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首页> 外文期刊>Cellular Oncology: Analytical Cellular Pathology >Groping for Quantitative Digital 3-D Image Analysis: An Approach to Quantitative Fluorescence In Situ Hybridization in Thick Tissue Sections of Prostate Carcinoma
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Groping for Quantitative Digital 3-D Image Analysis: An Approach to Quantitative Fluorescence In Situ Hybridization in Thick Tissue Sections of Prostate Carcinoma

机译:定量数字3-D图像分析的探索:前列腺癌厚组织切片中定量荧光原位杂交的方法

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In molecular pathology numerical chromosome aberrations have been found to be decisive for the prognosis of malignancy in tumours. The existence of such aberrations can be detected by interphase fluorescence in situ hybridization (FISH). The gain or loss of certain base sequences in the desoxyribonucleic acid (DNA) can be estimated by counting the number of FISH signalsper cell nucleus. The quantitative evaluation of such events is a necessary condition for a prospective use in diagnostic pathology. To avoid occlusions of signals, the cell nucleus has to be analyzed in three dimensions. Confocal laser scanning microscopy is the means to obtain series of optical thin sections from fluorescence stained or marked material to fulfill the conditions mentioned above. A graphical user interface (GUI) to a software package for display, inspection, count and (semi‐)automatic analysis of 3‐D images for pathologists is outlined including the underlying methods of 3‐D image interaction and segmentation developed. The preparative methods are briefly described. Main emphasis is given to the methodical questions of computer‐aided analysis of large 3‐D image data sets for pathologists. Several automated analysis steps can be performed for segmentation and succeeding quantification. However tumour material is in contrast to isolated or cultured cells even for visual inspection, a difficult material. For the present a fully automated digital image analysis of 3‐D data is not in sight. A semi‐automatic segmentation method is thus presented here.
机译:在分子病理学中,已经发现数字染色体畸变对于肿瘤恶性的预后具有决定性作用。可以通过相间荧光原位杂交(FISH)检测这种像差的存在。脱氧核糖核酸(DNA)中某些碱基序列的得失可以通过计算每个细胞核的FISH信号数来估算。此类事件的定量评估是在诊断病理学中预期使用的必要条件。为了避免信号的阻塞,必须在三个维度上分析细胞核。共聚焦激光扫描显微镜是从荧光染色或标记材料中获得一系列光学薄片以满足上述条件的方法。概述了软件包的图形用户界面(GUI),以供病理学家显示,检查,计数和(半)自动分析3D图像,包括开发的3D图像交互和分割的基本方法。简要描述了制备方法。主要重点是针对病理学家的大型3D图像数据集的计算机辅助分析的方法性问题。可以执行几个自动分析步骤以进行细分和后续量化。然而,即使是目视检查,肿瘤材料也与分离或培养的细胞相反,这是一种困难的材料。目前,还没有3D数据的全自动数字图像分析。因此,这里提出了一种半自动分割方法。

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