-invasiveness. However, imaging deep into biological tissues is challenging due to the scattering and absorption of light. Previous research has shown that 1300 nm and 1700 nm are the two best wavelength windows for deep brain imaging. Here, we combined long-wavelength illumination of ~1700 nm with reflectance confocal microscopy and achieved an imaging depth of ~1.3 mm with ~1-micrometer spatial resolution in adult mouse brains, which is 3-4 times deeper than that of conventional confocal microscopy using visible wavelength. We showed that the method can be added to any laser-scanning microscopy with simple and low-cost sources and detectors, such as continuous-wave diode lasers and InGaAs photodiodes. The long-wavelength, reflectance confocal imaging we demonstrated is label-free, and requires low illumination power. Furthermore, the imaging system is simple and low-cost, potentially creating new opportunities for biomedical research and clinical applications.

摘要

光学显微镜因其非侵入性而成为监测生物结构和功能的宝贵工具。然而,由于光的散射和吸收,对生物组织进行深度成像具有挑战性。先前的研究表明,1300纳米和1700纳米是用于深部脑成像的两个最佳波长窗口。在此,我们将约1700纳米的长波长照明与反射共聚焦显微镜相结合,在成年小鼠大脑中实现了约1.3毫米的成像深度和约1微米的空间分辨率,这比使用可见波长的传统共聚焦显微镜的成像深度深3至4倍。我们表明,该方法可以添加到任何使用简单且低成本的光源和探测器的激光扫描显微镜中,例如连续波二极管激光器和铟镓砷光电二极管。我们所展示的长波长反射共聚焦成像无需标记,且所需照明功率低。此外,该成像系统简单且成本低,可能为生物医学研究和临床应用创造新机会。

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