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基于光流的各向同性聚焦离子束扫描电镜重构插值方法。

Optical flow driven interpolation for isotropic FIB-SEM reconstructions.

机构信息

University of Almeria, Informatics Department, Agrifood Campus of International Excellence (ceiA3), Ctra. Sacramento, s/n, Almeria, 04120, Spain.

University of Almeria, Informatics Department, Agrifood Campus of International Excellence (ceiA3), Ctra. Sacramento, s/n, Almeria, 04120, Spain.

出版信息

Comput Methods Programs Biomed. 2022 Jun;221:106856. doi: 10.1016/j.cmpb.2022.106856. Epub 2022 May 5.

Abstract

BACKGROUND AND OBJECTIVE

Focused Ion Beam - Scanning Electron Microscopy (FIB-SEM) allows three-dimensional ultrastructural analysis of cells and tissues at the nanoscale. The technique iteratively removes a section of the sample with a FIB and takes an SEM image from the exposed surface. The section thickness is usually higher than the image pixel size to reduce acquisition time, thus resulting in anisotropic resolution. In this work, we explore novel interpolation methods along the sectioning direction to produce isotropic resolution and facilitate proper interpretation of the FIB-SEM 3D volumes.

METHODS

Classical interpolation methods are usually applied in this context under the assumption that the changes through successive images are relatively smooth. However, the actual 3D arrangement of the structures in the sample may cause significant changes in the biological features between consecutive images of the FIB-SEM stacks. We have developed a novel interpolation strategy that accounts for this variation by using the Optical Flow (OF) to estimate it. As an intermediate stage, OF-compensated images are produced by aligning the spatial regions of the biological structures. Interpolated images are then generated from these OF-compensated images. The final isotropic stack is assembled by interleaving the interpolated images with the original images of the anisotropic stack.

RESULTS

OF-driven and classical interpolation methods were compared using an objective assessment based on Pearson Correlation Coefficient (PCC) and a qualitative evaluation based on visual results, using public datasets and representative anisotropy conditions. The objective assessment demonstrated that the OF-driven interpolation always yields higher PCC values, with interpolated images closer to the ground truth. The qualitative evaluation corroborated those results and confirmed that classical interpolation may blur areas with substantial changes between consecutive images whereas OF-driven interpolation provides sharpness.

CONCLUSIONS

We have developed an OF-driven interpolation approach to generating FIB-SEM stacks with isotropic resolution from experimental anisotropic data. It adapts to the rapid variation of the biological structures observed through the images of the FIB-SEM stack. Our approach outperforms classical interpolation and manages to produce sharp interpolated views in cases where there are significant changes between consecutive experimental images.

摘要

背景与目的

聚焦离子束-扫描电子显微镜(FIB-SEM)允许在纳米尺度上对细胞和组织进行三维超微结构分析。该技术通过聚焦离子束(FIB)迭代地去除样品的一部分,并从暴露的表面获取扫描电子显微镜(SEM)图像。为了减少采集时间,通常会使切片厚度高于图像像素尺寸,从而导致各向异性分辨率。在这项工作中,我们探索了沿切片方向的新的插值方法,以产生各向同性分辨率,并便于正确解释 FIB-SEM 三维体积。

方法

在假设连续图像之间的变化相对平滑的情况下,通常在这种情况下应用经典的插值方法。然而,样品中结构的实际三维排列可能会导致 FIB-SEM 堆栈的连续图像之间的生物特征发生显著变化。我们开发了一种新的插值策略,通过使用光流(OF)来估计这种变化,从而考虑到这种变化。作为中间阶段,通过对齐生物结构的空间区域来生成 OF 补偿图像。然后从这些 OF 补偿图像生成插值图像。通过将插值图像与各向异性堆叠的原始图像交错来组装最终的各向同性堆叠。

结果

使用基于 Pearson 相关系数(PCC)的客观评估和基于视觉结果的定性评估,比较了 OF 驱动和经典插值方法,使用公共数据集和代表性各向异性条件。客观评估表明,OF 驱动的插值总是产生更高的 PCC 值,并且插值图像更接近真实值。定性评估证实了这些结果,并确认经典插值可能会使连续图像之间存在较大变化的区域模糊,而 OF 驱动的插值则提供了清晰度。

结论

我们开发了一种基于 OF 的插值方法,用于从实验性各向异性数据生成具有各向同性分辨率的 FIB-SEM 堆叠。它适应于通过 FIB-SEM 堆叠的图像观察到的生物结构的快速变化。在连续的实验图像之间存在显著变化的情况下,我们的方法优于经典插值,并设法生成清晰的插值视图。

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