학술논문
Integrative epigenomic and high-throughput functional enhancer profiling reveals determinants of enhancer heterogeneity in gastric cancer.
Document Type
Article
Author
Sheng, Taotao; Ho, Shamaine Wei Ting; Ooi, Wen Fong; Xu, Chang; Xing, Manjie; Padmanabhan, Nisha; Huang, Kie Kyon; Ma, Lijia; Ray, Mohana; Guo, Yu Amanda; Sim, Ngak Leng; Anene-Nzelu, Chukwuemeka George; Chang, Mei Mei; Razavi-Mohseni, Milad; Beer, Michael A.; Foo, Roger Sik Yin; Sundar, Raghav; Chan, Yiong Huak; Tan, Angie Lay Keng; Ong, Xuewen
Source
Subject
*CIS-regulatory elements (Genetics)
*SOMATIC mutation
*EPIGENOMICS
*STOMACH cancer
*GENETIC mutation
*CELL determination
*SINGLE nucleotide polymorphisms
*HETEROGENEITY
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Language
ISSN
1756-994X
Abstract
Background: Enhancers are distal cis-regulatory elements required for cell-specific gene expression and cell fate determination. In cancer, enhancer variation has been proposed as a major cause of inter-patient heterogeneity—however, most predicted enhancer regions remain to be functionally tested. Methods: We analyzed 132 epigenomic histone modification profiles of 18 primary gastric cancer (GC) samples, 18 normal gastric tissues, and 28 GC cell lines using Nano-ChIP-seq technology. We applied Capture-based Self-Transcribing Active Regulatory Region sequencing (CapSTARR-seq) to assess functional enhancer activity. An Activity-by-contact (ABC) model was employed to explore the effects of histone acetylation and CapSTARR-seq levels on enhancer-promoter interactions. Results: We report a comprehensive catalog of 75,730 recurrent predicted enhancers, the majority of which are GC-associated in vivo (> 50,000) and associated with lower somatic mutation rates inferred by whole-genome sequencing. Applying CapSTARR-seq to the enhancer catalog, we observed significant correlations between CapSTARR-seq functional activity and H3K27ac/H3K4me1 levels. Super-enhancer regions exhibited increased CapSTARR-seq signals compared to regular enhancers, even when decoupled from native chromatin contexture. We show that combining histone modification and CapSTARR-seq functional enhancer data improves the prediction of enhancer-promoter interactions and pinpointing of germline single nucleotide polymorphisms (SNPs), somatic copy number alterations (SCNAs), and trans-acting TFs involved in GC expression. We identified cancer-relevant genes (ING1, ARL4C) whose expression between patients is influenced by enhancer differences in genomic copy number and germline SNPs, and HNF4α as a master trans-acting factor associated with GC enhancer heterogeneity. Conclusions: Our results indicate that combining histone modification and functional assay data may provide a more accurate metric to assess enhancer activity than either platform individually, providing insights into the relative contribution of genetic (cis) and regulatory (trans) mechanisms to GC enhancer functional heterogeneity. [ABSTRACT FROM AUTHOR]