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教程:避免和纠正 3D 荧光显微镜中的样本诱导球差伪影。

Tutorial: avoiding and correcting sample-induced spherical aberration artifacts in 3D fluorescence microscopy.

机构信息

Harvard Center for Biological Imaging, Harvard University, Cambridge, MA, USA.

Department of Molecular and Cellular Biology, Harvard University, Cambridge, MA, USA.

出版信息

Nat Protoc. 2020 Sep;15(9):2773-2784. doi: 10.1038/s41596-020-0360-2. Epub 2020 Jul 31.

Abstract

Spherical aberration (SA) occurs when light rays entering at different points of a spherical lens are not focused to the same point of the optical axis. SA that occurs inside the lens elements of a fluorescence microscope is well understood and corrected for. However, SA is also induced when light passes through an interface of refractive index (RI)-mismatched substances (i.e., a discrepancy between the RI of the immersion medium and the RI of the sample). SA due to RI mismatches has many deleterious effects on imaging. Perhaps most important for 3D imaging is that the distance the image plane moves in a sample is not equivalent to the distance traveled by an objective (or stage) during z-stack acquisition. This non-uniform translation along the z axis gives rise to artifactually elongated images (if the objective is immersed in a medium with a higher RI than that of the sample) or compressed images (if the objective is immersed in a medium with a lower RI than that of the sample) and alters the optimal axial sampling rate. In this tutorial, we describe why this distortion occurs, how it impacts quantitative measurements and axial resolution, and what can be done to avoid SA and thereby prevent distorted images. In addition, this tutorial aims to better inform researchers of how to correct RI mismatch-induced axial distortions and provides a practical ImageJ/Fiji-based tool to reduce the prevalence of volumetric measurement errors and lost axial resolution.

摘要

球差是当光线从球形透镜的不同点进入时,无法聚焦到光轴上的同一点而产生的。荧光显微镜的透镜元件内部的球差已经得到了很好的理解和纠正。然而,当光线通过折射率(RI)不匹配物质的界面时,也会产生球差(即浸液介质的 RI 与样品的 RI 之间存在差异)。由于 RI 不匹配而产生的球差对成像有许多有害影响。对于 3D 成像来说,最重要的可能是图像平面在样品中移动的距离与物镜(或载物台)在 z 堆叠采集过程中移动的距离不相等。这种沿 z 轴的非均匀平移会导致图像出现人为拉长(如果物镜浸入的介质的 RI 高于样品的 RI)或压缩(如果物镜浸入的介质的 RI 低于样品的 RI),并改变最佳轴向采样率。在本教程中,我们将描述这种失真是如何产生的,它如何影响定量测量和轴向分辨率,以及可以采取什么措施来避免球差,从而防止图像失真。此外,本教程旨在让研究人员更好地了解如何纠正 RI 失配对轴向失真的影响,并提供一个实用的基于 ImageJ/Fiji 的工具,以减少体积测量误差和丢失的轴向分辨率的发生。

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