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从侧向折射率阶跃变化附近的共焦图像中恢复荧光团浓度分布。

Recovering fluorophore concentration profiles from confocal images near lateral refractive index step changes.

机构信息

Norwegian University of Science and Technology (NTNU), Section for Biophysics and Medical Technology, Department of Physics, Høgskoleringen 5, Trondheim 7491, Norway.

出版信息

J Biomed Opt. 2016 Dec 1;21(12):126014. doi: 10.1117/1.JBO.21.12.126014.

Abstract

Optical aberrations due to refractive index mismatches occur in various types of microscopy due to refractive differences between the sample and the immersion fluid or within the sample. We study the effects of lateral refractive index differences by fluorescence confocal laser scanning microscopy due to glass or polydimethylsiloxane cuboids and glass cylinders immersed in aqueous fluorescent solution, thereby mimicking realistic imaging situations in the proximity of these materials. The reduction in fluorescence intensity near the embedded objects was found to depend on the geometry and the refractive index difference between the object and the surrounding solution. The observed fluorescence intensity gradients do not reflect the fluorophore concentration in the solution. It is suggested to apply a Gaussian fit or smoothing to the observed fluorescence intensity gradient and use this as a basis to recover the fluorophore concentration in the proximity of the refractive index step change. The method requires that the reference and sample objects have the same geometry and refractive index. The best results were obtained when the sample objects were also used for reference since small differences such as uneven surfaces will result in a different extent of aberration.

摘要

由于样品与浸液或样品内部的折射率差异,各种类型的显微镜都会出现折射率不匹配引起的像差。我们通过荧光共焦激光扫描显微镜研究了玻璃或聚二甲基硅氧烷长方体和玻璃圆柱体浸入水荧光溶液后由于横向折射率差异引起的影响,从而模拟了这些材料附近的实际成像情况。发现嵌入物体附近的荧光强度降低取决于物体的几何形状和与周围溶液的折射率差异。观察到的荧光强度梯度并不反映溶液中的荧光染料浓度。建议对观察到的荧光强度梯度进行高斯拟合或平滑处理,并以此为基础恢复折射率阶跃变化附近的荧光染料浓度。该方法要求参考和样品物体具有相同的几何形状和折射率。当样品物体也被用作参考时,会得到最佳结果,因为微小的差异,如不平整的表面,会导致不同程度的像差。

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