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免疫荧光断层扫描:通过对甲基丙烯酸盐包埋组织进行连续切片和 2-D 免疫荧光图像的对齐实现高分辨率 3-D 重建。

Immunofluorescence Tomography: High-resolution 3-D reconstruction by serial-sectioning of methacrylate embedded tissues and alignment of 2-D immunofluorescence images.

机构信息

European Cancer Stem Cell Research Institute, Cardiff University, Maindy Rd, Cardiff, Wales, United Kingdom.

School of Optometry & Vision Sciences, Cardiff University, Maindy Rd, Cardiff, Wales, United Kingdom.

出版信息

Sci Rep. 2019 Feb 13;9(1):1992. doi: 10.1038/s41598-018-38232-9.

Abstract

Immunofluorescence tomography is a high-resolution 3-D reconstruction method based on methacrylate embedding and serial-sectioning, where 2-D images of immuno-stained serial-sections are computationally aligned into image stacks, and the 3-D volume rendered. Butyl-Methyl Methacrylate (BMMA) plastic was adopted as it preserves excellent tissue morphology and can be de-plasticized easily using an organic solvent, which enables immuno-staining of serial-sections without antibody penetration issues over millimeters of 3-D reconstructed tissue (Z-depth). High axial Z-resolution over a large volume was achieved by cutting serial-sections at 2 µm thickness. Stained sections were imaged by multiple modalities, including immunofluorescence, electron microscopy and second harmonic generation (SHG), and there are advantages over confocal microscopy as the tissue does not need to be cleared, while antibody penetration or light scattering issues are minimized. The plastic serial-sections can be re-probed, without a loss in tissue structure, using low pH glycine hydrochloride antibody elution. It is a cost-effective approach as the microscopes needed are significantly cheaper than confocal microscopes and sections can be kept indefinitely. Therefore, immunofluorescence tomography is a powerful new tool to quantify sub-populations of cells in high-resolution 3-D using antibody fluorescence. This article describes the immunofluorescence tomography method for 3-D reconstruction of epithelial tissues such as mammary gland, cornea and the hair follicle.

摘要

免疫荧光断层扫描是一种基于甲基丙烯酸酯包埋和连续切片的高分辨率 3D 重建方法,其中免疫染色的连续切片的 2D 图像通过计算进行配准成图像堆栈,并进行 3D 体积渲染。但采用丁基甲基甲基丙烯酸酯 (BMMA) 塑料,因为它可以很好地保存组织形态,并且可以很容易地使用有机溶剂进行去塑化,这使得可以对毫米级的 3D 重建组织(Z 深度)进行免疫染色,而不会出现抗体穿透问题。通过以 2μm 的厚度切割连续切片,实现了高轴向 Z 分辨率和大体积。通过多种模态对染色切片进行成像,包括免疫荧光、电子显微镜和二次谐波产生 (SHG),与共聚焦显微镜相比具有优势,因为组织不需要被清除,同时最小化了抗体穿透或光散射问题。塑料连续切片可以使用低 pH 甘氨酸盐酸盐抗体洗脱进行重新探测,而不会损失组织结构。这是一种具有成本效益的方法,因为所需的显微镜比共聚焦显微镜便宜得多,并且可以无限期保存切片。因此,免疫荧光断层扫描是一种强大的新工具,可使用抗体荧光对高分辨率 3D 中的细胞亚群进行定量。本文描述了用于重建乳腺、角膜和毛囊等上皮组织的 3D 免疫荧光断层扫描方法。

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