Methylation profiling of ductal carcinoma in situ and its relationship to histopathological features

Jia Min B. Pang; Siddhartha Deb; Elena A. Takano; David J. Byrne; Nicholas Jene; Alice Boulghourjian; Anne Holliday; Ewan Millar; C. Soon Lee; Sandra A. O'Toole; Alexander Dobrovic; Stephen B. Fox

doi:10.1186/s13058-014-0423-9

Methylation profiling of ductal carcinoma in situ and its relationship to histopathological features

Jia Min B. Pang
, Siddhartha Deb
, Elena A. Takano
, David J. Byrne
, Nicholas Jene
, Alice Boulghourjian
, Anne Holliday
, Ewan Millar
, C. Soon Lee
, Sandra A. O'Toole
, Alexander Dobrovic
, Stephen B. Fox

School of Medicine

Peter Maccallum Cancer Centre
University of Melbourne
Garvan Institute of Medical Research
St. George Hospital
University of New South Wales
Western Sydney University
Royal Prince Alfred Hospital
The University of Sydney
Ludwig Institute for Cancer Research

Research output: Contribution to journal › Article › peer-review

23 Citations (Scopus)

Abstract

Introduction: DNA methylation is a well-studied biomarker in invasive breast cancer, but its role in ductal carcinoma in situ (DCIS) is less well characterized. The aims of this study are to assess the methylation profile in DCIS for a panel of well-characterized genes that are frequently methylated in breast cancer, to investigate the relationship of methylation with pathological features, and to perform a proof-of-principle study to evaluate the practicality of methylation as a biomarker in diagnostic DCIS material. Methods: Promoter CpG island methylation for a panel of 11 breast cancer-related genes was performed by methylation-sensitive high resolution melting (MS-HRM). Formalin-fixed, paraffin-embedded (FFPE) biopsies from 72 samples of pure DCIS (DCIS occurring in the absence of synchronous invasive carcinoma), 10 samples of mixed DCIS (DCIS adjacent to invasive carcinoma), and 18 samples of normal breast epithelium adjacent to a DCIS lesion were micro-dissected prior to DNA extraction. Results: Methylation was seen for all the tested genes except BRCA1. RASSF1A was the most frequently methylated gene (90% of DCIS samples) and its methylation was associated with comedo necrosis (p = 0.018). Cluster analysis based on the methylation profile revealed four groups, the highly methylated cluster being significantly associated with high nuclear grade, HER2 amplification, negative estrogen receptor (ER) a status, and negative progesterone receptor (PgR) status, (p = 0.038, p = 0.018, p < 0.001, p = 0.001, respectively). Methylation of APC (p = 0.017), CDH13 (p = 0.017), and RARβ (p < 0.001) was associated with negative ERa status. Methylation of CDH13 (p < 0.001), and RARβ (p = 0.001) was associated with negative PgR status. Methylation of APC (p = 0.013) and CDH13 (p = 0.026) was associated with high nuclear grade. Methylation of CDH13 (p = 0.009), and RARβ (p = 0.042) was associated with HER2-amplification. Conclusions: DNA methylation can be assessed in FFPE-derived samples using suitable methodologies. Methylation of a panel of genes that are known to be methylated in invasive breast cancer was able to classify DCIS into distinct groups and was differentially associated with phenotypic features in DCIS.

Original language	English
Article number	423
Journal	Breast Cancer Research
Volume	16
Issue number	1
DOIs	https://doi.org/10.1186/s13058-014-0423-9
Publication status	Published - 2014

Bibliographical note

Publisher Copyright:
© 2014 Pang et al.

