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小鼠肝细胞核连续切片的登记

Registration of serial sections of mouse liver cell nuclei.

作者信息

Baheerathan S, Albregtsen F, Danielsen H E

机构信息

Image Processing Laboratory, Department of Informatics, University of Oslo, Norway.

出版信息

J Microsc. 1998 Oct;192(Pt 1):37-53. doi: 10.1046/j.1365-2818.1998.00405.x.

DOI:10.1046/j.1365-2818.1998.00405.x
PMID:9848269
Abstract

Image registration of biological tissue is essential for 3D reconstruction, which is important for visualizing and quantifying the 3D relationships between internal structures of an object. The biological role of DNA organization, which is an extremely complex 3D architecture within the cell nucleus, has come into focus since it has become clear that the chromatin structure in itself functions as a regulator of DNA. Thus, 3D reconstruction of cell nuclei based on consecutive series of high-resolution ultrathin slices may provide new information about the chromatin structure and its organizational changes during carcinogenesis. This work focuses mainly on the problem of registering successive serial transmission electron micrographs of ultrathin sections of mouse liver cell nuclei to analyse the 3D chromatin structure. A five-step semiautomatic interactive registration method is proposed. The first two steps of the procedure correct the rotation and translation components by using the phase correlation. The third, fourth and fifth steps correct the global distortion, employing a point mapping method based on different ways of selecting the control points. In step three, the control points were automatically computed by phase correlating corresponding subimages of the reference and sensed image. A semiautomatic method is used in the fourth step to select the control points, i.e. an automated method for computing the centre of mass of manually identified anatomical structures in neighbouring slices. For the sections which could not be properly corrected by the four steps, a final step is introduced, where control points are manually selected in the reference and sensed images. An algorithm is proposed to examine the spatial distribution of selected control points. Four sets of serial sections of mouse liver cell nuclei, each with approximately 100 sections, are registered by the proposed method and also registered manually for the comparison of registration accuracy. Artificial X-Z and Z-Y sections of registered series were visually compared for the smoothness of the nuclear membrane. To quantify the registration accuracy and the extent of registration, the correlation coefficient (C) and the overlap index (Co) were computed over the registered structure of interest. In addition to the visual comparison and the comparison of C and Co, the registered serial sets were compared by 3D GLCM-based texture features in the Z direction. The results demonstrate that the proposed semiautomatic registration technique achieved accurate results comparable to the manual registration. The proposed registration method relies only on the operator for rough pinpointing of cellular structures. Therefore, it should provide better reproducibility, and allow the user to operate the system faster and in a more relaxed manner than in a manual registration.

摘要

生物组织的图像配准对于三维重建至关重要,而三维重建对于可视化和量化物体内部结构之间的三维关系非常重要。DNA组织的生物学作用是细胞核内极其复杂的三维结构,自从明确染色质结构本身作为DNA的调节因子以来,它已成为焦点。因此,基于连续系列高分辨率超薄切片的细胞核三维重建可能会提供有关染色质结构及其在癌变过程中组织变化的新信息。这项工作主要关注对小鼠肝细胞核超薄切片的连续系列透射电子显微镜图像进行配准的问题,以分析三维染色质结构。提出了一种五步半自动交互式配准方法。该过程的前两步通过使用相位相关来校正旋转和平移分量。第三步、第四步和第五步采用基于不同控制点选择方式的点映射方法来校正全局失真。在第三步中,通过对参考图像和感测图像的相应子图像进行相位相关自动计算控制点。第四步使用半自动方法选择控制点,即一种用于计算相邻切片中手动识别的解剖结构质心的自动方法。对于无法通过这四个步骤正确校正的切片,引入了最后一步,即在参考图像和感测图像中手动选择控制点。提出了一种算法来检查所选控制点的空间分布。通过所提出的方法对四组小鼠肝细胞核连续切片进行配准,每组约100个切片,并且也进行手动配准以比较配准精度。对配准系列的人工X-Z和Z-Y切片进行视觉比较以观察核膜的平滑度。为了量化配准精度和配准程度,在感兴趣的配准结构上计算相关系数(C)和重叠指数(Co)。除了视觉比较以及C和Co的比较之外,还通过基于三维灰度共生矩阵的Z方向纹理特征对配准的连续集进行比较。结果表明,所提出的半自动配准技术取得了与手动配准相当的准确结果。所提出的配准方法仅依赖操作员对细胞结构进行粗略定位。因此,它应该具有更好的可重复性,并且与手动配准相比,允许用户更快且更轻松地操作该系统。

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