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反转录定量 PCR 法比较新鲜冰冻与福尔马林固定石蜡包埋乳腺癌组织基因表达谱。

Comparison of gene expression profiling by reverse transcription quantitative PCR between fresh frozen and formalin-fixed, paraffin-embedded breast cancer tissues.

机构信息

Laboratory of Molecular Pathology and Oncology, Research Unit, Hospital Universitario La Paz, Madrid, Spain.

出版信息

Biotechniques. 2010 May;48(5):389-97. doi: 10.2144/000113388.

Abstract

Recent reports demonstrate the feasibility of quantifying gene expression by using RNA isolated from blocks of formalin-fixed, paraffin-embedded (FFPE) tumor tissue. The development of molecular tests for clinical use based on archival materials would be of great utility in the search for and validation of important genes or gene expression profiles. In this study, we compared the performance of different normalization strategies in the correlation of quantitative data between fresh frozen (FF) and FFPE samples and analyzed the parameters that characterize such correlation for each gene. Total RNA extracted from FFPE samples presented a shift in raw cycle threshold (Cq) values that can be explained by its extensive degradation. Proper normalization can compensate for the effects of RNA degradation in gene expression measurements. We show that correlation between normalized expression values is better for moderately to highly expressed genes whose expression varies significantly between samples. Nevertheless, some genes had no correlation. These genes should not be included in molecular tests for clinical use based on FFPE samples. Our results could serve as a guide when developing clinical diagnostic tests based on RT-qPCR analyses of FFPE tissues in the coming era of treatment decision-making based on gene expression profiling.

摘要

最近的报告表明,通过使用从福尔马林固定、石蜡包埋(FFPE)肿瘤组织块中分离的 RNA 来定量基因表达是可行的。基于存档材料开发用于临床的分子检测将非常有助于寻找和验证重要的基因或基因表达谱。在这项研究中,我们比较了不同标准化策略在新鲜冷冻(FF)和 FFPE 样本之间定量数据相关性中的性能,并分析了每个基因特征化这种相关性的参数。从 FFPE 样本中提取的总 RNA 呈现出原始循环阈值(Cq)值的偏移,这可以通过其广泛的降解来解释。适当的归一化可以补偿基因表达测量中 RNA 降解的影响。我们表明,对于中度至高度表达的基因,其表达在样本之间差异很大,归一化表达值之间的相关性更好。然而,有些基因没有相关性。这些基因不应该包含在基于 FFPE 样本的临床分子检测中。当在基于基因表达谱的治疗决策时代即将到来之际,基于 FFPE 组织的 RT-qPCR 分析开发临床诊断检测时,我们的结果可以作为指导。

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