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Evaluation of global DNA hypomethylation in human colon cancer tissues by immunohistochemistry and image analysis

机译:通过免疫组织化学和图像分析评估人类结肠癌组织中的整体DNA低甲基化

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摘要

BACKGROUND—Global hypomethylation of DNA is frequently observed in human tumours. This alteration is detected in early adenomas in colorectal tumorigenesis. Information is currently acquired after extraction of DNA from tissues, digestion with nucleases, and analysis by reverse phase chromatography, or treatment with restriction enzymes followed by gel electrophoresis analysis and Southern hybridisation with radiolabelled probes.
AIMS—The purpose of our work was to evaluate the global methylation status of DNA in malignant lesions without loosing the histopathological features of the samples.
PATIENTS—The investigation was performed on paired normal-tumour tissues from 13 patients undergoing surgical resection of colorectal adenocarcinomas.
METHODS—Antibodies raised against 5-methylcytidine can be used to label methyl rich regions in interphase nuclei. This technique was adapted to the study of paraffin embedded tissues and an immunohistochemical method was developed to assess the global methylation status of individual nuclei while preserving cell morphology and tissue architecture. Computer assisted quantification of the staining intensity was performed on malignant and normal zones of human colon tissues to test the correlation between the immunolabelling signal and the respective histological patterns observed.
RESULTS—Qualitative and quantitative differences were observed and measured between the normal and malignant part of each sample. Morphologically altered nuclei displayed densely labelled spots within faintly labelled areas whereas normal nuclei were darker and uniformly stained. Image analysis allowed calculation of the average integrated optical density of the nuclei in both types of tissues, demonstrating a constant and significantly lower intensity for the former type of cells.


>Keywords: colon adenocarcinoma; DNA hypomethylation; immunohistochemistry
机译:背景技术在人类肿瘤中经常观察到DNA的整体甲基化不足。在大肠肿瘤发生的早期腺瘤中检测到这种改变。从组织中提取DNA,用核酸酶消化,通过反相色谱法分析,或用限制性内切酶处理,然后进行凝胶电泳分析并用放射性标记探针进行Southern杂交后,目前可获得信息。
AIMS —我们工作的目的旨在评估恶性病变中DNA的整体甲基化状态,而不会失去样品的组织病理学特征。
患者—研究对象是13例接受结直肠腺癌手术切除的患者的正常肿瘤组织。 >方法—针对5-甲基胞嘧啶的抗体可用于标记相间核中富含甲基的区域。这项技术适用于石蜡包埋组织的研究,并开发了一种免疫组织化学方法来评估单个核的整体甲基化状态,同时保留细胞形态和组织结构。在人结肠组织的恶性和正常区域进行计算机辅助的染色强度定量,以测试免疫标记信号与观察到的各个组织学模式之间的相关性。
结果-观察并测量了正常人与人之间的定性和定量差异和每个样品的恶性部分。形态改变的核在淡淡标记的区域内显示密集标记的斑点,而正常核则更黑且均匀染色。图像分析可以计算两种组织中细胞核的平均整合光密度,从而表明前一种细胞的强度恒定且显着降低。



>关键字: 结肠腺癌; DNA低甲基化;免疫组化

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