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Fast Optical Sectioning for Widefield Fluorescence Mesoscopy with the Mesolens based on HiLo Microscopy

机译:基于HiLo显微镜的Mesolens的快速光学切片用于宽视野荧光镜检

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摘要

We present here a fast optical sectioning method for mesoscopy based on HiLo microscopy, which makes possible imaging of specimens of up to 4.4 mm × 3 mm × 3 mm in volume in under 17 hours (estimated for a z-stack comprising 1000 images excluding computation time) with subcellular resolution throughout. Widefield epifluorescence imaging is performed with the Mesolens using a high pixel-number camera capable of sensor-shifting to generate a 259.5 Megapixel image, and we have developed custom software to perform HiLo processing of the very large datasets. Using this method, we obtain comparable sectioning strength to confocal laser scanning microscopy (CLSM), with sections as thin as 6.8 ± 0.2 μm and raw acquisition speed of 1 minute per slice which is up to 30 times faster than CLSM on the full field of view (FOV) of the Mesolens of 4.4 mm with lateral resolution of 0.7 μm and axial resolution of 7 μm. We have applied this HiLo mesoscopy method to image fixed and fluorescently stained hippocampal neuronal specimens and a 5-day old zebrafish larva.
机译:我们在此介绍一种基于HiLo显微镜的介观快速光学切片方法,该方法可以在17小时内对体积达4.4 mm×3 mm×3 mm的标本成像(估计Z轴包括1000张图像,但不包括计算量)时间)与整个亚细胞的分辨率。 Mesolens使用能够感应器移位的高像素数相机执行宽场落射荧光成像,从而生成259.5兆像素图像,并且我们已经开发了定制软件来对非常大的数据集进行HiLo处理。使用这种方法,我们可以获得与共聚焦激光扫描显微镜(CLSM)相当的切片强度,切片薄至6.8±0.2μm,每片的原始采集速度为1分钟,比CLSM的整个视野​​快30倍。视场图(FOV)为4.4μmm的介电层,横向分辨率为0.7μm,轴向分辨率为7μm。我们已经应用这种HiLo介观方法对固定和荧光染色的海马神经元标本和5天大的斑马鱼幼虫进行成像。

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