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Spatially-controlled illumination with rescan confocal microscopy enhances image quality, resolution and reduces photodamage

机译:具有重新扫描共聚焦显微镜的空间控制的照明提高了图像质量,分辨率和减少了光电模压

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Fluorescence microscopy is an important tool in biomedical imaging. An inherent trade-off lies between image quality and photodamage. Recently, we have introduced rescan confocal microscopy (RCM) that improves the lateral resolution of a confocal microscope down to 170 nm. Previously, we have demonstrated that with controlled-light exposure microscopy, spatial control of illumination reduces photodamage without compromising image quality. Here, we show that the combination of these two techniques leads to high resolution imaging with reduced photodamage without compromising image quality. Implementation of spatially-controlled illumination was carried out in RCM using a line scanning-based approach. Illumination is spatially-controlled for every line during imaging with the help of a prediction algorithm that estimates the spatial profile of the fluorescent specimen. The estimation is based on the information available from previously acquired line images. As a proof-of-principle, we show images of N1E-115 neuroblastoma cells, obtained by this new setup with reduced illumination dose, improved resolution and without compromising image quality.
机译:荧光显微镜是生物医学成像的重要工具。一种固有的权衡在于图像质量和光损伤之间。最近,我们引入了一个提高共焦显微镜下至170nm的横向分辨率重新扫描共聚焦显微镜(RCM)。以前,我们已经证明,与受控曝光显微镜,照明的空间控制减少光损伤而不损害图像质量。在这里,我们表明,这两种技术导致与减少光损伤高分辨率成像的同时不会影响图像质量相结合。空间上受控照明的实现是使用基于扫描线的方法在RCM中进行。与估计所述荧光试样的空间分布的预测算法的帮助下成像期间照明在空间上被控制的每行。估计是基于从先前获取的线图像信息。作为验证的原理,我们显示N1E-115神经母细胞瘤细胞的图像,通过具有降低的照射剂量,提高的分辨率这个新的设置和不影响图像质量获得。

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