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Literature DB >> 34382191

Analysis of Enhancer-Promoter Interactions using CAGE and RADICL-Seq Technologies.

Alessandro Bonetti^1,2, Andrew Tae-Jun Kwon³, Erik Arner³, Piero Carninci^4,5.

Abstract

Regulation of gene expression is a key feature for higher eukaryotes and how chromatin topology relates to gene activation is an intense area of research. Enhancer-promoter interactions are believed to mediate activation of target genes. Bidirectional transcription represents one hallmark of active enhancers that can be measured using transcriptome technologies such as Cap analysis of gene expression (CAGE). Recently, we have developed RNA and DNA interacting complexes ligated and sequenced (RADICL-Seq) a novel methodology to map genome-wide RNA-chromatin interactions in intact nuclei. Here, we describe how CAGE and RADICL-Seq data can be used to characterize enhancer elements and identify their target genes.

Entities: Chemical

Keywords: Chromatin; Enhancer; Promoter; RNA; TSS

Mesh：

Substances：
Chromatin
RNA Caps

Year: 2021 PMID： 34382191 DOI： 10.1007/978-1-0716-1597-3_11

Source DB: PubMed Journal: Methods Mol Biol ISSN： 1064-3745

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Review 2. Methods for mapping 3D chromosome architecture.

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3. Environment drives selection and function of enhancers controlling tissue-specific macrophage identities.

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Journal: Cell Date: 2014-12-04 Impact factor: 41.582

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9. CAGEfightR: analysis of 5'-end data using R/Bioconductor.

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10. RADICL-seq identifies general and cell type-specific principles of genome-wide RNA-chromatin interactions.

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