Optimal reference genes for normalization of qRT-PCR data from archival formalin-fixed, paraffin-embedded breast tumors controlling for tumor cell content and decay of mRNA.

Trine Tramm, Brita S Sørensen, Jens Overgaard, Jan Alsner
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引用次数: 25

Abstract

Reliable determination of gene-expression levels from qRT-PCR requires accurate normalization of target genes to reference genes in order to remove nonbiological variation. Reference genes are ideally constitutively expressed in every cell, but many genes used for normalization has been shown to vary with tissue type, cellular proliferation, cancer progression, and degradation of nucleic acids. Gene-expression analysis is increasingly performed on degraded mRNA from formalin-fixed, paraffin-embedded tissue (FFPE), giving the option of examining retrospective cohorts. The aim of this study was to select robust reference genes showing stable expression over time in FFPE, controlling for various content of tumor tissue and decay of mRNA because of variable length of storage of the tissue. Sixteen reference genes were quantified by qRT-PCR in 40 FFPE breast tumor samples, stored for 1 to 29 years. Samples included 2 benign lesions and 38 carcinomas with varying tumor content. Stability of the reference genes were determined by the geNorm algorithm. mRNA was successfully extracted from all samples, and the 16 genes quantified in the majority of samples. Results showed 14% loss of amplifiable mRNA per year, corresponding to a half-life of 4.6 years. The 4 most stable expressed genes were CALM2, RPL37A, ACTB, and RPLP0. Several of the other examined genes showed considerably instability over time (GAPDH, PSMC4, OAZ1, IPO8). In conclusion, we identified 4 genes robustly expressed over time and independent of neoplastic tissue content in the FFPE block. Other widely used reference genes were concluded to be less suited for retrospective analysis of FFPE breast samples.

对福尔马林固定、石蜡包埋乳腺肿瘤档案中qRT-PCR数据归一化的最佳内参基因,控制肿瘤细胞含量和mRNA的衰减。
为了从qRT-PCR中可靠地确定基因表达水平,需要准确地将靶基因归一化为参考基因,以消除非生物学变异。理想情况下,内参基因在每个细胞中都是组成性表达的,但许多用于规范化的基因已被证明随着组织类型、细胞增殖、癌症进展和核酸降解而变化。基因表达分析越来越多地用于福尔马林固定石蜡包埋组织(FFPE)的降解mRNA,从而提供了回顾性队列检查的选择。本研究的目的是选择在FFPE中随时间稳定表达的健壮内参基因,控制肿瘤组织的各种含量和由于组织储存长度的变化而导致的mRNA的衰减。采用qRT-PCR对保存1 ~ 29年的40例FFPE乳腺肿瘤样本进行16个内参基因的定量分析。样本包括2个良性病变和38个不同肿瘤含量的癌。采用geNorm算法确定内参基因的稳定性。从所有样品中成功提取mRNA,并在大多数样品中定量了16个基因。结果显示,可扩增mRNA每年损失14%,半衰期为4.6年。最稳定表达的4个基因是CALM2、RPL37A、ACTB和RPLP0。其他几个被检测的基因(GAPDH、PSMC4、OAZ1、IPO8)随着时间的推移显示出相当大的不稳定性。总之,我们在FFPE块中发现了4个随着时间的推移而稳定表达且不依赖于肿瘤组织含量的基因。其他广泛使用的参考基因被认为不太适合FFPE乳腺样本的回顾性分析。
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>12 weeks
期刊介绍: Diagnostic Molecular Pathology focuses on providing clinical and academic pathologists with coverage of the latest molecular technologies, timely reviews of established techniques, and papers on the applications of these methods to all aspects of surgical pathology and laboratory medicine. It publishes original, peer-reviewed contributions on molecular probes for diagnosis, such as tumor suppressor genes, oncogenes, the polymerase chain reaction (PCR), and in situ hybridization. Articles demonstrate how these highly sensitive techniques can be applied for more accurate diagnosis.
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