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首页> 外文会议>Confocal, Multiphoton, and Nonlinear Microscopic Imaging III; Progress in Biomedical Optics and Imaging; vol.8 no.43; Proceedings of SPIE-The International Society for Optical Engineering; vol.6630 >Simultaneous Imaging of Confocal Fluorescence and Raman Spectrum
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Simultaneous Imaging of Confocal Fluorescence and Raman Spectrum

机译:共焦荧光和拉曼光谱的同时成像

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摘要

The advantage of confocal fluorescence microscopy is the ability to acquire high resolution images of fluorescent specimens non-invasively. On the other hand, the advantage of Raman microscopy is the ability to provide the chemical characteristics of specimens from spectroscopy. To obtain simultaneously high resolution images and chemical characteristics of specimens, fluorescence signals from stained cell and Raman spectrum from cell itself should be separated. By separating two kinds of signals, confocal fluorescence image and Raman spectrum are acquired simultaneously at the same position. In this paper, we demonstrate a confocal fluorescence microscopy combined with the Raman microscopy. And we propose a method that eliminates Raman spectrum of fluorophore itself from Raman spectrum of the stained cell and that obtains simultaneously confocal fluorescence image from stained cell and Raman spectrum of cell itself without replacing a cell.
机译:共聚焦荧光显微镜的优点是能够以非侵入方式获取荧光标本的高分辨率图像。另一方面,拉曼显微镜的优点是能够提供光谱学样本的化学特性。为了同时获得高分辨率的图像和标本的化学特性,应分离染色细胞的荧光信号和细胞本身的拉曼光谱。通过分离两种信号,可以在同一位置同时获取共焦荧光图像和拉曼光谱。在本文中,我们证明了共焦荧光显微镜与拉曼显微镜相结合。并且我们提出了一种方法,其从染色细胞的拉曼光谱中消除荧光团本身的拉曼光谱,并且从染色细胞和细胞本身的拉曼光谱中同时获得共焦荧光图像而无需更换细胞。

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