Transfer of clinically relevant gene expression signatures in breast cancer: from Affymetrix microarray to Illumina RNA-Sequencing technology

被引:44
|
作者
Fumagalli, Debora [1 ]
Blanchet-Cohen, Alexis [2 ]
Brown, David [1 ]
Desmedt, Christine [1 ]
Gacquer, David [3 ]
Michiels, Stefan [4 ,5 ]
Rothe, Francoise [1 ]
Majjaj, Samira [1 ]
Salgado, Roberto [6 ]
Larsimont, Denis [7 ]
Ignatiadis, Michail [1 ]
Maetens, Marion [1 ]
Piccart, Martine [6 ]
Detours, Vincent [3 ]
Sotiriou, Christos
Haibe-Kains, Benjamin [1 ,8 ,9 ]
机构
[1] Inst Jules Bordet, Breast Canc Translat Res Lab BCTL, B-1000 Brussels, Belgium
[2] Inst Rech Clin Montreal, Bioinformat Core Fac, Montreal, PQ H2W 1R7, Canada
[3] Univ Libre Bruxelles, IRIBHM, Brussels, Belgium
[4] Inst Gustave Roussy, Dept Biostat & Epidemiol, Villejuif, France
[5] Univ Paris Sud, Paris, France
[6] Breast Int Grp, Brussels, Belgium
[7] Inst Jules Bordet, Dept Pathol, B-1000 Brussels, Belgium
[8] Univ Hlth Network, Princess Margaret Canc Ctr, Toronto, ON, Canada
[9] Univ Toronto, Dept Med Biophys, Toronto, ON, Canada
来源
BMC GENOMICS | 2014年 / 15卷
关键词
Breast cancer; Gene expression signatures; Affymetrix; Microarray; Illumina; RNA-Seq; Immunohistochemistry; Estrogen receptor; Progesterone receptor; HER2; receptor; AMERICAN SOCIETY; MOLECULAR PORTRAITS; SEQ; PROGNOSIS; PROFILES; ESTROGEN; RECOMMENDATIONS; CELLS; ONCOLOGY/COLLEGE; RECURRENCE;
D O I
10.1186/1471-2164-15-1008
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
Background: Microarrays have revolutionized breast cancer (BC) research by enabling studies of gene expression on a transcriptome wide scale. Recently, RNA-Sequencing (RNA-Seq) has emerged as an alternative for precise readouts of the transcriptome. To date, no study has compared the ability of the two technologies to quantify clinically relevant individual genes and microarray-derived gene expression signatures (GES) in a set of BC samples encompassing the known molecular BC's subtypes. To accomplish this, the RNA from 57 BCs representing the four main molecular subtypes (triple negative, HER2 positive, luminal A, luminal B), was profiled with Affymetrix HG-U133 Plus 2.0 chips and sequenced using the Illumina HiSeq 2000 platform. The correlations of three clinically relevant BC genes, six molecular subtype classifiers, and a selection of 21 GES were evaluated. Results: 16,097 genes common to the two platforms were retained for downstream analysis. Gene-wise comparison of microarray and RNA-Seq data revealed that 52% had a Spearman's correlation coefficient greater than 0.7 with highly correlated genes displaying significantly higher expression levels. We found excellent correlation between microarray and RNA-Seq for the estrogen receptor (ER; r(s) = 0.973; 95% CI: 0.971-0.975), progesterone receptor (PgR; r(s) = 0.95; 0.947-0.954), and human epidermal growth factor receptor 2 (HER2; r(s) = 0.918; 0.912-0.923), while a few discordances between ER and PgR quantified by immunohistochemistry and RNA-Seq/microarray were observed. All the subtype classifiers evaluated agreed well (Cohen's kappa coefficients >0.8) and all the proliferation-based GES showed excellent Spearman correlations between microarray and RNA-Seq (all r(s) >0.965). Immune-, stroma- and pathway-based GES showed a lower correlation relative to prognostic signatures (all r(s) >0.6). Conclusions: To our knowledge, this is the first study to report a systematic comparison of RNA-Seq to microarray for the evaluation of single genes and GES clinically relevant to BC. According to our results, the vast majority of single gene biomarkers and well-established GES can be reliably evaluated using the RNA-Seq technology.
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页数:12
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