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10.1186/s13058-014-0423-9

Cite this

@article{b32d46eefe0149c69eb992818cff6df2,

title = "Methylation profiling of ductal carcinoma in situ and its relationship to histopathological features",

abstract = "Introduction: DNA methylation is a well-studied biomarker in invasive breast cancer, but its role in ductal carcinoma in situ (DCIS) is less well characterized. The aims of this study are to assess the methylation profile in DCIS for a panel of well-characterized genes that are frequently methylated in breast cancer, to investigate the relationship of methylation with pathological features, and to perform a proof-of-principle study to evaluate the practicality of methylation as a biomarker in diagnostic DCIS material. Methods: Promoter CpG island methylation for a panel of 11 breast cancer-related genes was performed by methylation-sensitive high resolution melting (MS-HRM). Formalin-fixed, paraffin-embedded (FFPE) biopsies from 72 samples of pure DCIS (DCIS occurring in the absence of synchronous invasive carcinoma), 10 samples of mixed DCIS (DCIS adjacent to invasive carcinoma), and 18 samples of normal breast epithelium adjacent to a DCIS lesion were micro-dissected prior to DNA extraction. Results: Methylation was seen for all the tested genes except BRCA1. RASSF1A was the most frequently methylated gene (90\% of DCIS samples) and its methylation was associated with comedo necrosis (p = 0.018). Cluster analysis based on the methylation profile revealed four groups, the highly methylated cluster being significantly associated with high nuclear grade, HER2 amplification, negative estrogen receptor (ER) a status, and negative progesterone receptor (PgR) status, (p = 0.038, p = 0.018, p < 0.001, p = 0.001, respectively). Methylation of APC (p = 0.017), CDH13 (p = 0.017), and RARβ (p < 0.001) was associated with negative ERa status. Methylation of CDH13 (p < 0.001), and RARβ (p = 0.001) was associated with negative PgR status. Methylation of APC (p = 0.013) and CDH13 (p = 0.026) was associated with high nuclear grade. Methylation of CDH13 (p = 0.009), and RARβ (p = 0.042) was associated with HER2-amplification. Conclusions: DNA methylation can be assessed in FFPE-derived samples using suitable methodologies. Methylation of a panel of genes that are known to be methylated in invasive breast cancer was able to classify DCIS into distinct groups and was differentially associated with phenotypic features in DCIS.",

author = "Pang, \{Jia Min B.\} and Siddhartha Deb and Takano, \{Elena A.\} and Byrne, \{David J.\} and Nicholas Jene and Alice Boulghourjian and Anne Holliday and Ewan Millar and \{Soon Lee\}, C. and O'Toole, \{Sandra A.\} and Alexander Dobrovic and Fox, \{Stephen B.\}",

note = "Publisher Copyright: {\textcopyright} 2014 Pang et al.",

year = "2014",

doi = "10.1186/s13058-014-0423-9",

language = "English",

volume = "16",

journal = "Breast Cancer Research",

issn = "1465-5411",

publisher = "BioMed Central Ltd.",

number = "1",

}

TY - JOUR

T1 - Methylation profiling of ductal carcinoma in situ and its relationship to histopathological features

AU - Pang, Jia Min B.

AU - Deb, Siddhartha

AU - Takano, Elena A.

AU - Byrne, David J.

AU - Jene, Nicholas

AU - Boulghourjian, Alice

AU - Holliday, Anne

AU - Millar, Ewan

AU - Soon Lee, C.

AU - O'Toole, Sandra A.

AU - Dobrovic, Alexander

AU - Fox, Stephen B.

