Dynamic reorganization of the AC16 cardiomyocyte transcriptome in response to TNFα signaling revealed by integrated genomic analyses

Luo, Xin; Chae, Minho; Krishnakumar, Raga; Danko, Charles G.; Kraus, W. Lee

doi:10.1186/1471-2164-15-155

Cited by 37 publications

(46 citation statements)

References 65 publications

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“…These results suggest that the promoter activity of an enhancer across cells is a proxy of its enhancer activity. This conclusion is also supported by the observation that transcription at enhancers often changes in a stimulus-dependent manner [32][33][34][35][36] and correlates with changes in the transcriptional output of target genes [18,21], often with dynamics that match or precede gene activation [20,33,35] ( Figure 1B). …”

supporting

confidence: 53%

A unified architecture of transcriptional regulatory elements

2015

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Gene expression is precisely controlled in time and space through the integration of signals that act at gene promoters and gene-distal enhancers. Classically, promoters and enhancers are considered separate classes of regulatory elements, often distinguished by histone modifications. However, recent studies have revealed broad similarities between enhancers and promoters, blurring the distinction: active enhancers often initiate transcription, and some gene promoters have the potential to enhance transcriptional output of other promoters. Here, we propose a model in which promoters and enhancers are considered a single class of functional element, with a unified architecture for transcription initiation. The context of interacting regulatory elements and the surrounding sequences determine local transcriptional output as well as the enhancer and promoter activities of individual elements.

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supporting

confidence: 53%

A unified architecture of transcriptional regulatory elements

2015

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“…3B, C). Despite the fact that treatments involving Nutlin-3a, TNF, and estradiol are known to modulate gene expression Allen et al 2014;Luo et al 2014), we observed no detectable differences in MD-scores when considering only promoter-associated bidirectional transcript sites (Supplemental Fig. S15).…”

Section: −33mentioning

confidence: 75%

Enhancer RNA profiling predicts transcription factor activity

et al. 2018

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Transcription factors (TFs) exert their regulatory influence through the binding of enhancers, resulting in coordination of gene expression programs. Active enhancers are often characterized by the presence of short, unstable transcripts termed enhancer RNAs (eRNAs). While their function remains unclear, we demonstrate that eRNAs are a powerful readout of TF activity. We infer sites of eRNA origination across hundreds of publicly available nascent transcription data sets and show that eRNAs initiate from sites of TF binding. By quantifying the colocalization of TF binding motif instances and eRNA origins, we derive a simple statistic capable of inferring TF activity. In doing so, we uncover dozens of previously unexplored links between diverse stimuli and the TFs they affect.

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“…ChIP-seq library preparation ChIP-seq libraries were prepared from chromatin-immunoprecipitated DNA as described previously with some minor modifications (Luo et al 2014). The quality of the libraries was assessed using a D1000 ScreenTape on a 2200 TapeStation (Agilent) and quantified using a Qubit dsDNA HS assay kit (Thermo Fisher).…”

Section: Chip-seqmentioning

confidence: 99%

“…Preparation of GRO-seq libraries GRO-seq libraries were prepared as described previously with some minor modifications (Luo et al 2014). Library quality was assessed as described above for the ChIP-seq libraries and then sequenced on an Illumina HiSeq 2000 (single-end, 50-bp reads) for a total of ∼47 million raw reads per biological replicate.…”

Section: Gro-seqmentioning

confidence: 99%

Dynamic assembly and activation of estrogen receptor α enhancers through coregulator switching

Murakami

Nagari

Kraus³

2017

Genes Dev.

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Although many features of active transcriptional enhancers have been defined by genomic assays, we lack a clear understanding of the order of events leading to enhancer formation and activation as well as the dynamics of coregulator interactions within the enhancer complex. Here, we used selective loss-or gain-of-function mutants of estrogen receptor α (ERα) to define two distinct phases of ligand-dependent enhancer formation. In the first phase (0-20 min), p300 is recruited to ERα by Mediator as well as p300's acetylhistone-binding bromodomain to promote initial enhancer formation, which is not competent for sustained activation. In the second phase (20-45 min), p300 is recruited to ERα by steroid receptor coregulators (SRCs) for enhancer maturation and maintenance. Successful transition between these two phases ("coregulator switching") is required for proper enhancer function. Failure to recruit p300 during either phase leads to abortive enhancer formation and a lack of target gene expression. Our results reveal an ordered and cooperative assembly of ERα enhancers requiring functional interplay among p300, Mediator, and SRCs, which has implications for hormone-dependent gene regulation in breast cancers. More broadly, our results demonstrate the unexpectedly dynamic nature of coregulator interactions within enhancer complexes, which are likely to be a defining feature of all enhancers.

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Dynamic reorganization of the AC16 cardiomyocyte transcriptome in response to TNFα signaling revealed by integrated genomic analyses

Cited by 37 publications

References 65 publications

A unified architecture of transcriptional regulatory elements

A unified architecture of transcriptional regulatory elements

Enhancer RNA profiling predicts transcription factor activity

Dynamic assembly and activation of estrogen receptor α enhancers through coregulator switching

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