Literature DB >> 25517091

Enhancer-core-promoter specificity separates developmental and housekeeping gene regulation.

Muhammad A Zabidi1, Cosmas D Arnold1, Katharina Schernhuber1, Michaela Pagani1, Martina Rath1, Olga Frank1, Alexander Stark1.   

Abstract

Gene transcription in animals involves the assembly of RNA polymerase II at core promoters and its cell-type-specific activation by enhancers that can be located more distally. However, how ubiquitous expression of housekeeping genes is achieved has been less clear. In particular, it is unknown whether ubiquitously active enhancers exist and how developmental and housekeeping gene regulation is separated. An attractive hypothesis is that different core promoters might exhibit an intrinsic specificity to certain enhancers. This is conceivable, as various core promoter sequence elements are differentially distributed between genes of different functions, including elements that are predominantly found at either developmentally regulated or at housekeeping genes. Here we show that thousands of enhancers in Drosophila melanogaster S2 and ovarian somatic cells (OSCs) exhibit a marked specificity to one of two core promoters--one derived from a ubiquitously expressed ribosomal protein gene and another from a developmentally regulated transcription factor--and confirm the existence of these two classes for five additional core promoters from genes with diverse functions. Housekeeping enhancers are active across the two cell types, while developmental enhancers exhibit strong cell-type specificity. Both enhancer classes differ in their genomic distribution, the functions of neighbouring genes, and the core promoter elements of these neighbouring genes. In addition, we identify two transcription factors--Dref and Trl--that bind and activate housekeeping versus developmental enhancers, respectively. Our results provide evidence for a sequence-encoded enhancer-core-promoter specificity that separates developmental and housekeeping gene regulatory programs for thousands of enhancers and their target genes across the entire genome.

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Year:  2014        PMID: 25517091      PMCID: PMC6795551          DOI: 10.1038/nature13994

Source DB:  PubMed          Journal:  Nature        ISSN: 0028-0836            Impact factor:   49.962


  44 in total

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Journal:  Development       Date:  2010-01       Impact factor: 6.868

3.  Hormone-responsive enhancer-activity maps reveal predictive motifs, indirect repression, and targeting of closed chromatin.

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5.  Promoter specificity mediates the independent regulation of neighboring genes.

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7.  Switching of the core transcription machinery during myogenesis.

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9.  A global change in RNA polymerase II pausing during the Drosophila midblastula transition.

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10.  Global analysis of patterns of gene expression during Drosophila embryogenesis.

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  171 in total

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3.  CRISPR/Cas9-Mediated Scanning for Regulatory Elements Required for HPRT1 Expression via Thousands of Large, Programmed Genomic Deletions.

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4.  Genome-wide quantification of the effects of DNA methylation on human gene regulation.

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Review 5.  Towards a comprehensive catalogue of validated and target-linked human enhancers.

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6.  Suppression of Enhancer Overactivation by a RACK7-Histone Demethylase Complex.

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7.  The Pioneer Transcription Factor FoxA Maintains an Accessible Nucleosome Configuration at Enhancers for Tissue-Specific Gene Activation.

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Review 8.  Architectural proteins, transcription, and the three-dimensional organization of the genome.

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Review 9.  Eukaryotic enhancers: common features, regulation, and participation in diseases.

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