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Space- and time-resolved spectrophotometry in microsystems

机译:微系统中的空间和时间分辨分光光度法

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This work describes a simple optical method for obtaining, in a single still-capture image, the continuous absorbance spectra of samples at multiple locations of microsystems. This technique uses an unmodified bright-field microscope, an array of microlenses, and a diffraction grating to disperse the light transmitted by samples of 10- to 500-μm dimensions. By analyzing in a single image the first-order diffracted light, it is possible to collect the full and continuous absorbance spectra of samples at multiple locations (to a spatial resolution of ≈ 8 μm) in microwells and micro-channels to examine dynamic chemical events (to a time resolution of <10 ms). This article also discusses the optical basis of this method. The simultaneous resolution of wavelength, time, and space at a scale <10 μm provides additional capabilities for chemical and biological analysis.
机译:这项工作描述了一种简单的光学方法,用于在单个静止捕获的图像中获得微系统多个位置处的样品的连续吸收光谱。该技术使用未经修改的明场显微镜,微透镜阵列和衍射光栅来分散10到500μm尺寸的样本透射的光。通过在单张图像中分析一阶衍射光,可以在微孔和微通道中的多个位置(达到约8μm的空间分辨率)收集样品的完整和连续吸收光谱,以检查动态化学事件(时间分辨率小于10毫秒)。本文还讨论了此方法的光学基础。波长,时间和空间的同时分辨率小于10μm,为化学和生物学分析提供了额外的功能。

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