乳腺癌中用于实时逆转录聚合酶链反应数据标准化的基因鉴定

Identification of genes for normalization of real-time RT-PCR data in breast carcinomas.

作者信息

Lyng Maria B, Laenkholm Anne-Vibeke, Pallisgaard Niels, Ditzel Henrik J

机构信息

Department of Pathology, Odense University Hospital, Odense, Denmark.

出版信息

BMC Cancer. 2008 Jan 22;8:20. doi: 10.1186/1471-2407-8-20.

DOI:10.1186/1471-2407-8-20

PMID:18211679

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2248196/

Abstract

BACKGROUND

Quantitative real-time RT-PCR (RT-qPCR) has become a valuable molecular technique in basic and translational biomedical research, and is emerging as an equally valuable clinical tool. Correlation of inter-sample values requires data normalization, which can be accomplished by various means, the most common of which is normalization to internal, stably expressed, reference genes. Recently, such traditionally utilized reference genes as GAPDH and B2M have been found to be regulated in various circumstances in different tissues, emphasizing the need to identify genes independent of factors influencing the tissue, and that are stably expressed within the experimental milieu. In this study, we identified genes for normalization of RT-qPCR data for invasive breast cancer (IBC), with special emphasis on estrogen receptor positive (ER+) IBC, but also examined their applicability to ER- IBC, normal breast tissue and breast cancer cell lines.

METHODS

The reference genes investigated by qRT-PCR were RPLP0, TBP, PUM1, ACTB, GUS-B, ABL1, GAPDH and B2M. Biopsies of 18 surgically-excised tissue specimens (11 ER+ IBCs, 4 ER- IBCs, 3 normal breast tissues) and 3 ER+ cell lines were examined and the data analyzed by descriptive statistics, geNorm and NormFinder. In addition, the expression of selected reference genes in laser capture microdissected ER+ IBC cells were compared with that of whole-tissue.

RESULTS

A group of 3 genes, TBP, RPLP0 and PUM1, were identified for both the combined group of human tissue samples (ER+ and ER- IBC and normal breast tissue) and for the invasive cancer samples (ER+ and ER- IBC) by GeNorm, where NormFinder consistently identified PUM1 at the single best gene for all sample combinations.

CONCLUSION

The reference genes of choice when performing RT-qPCR on normal and malignant breast specimens should be either the collected group of 3 genes (TBP, RPLP0 and PUM1) employed as an average, or PUM1 as a single gene.

摘要

背景

定量实时逆转录聚合酶链反应（RT-qPCR）已成为基础和转化生物医学研究中有价值的分子技术，并且正成为一种同样有价值的临床工具。样本间数值的相关性需要数据归一化，这可以通过多种方式实现，其中最常见的是以内在稳定表达的参考基因进行归一化。最近，诸如甘油醛-3-磷酸脱氢酶（GAPDH）和β2微球蛋白（B2M）等传统使用的参考基因已被发现在不同组织的各种情况下受到调控，这凸显了识别不受影响组织的因素影响且在实验环境中稳定表达的基因的必要性。在本研究中，我们鉴定了用于浸润性乳腺癌（IBC）的RT-qPCR数据归一化的基因，特别强调雌激素受体阳性（ER+）IBC，但也研究了它们在ER- IBC、正常乳腺组织和乳腺癌细胞系中的适用性。

方法

通过qRT-PCR研究的参考基因有核糖体蛋白L35A（RPLP0）、TATA盒结合蛋白（TBP）、Pumilio RNA结合家族成员1（PUM1）、肌动蛋白β（ACTB）、β-葡萄糖醛酸酶B（GUS-B）、Abelson鼠白血病病毒癌基因同源物1（ABL1）、GAPDH和B2M。对18个手术切除的组织标本（11个ER+ IBC、4个ER- IBC、3个正常乳腺组织）的活检样本和3个ER+细胞系进行检测，并通过描述性统计、geNorm和NormFinder软件对数据进行分析。此外，还比较了激光捕获显微切割的ER+ IBC细胞中选定参考基因的表达与全组织中的表达。

结果

通过geNorm软件鉴定出一组3个基因，即TBP、RPLP0和PUM1，适用于人类组织样本（ER+和ER- IBC以及正常乳腺组织）的组合组以及浸润性癌样本（ER+和ER- IBC），而NormFinder软件始终将PUM1确定为所有样本组合的最佳单一基因。

结论

对正常和恶性乳腺标本进行RT-qPCR时，首选的参考基因应为作为一个整体使用的3个基因组合（TBP、RPLP0和PUM1），或者单一基因PUM1。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a147/2248196/024465be29df/1471-2407-8-20-1.jpg

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Brain Res. 2007 Feb 9;1132(1):20-8. doi: 10.1016/j.brainres.2006.11.026. Epub 2006 Dec 26.

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乳腺癌中用于实时逆转录聚合酶链反应数据标准化的基因鉴定

Identification of genes for normalization of real-time RT-PCR data in breast carcinomas.

作者信息

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BACKGROUND

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