Biological subtyping of early breast cancer: a study comparing RT-qPCR with immunohistochemistry

被引:0
作者
Ralph M. Wirtz
Harri Sihto
Jorma Isola
Päivi Heikkilä
Pirkko-Liisa Kellokumpu-Lehtinen
Päivi Auvinen
Taina Turpeenniemi-Hujanen
Sirkku Jyrkkiö
Sotiris Lakis
Kornelia Schlombs
Mark Laible
Stefan Weber
Sebastian Eidt
Ugur Sahin
Heikki Joensuu
机构
[1] STRATIFYER Molecular Pathology GmbH,Laboratory of Molecular Oncology, Translational Cancer Biology Program
[2] University of Helsinki,Laboratory of Cancer Biology
[3] Institute of Medical Technology,Department of Pathology, HUSLAB
[4] Helsinki University Hospital and Helsinki University,Department of Oncology
[5] Tampere University Hospital and University of Tampere,Cancer Center
[6] Kuopio University Hospital,Department of Oncology and Radiotherapy
[7] Oulu University Hospital,Department of Oncology
[8] Turku University Hospital,Department of Oncology
[9] BioNTech Diagnostics GmbH,undefined
[10] Acomed Statistik,undefined
[11] Institute of Pathology at the St-Elisabeth-Hospital,undefined
[12] Helsinki University Hospital and University of Helsinki,undefined
来源
Breast Cancer Research and Treatment | 2016年 / 157卷
关键词
Breast cancer; Molecular subtypes; Ki-67; Prediction; Immunohistochemistry; RT-qPCR;
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学科分类号
摘要
The biological subtype of breast cancer influences the selection of systemic therapy. Distinction between luminal A and B cancers depends on consistent assessment of Ki-67, but substantial intra-observer and inter-observer variability exists when immunohistochemistry (IHC) is used. We compared RT-qPCR with IHC in the assessment of Ki-67 and other standard factors used in breast cancer subtyping. RNA was extracted from archival breast tumour tissue of 769 women randomly assigned to the FinHer trial. Cancer ESR1, PGR, ERBB2 and MKI67 mRNA content was quantitated with an RT-qPCR assay. Local pathologists assessed ER, PgR and Ki-67 expression using IHC. HER2 amplification was identified with chromogenic in situ hybridization (CISH) centrally. The results were correlated with distant disease-free survival (DDFS) and overall survival (OS). qPCR-based and IHC-based assessments of ER and PgR showed good concordance. Both low tumour MKI67 mRNA (RT-qPCR) and Ki-67 protein (IHC) levels were prognostic for favourable DDFS [hazard ratio (HR) 0.42, 95 % CI 0.25–0.71, P = 0.001; and HR 0.56, 0.37–0.84, P = 0.005, respectively] and OS. In multivariable analyses, cancer MKI67 mRNA content had independent influence on DDFS (adjusted HR 0.51, 95 % CI 0.29–0.89, P = 0.019) while Ki-67 protein expression had not any influence (P = 0.266) whereas both assessments influenced independently OS. Luminal B patients treated with docetaxel-FEC had more favourable DDFS and OS than those treated with vinorelbine-FEC when the subtype was defined by RT-qPCR (for DDFS, HR 0.52, 95 % CI 0.29–0.94, P = 0.031), but not when defined using IHC. Breast cancer subtypes approximated with RT-qPCR and IHC show good concordance, but cancer MKI67 mRNA content correlated slightly better with DDFS than Ki-67 expression. The findings based on MKI67 mRNA content suggest that patients with luminal B cancer benefit more from docetaxel-FEC than from vinorelbine-FEC.
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收藏
页码:437 / 446
页数:9
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