Exploring DNA methylation changes in promoter, intragenic, and intergenic regions as early and late events in breast cancer formation.

BMC cancer 2015 Vol.15() p. 816

Rauscher GH, Kresovich JK, Poulin M, Yan L, Macias V, Mahmoud AM, Al-Alem U, Kajdacsy-Balla A, Wiley EL, Tonetti D, Ehrlich M

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Abstract

[BACKGROUND] Breast cancer formation is associated with frequent changes in DNA methylation but the extent of very early alterations in DNA methylation and the biological significance of cancer-associated epigenetic changes need further elucidation.

[METHODS] Pyrosequencing was done on bisulfite-treated DNA from formalin-fixed, paraffin-embedded sections containing invasive tumor and paired samples of histologically normal tissue adjacent to the cancers as well as control reduction mammoplasty samples from unaffected women. The DNA regions studied were promoters (BRCA1, CD44, ESR1, GSTM2, GSTP1, MAGEA1, MSI1, NFE2L3, RASSF1A, RUNX3, SIX3 and TFF1), far-upstream regions (EN1, PAX3, PITX2, and SGK1), introns (APC, EGFR, LHX2, RFX1 and SOX9) and the LINE-1 and satellite 2 DNA repeats. These choices were based upon previous literature or publicly available DNA methylome profiles. The percent methylation was averaged across neighboring CpG sites.

[RESULTS] Most of the assayed gene regions displayed hypermethylation in cancer vs. adjacent tissue but the TFF1 and MAGEA1 regions were significantly hypomethylated (p ≤0.001). Importantly, six of the 16 regions examined in a large collection of patients (105 - 129) and in 15-18 reduction mammoplasty samples were already aberrantly methylated in adjacent, histologically normal tissue vs. non-cancerous mammoplasty samples (p ≤0.01). In addition, examination of transcriptome and DNA methylation databases indicated that methylation at three non-promoter regions (far-upstream EN1 and PITX2 and intronic LHX2) was associated with higher gene expression, unlike the inverse associations between cancer DNA hypermethylation and cancer-altered gene expression usually reported. These three non-promoter regions also exhibited normal tissue-specific hypermethylation positively associated with differentiation-related gene expression (in muscle progenitor cells vs. many other types of normal cells). The importance of considering the exact DNA region analyzed and the gene structure was further illustrated by bioinformatic analysis of an alternative promoter/intron gene region for APC.

[CONCLUSIONS] We confirmed the frequent DNA methylation changes in invasive breast cancer at a variety of genome locations and found evidence for an extensive field effect in breast cancer. In addition, we illustrate the power of combining publicly available whole-genome databases with a candidate gene approach to study cancer epigenetics.

추출된 의학 개체 (NER)

유형영어 표현한국어 / 풀이UMLS CUI출처등장
해부 breast 유방 dict 4
시술 reduction mammoplasty 유방성형술 dict 2
시술 mammoplasty 유방성형술 dict 1
해부 LINE-1 scispacy 1
해부 muscle progenitor cells scispacy 1
해부 cells scispacy 1
해부 genome scispacy 1
해부 DNA scispacy 1
해부 tissue scispacy 1
약물 [CONCLUSIONS] scispacy 1
약물 [BACKGROUND] Breast cancer scispacy 1
질환 cancer DNA scispacy 1
질환 breast cancer C0006142
Malignant neoplasm of breast
scispacy 1
질환 tumor C0027651
Neoplasms
scispacy 1
질환 cancers C0006826
Malignant Neoplasms
scispacy 1
질환 cancer C0006826
Malignant Neoplasms
scispacy 1
질환 formalin-fixed scispacy 1
기타 women scispacy 1
기타 BRCA1 scispacy 1
기타 CD44 scispacy 1
기타 ESR1 scispacy 1
기타 GSTM2 scispacy 1
기타 GSTP1 scispacy 1
기타 MAGEA1 scispacy 1
기타 MSI1 scispacy 1
기타 NFE2L3 scispacy 1
기타 RASSF1A scispacy 1
기타 RUNX3 scispacy 1
기타 SIX3 scispacy 1
기타 TFF1 scispacy 1
기타 EN1 scispacy 1
기타 PAX3 scispacy 1
기타 PITX2 scispacy 1
기타 SGK1 scispacy 1
기타 APC scispacy 1
기타 EGFR scispacy 1
기타 LHX2 scispacy 1
기타 RFX1 scispacy 1
기타 SOX9 scispacy 1
기타 patients scispacy 1
기타 far-upstream EN1 scispacy 1

MeSH Terms

Adult; Aged; Breast Neoplasms; Computational Biology; CpG Islands; DNA Methylation; DNA, Intergenic; Databases, Genetic; Epigenesis, Genetic; Female; Gene Expression Regulation, Neoplastic; Histones; Humans; Middle Aged; Promoter Regions, Genetic; Sequence Analysis, DNA

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