PY - 2014

Y1 - 2014

N2 - Introduction: DNA methylation is a well-studied biomarker in invasive breast cancer, but its role in ductal carcinoma in situ (DCIS) is less well characterized. The aims of this study are to assess the methylation profile in DCIS for a panel of well-characterized genes that are frequently methylated in breast cancer, to investigate the relationship of methylation with pathological features, and to perform a proof-of-principle study to evaluate the practicality of methylation as a biomarker in diagnostic DCIS material. Methods: Promoter CpG island methylation for a panel of 11 breast cancer-related genes was performed by methylation-sensitive high resolution melting (MS-HRM). Formalin-fixed, paraffin-embedded (FFPE) biopsies from 72 samples of pure DCIS (DCIS occurring in the absence of synchronous invasive carcinoma), 10 samples of mixed DCIS (DCIS adjacent to invasive carcinoma), and 18 samples of normal breast epithelium adjacent to a DCIS lesion were micro-dissected prior to DNA extraction. Results: Methylation was seen for all the tested genes except BRCA1. RASSF1A was the most frequently methylated gene (90% of DCIS samples) and its methylation was associated with comedo necrosis (p = 0.018). Cluster analysis based on the methylation profile revealed four groups, the highly methylated cluster being significantly associated with high nuclear grade, HER2 amplification, negative estrogen receptor (ER) a status, and negative progesterone receptor (PgR) status, (p = 0.038, p = 0.018, p < 0.001, p = 0.001, respectively). Methylation of APC (p = 0.017), CDH13 (p = 0.017), and RARβ (p < 0.001) was associated with negative ERa status. Methylation of CDH13 (p < 0.001), and RARβ (p = 0.001) was associated with negative PgR status. Methylation of APC (p = 0.013) and CDH13 (p = 0.026) was associated with high nuclear grade. Methylation of CDH13 (p = 0.009), and RARβ (p = 0.042) was associated with HER2-amplification. Conclusions: DNA methylation can be assessed in FFPE-derived samples using suitable methodologies. Methylation of a panel of genes that are known to be methylated in invasive breast cancer was able to classify DCIS into distinct groups and was differentially associated with phenotypic features in DCIS.

AB - Introduction: DNA methylation is a well-studied biomarker in invasive breast cancer, but its role in ductal carcinoma in situ (DCIS) is less well characterized. The aims of this study are to assess the methylation profile in DCIS for a panel of well-characterized genes that are frequently methylated in breast cancer, to investigate the relationship of methylation with pathological features, and to perform a proof-of-principle study to evaluate the practicality of methylation as a biomarker in diagnostic DCIS material. Methods: Promoter CpG island methylation for a panel of 11 breast cancer-related genes was performed by methylation-sensitive high resolution melting (MS-HRM). Formalin-fixed, paraffin-embedded (FFPE) biopsies from 72 samples of pure DCIS (DCIS occurring in the absence of synchronous invasive carcinoma), 10 samples of mixed DCIS (DCIS adjacent to invasive carcinoma), and 18 samples of normal breast epithelium adjacent to a DCIS lesion were micro-dissected prior to DNA extraction. Results: Methylation was seen for all the tested genes except BRCA1. RASSF1A was the most frequently methylated gene (90% of DCIS samples) and its methylation was associated with comedo necrosis (p = 0.018). Cluster analysis based on the methylation profile revealed four groups, the highly methylated cluster being significantly associated with high nuclear grade, HER2 amplification, negative estrogen receptor (ER) a status, and negative progesterone receptor (PgR) status, (p = 0.038, p = 0.018, p < 0.001, p = 0.001, respectively). Methylation of APC (p = 0.017), CDH13 (p = 0.017), and RARβ (p < 0.001) was associated with negative ERa status. Methylation of CDH13 (p < 0.001), and RARβ (p = 0.001) was associated with negative PgR status. Methylation of APC (p = 0.013) and CDH13 (p = 0.026) was associated with high nuclear grade. Methylation of CDH13 (p = 0.009), and RARβ (p = 0.042) was associated with HER2-amplification. Conclusions: DNA methylation can be assessed in FFPE-derived samples using suitable methodologies. Methylation of a panel of genes that are known to be methylated in invasive breast cancer was able to classify DCIS into distinct groups and was differentially associated with phenotypic features in DCIS.

UR - https://www.scopus.com/pages/publications/84988844510

U2 - 10.1186/s13058-014-0423-9

DO - 10.1186/s13058-014-0423-9

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C2 - 25331261

AN - SCOPUS:84988844510

SN - 1465-5411

VL - 16

JO - Breast Cancer Research

JF - Breast Cancer Research

IS - 1

M1 - 423

ER -

Methylation profiling of ductal carcinoma in situ and its relationship to histopathological features

Abstract

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