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首页> 外文OA文献 >Comparison of the QuantiGene 2.0 assay and real-time RT-PCR in the detection of p53 isoform mRNA expression in formalin-fixed paraffin-embedded tissues- a preliminary study
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Comparison of the QuantiGene 2.0 assay and real-time RT-PCR in the detection of p53 isoform mRNA expression in formalin-fixed paraffin-embedded tissues- a preliminary study

机译:在福尔马林固定石蜡包埋的组织中检测QuantiGene 2.0分析和实时RT-PCR在检测p53亚型mRNA表达方面的比较-初步研究

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p53 is expressed as multiple smaller isoforms whose functions in cancer are not well understood. The p53 isoforms demonstrate abnormal expression in different cancers, suggesting they are important in modulating the function of full-length p53 (FLp53). The quantification of relative mRNA expression has routinely been performed using real-time PCR (qPCR). However, there are serious limitations when detecting p53 isoforms using this method, particularly for formalin-fixed paraffin-embedded (FFPE) tissues. The use of FFPE tumours would be advantageous to correlate expression of p53 isoforms with important clinical features of cancer. One alternative method of RNA detection is the hybridization-based QuantiGene 2.0 Assay, which has been shown to be advantageous for the detection of RNA from FFPE tissues. In this pilot study, we compared the QuantiGene 2.0 Assay to qPCR for the detection of FLp53 and its isoform Δ40p53 in matched fresh frozen (FF) and FFPE breast tumours. FLp53 mRNA expression was detected using qPCR in FF and FFPE tissues, but Δ40p53 mRNA was only detectable in FF tissues. Similar results were obtained for the QuantiGene 2.0 Assay. FLp53 relative mRNA expression was shown to be strongly correlated between the two methods (R² = 0.9927, p = 0.0031) in FF tissues, however Δ40p53 was not (R² = 0.4429, p = 0.3345). When comparing the different methods for the detection of FLp53 mRNA from FFPE and FF samples, no correlation (R² = 0.0002, p = 0.9863) was shown using the QuantiGene 2.0 Assay, and in contrast, the level of expression was highly correlated between the two tissues using qPCR (R² = 0.8753, p = 0.0644). These results suggest that both the QuantiGene 2.0 Assay and qPCR methods are inadequate for the quantification of Δ40p53 mRNA in FFPE tissues. Therefore, alternative methods of RNA detection and quantification are required to study the relative expression of Δ40p53 in FFPE samples.
机译:p53被表达为多种较小的同工型,其在癌症中的功能尚不清楚。 p53亚型在不同的癌症中表现出异常表达,表明它们在调节全长p53(FLp53)的功能中很重要。相对mRNA表达的定量通常使用实时PCR(qPCR)进行。但是,使用这种方法检测p53异构体时存在严重的局限性,特别是对于福尔马林固定的石蜡包埋(FFPE)组织。 FFPE肿瘤的使用将有利于将p53亚型的表达与癌症的重要临床特征相关联。 RNA检测的另一种方法是基于杂交的QuantiGene 2.0分析法,该方法已显示出对从FFPE组织中检测RNA的优势。在这项初步研究中,我们将QuantiGene 2.0分析法与qPCR进行了比较,以检测匹配的新鲜冷冻(FF)和FFPE乳腺肿瘤中的FLp53及其同工型Δ40p53。使用qPCR在FF和FFPE组织中检测到FLp53 mRNA表达,但仅在FF组织中检测到Δ40p53mRNA。 QuantiGene 2.0分析获得了相似的结果。在FF组织中,两种方法之间的FLp53相对mRNA表达高度相关(R 2 = 0.9927,p = 0.0031),而Δ40p53则没有(R 2 = 0.4429,p = 0.3345)。当比较从FFPE和FF样品中检测FLp53 mRNA的不同方法时,使用QuantiGene 2.0分析没有发现相关性(R²= 0.0002,p = 0.9863),相比之下,两者之间的表达水平高度相关使用qPCR检测组织(R 2 = 0.8753,p = 0.0644)。这些结果表明,QuantiGene 2.0分析法和qPCR方法均不足以定量FFPE组织中的Δ40p53mRNA。因此,需要其他的RNA检测和定量方法来研究FFPE样品中Δ40p53的相对表达。

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