首页> 外文期刊>Analytical Biochemistry: An International Journal of Analytical and Preparative Methods >Gene expression analysis of interferon kappa in laser capture microdissected cervical epithelium
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Gene expression analysis of interferon kappa in laser capture microdissected cervical epithelium

机译:激光捕获显微切割宫颈上皮中干扰素κ的基因表达分析

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Optimal sample handling techniques for tissue preparation and storage, RNA extraction and quantification, and target gene detection are crucial for reliable gene expression analysis. Methods for measuring low-expressing genes, such as interferons, in human cervical samples are not described in the scientific literature. To detect interferon mRNA in human cervical samples we obtained normal and dysplastic frozen and formalin-fixed cervical biopsies from colposcopy. Histopathological diagnosis was performed by one pathologist. Cervical keratinocytes were isolated using laser Capture microdissection. Immortalized keratinocytes transduced with OF devoid of an HPV oncogene were used for initial method development. RNA from samples was extracted and integrity tested to compare tissue storage and extraction methods. The expression of five housekeeping genes was analyzed in cell lines and patient tissue to permit normalization between samples using quantitative real-time polymerase chain reaction. The usefulness of cDNA amplification was assessed for the detection of low-expressing interferon K in cervical tissue. Here we report optimal tissue storage conditions, RNA extraction, sample normalization, and transcript amplification, as well as the sensitivity of quantitative real-time polymerase chain reaction and laser capture microdissection, for interferon K detection in cervical tissue. Without these optimized techniques, interferon K detection Would be unattainable in cervical samples. (c) 2008 Elsevier Inc. All rights reserved.
机译:用于组织制备和存储,RNA提取和定量以及靶基因检测的最佳样品处理技术对于可靠的基因表达分析至关重要。科学文献中没有描述测量人宫颈样品中低表达基因(如干扰素)的方法。为了检测人类宫颈样本中的干扰素mRNA,我们从阴道镜获得了正常和异常增生的冷冻和福尔马林固定的宫颈活检组织。组织病理学诊断由一名病理学家进行。使用激光捕获显微切割术分离宫颈角质形成细胞。用缺乏HPV癌基因的OF转导的永生化角质形成细胞用于初始方法开发。从样品中提取RNA并进行完整性测试,以比较组织存储和提取方法。分析了五个管家基因在细胞系和患者组织中的表达,以允许使用定量实时聚合酶链反应在样品之间进行归一化。评估cDNA扩增在检测宫颈组织中低表达干扰素K方面的有用性。在这里,我们报告了宫颈癌组织中干扰素K检测的最佳组织储存条件,RNA提取,样品标准化和转录本扩增,以及定量实时聚合酶链反应和激光捕获显微切割的敏感性。如果没有这些优化的技术,在子宫颈样本中将无法获得干扰素K的检测。 (c)2008 Elsevier Inc.保留所有权利。

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