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GENE EXPRESSION PROFILING IN BREAST CANCER BY SRPP METHOD

机译:SRPP方法在乳腺癌中的基因表达分析

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Background : Gene expression profiling has provided us with insight into the prognostic of breast cancer and led to the development of molecular gene signature models designed to aid in clinical decision-making. We sought to develop a quantitative analysis of the relative expression levels of a target gene from tumor tissues and normal tissues in a single assay. Methods: Sequence-tagged reverse-transcription polymerase chain reaction coupled with pyrosequencing (SRPP) was used for comparing prognostic gene relative expression levels in breast tumor. In the pyrogram, the sequence represents the gene source and the peak intensity represents the relative expression level of the gene in corresponding source.Results:The expression levels of ten kinds of prognostic marker genes (AL080059, MMP9, EXT1, ORC6L, AF052162, C9orf30, FBXO31, IGFBP5, ESM1 and RUNDC1) among the breast tumor tissues and normal tissues in the patients were accurately detected (n=3). The accuracy of SRPP was contrasted to the result of real-time PCR (n=3).Conclusions: The results show that SRPP method is reliable and reproducible in quantitatively comparing gene expression levels among different sources at a low cost. It can be apply to the prognostic gene relative expression assay in breast cancer.
机译:背景:基因表达分析已经为我们提供了洞察乳腺癌的预后,并导致了旨在帮助临床决策的分子基因特征模型的发展。我们寻求从单一测定中的肿瘤组织和正常组织的靶基因的相对表达水平进行定量分析。方法:用焦磷酸酶(SRPP)偶联的序列标记的逆转录聚合酶链反应比较乳腺肿瘤中的预后基因相对表达水平。在曲面图中,序列表示基因源,峰值强度表示相应来源中基因的相对表达水平。结果:十种预后标记基因的表达水平(Al080059,MMP9,EXT1,ORC6L,AF052162,C9ORF30在乳腺肿瘤组织和患者的正常组织中,FBXO31,IGFBP5,ESM1和RONDC1被精确地检测到(n = 3)。 SRPP的准确性与实时PCR(n = 3)的结果形成对比:结果表明,SRPP方法可靠且可再现,以以低成本定量比较不同来源之间的基因表达水平。它可以应用于乳腺癌中的预后基因相对表达测定。

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