In vivo dynamics of RNA polymerase II transcription

Darzacq, Xavier; Shav‐Tal, Yaron; Turris, Valeria de; Brody, Yehuda; Shenoy, Shailesh M.; Phair, Robert D.; Singer, Robert H.

doi:10.1038/nsmb1280

Cited by 613 publications

(716 citation statements)

References 61 publications

(87 reference statements)

Supporting

Mentioning

646

Contrasting

Order By: Relevance

“…First, we chose RPB1 (the largest subunit of Pol II) known to have stable interactions with chromatin (Kimura et al , 2002; Hieda et al , 2005; Boireau et al , 2007; Darzacq et al , 2007; Fromaget & Cook, 2007) and also highly dynamic nuclear factors, like the TFIID subunit TAF5 and the GTF TFIIB (Chen et al , 2002; Sprouse et al , 2008; de Graaf et al , 2010; Ihalainen et al , 2012). In addition, eGFP was used as a control for a freely diffusing protein that should exhibit no specific interactions with the nuclear environment.…”

Section: Resultsmentioning

confidence: 99%

Coactivators and general transcription factors have two distinct dynamic populations dependent on transcription

et al. 2017

View full text Add to dashboard Cite

SAGA and ATAC are two distinct chromatin modifying co‐activator complexes with distinct enzymatic activities involved in RNA polymerase II (Pol II) transcription regulation. To investigate the mobility of co‐activator complexes and general transcription factors in live‐cell nuclei, we performed imaging experiments based on photobleaching. SAGA and ATAC, but also two general transcription factors (TFIID and TFIIB), were highly dynamic, exhibiting mainly transient associations with chromatin, contrary to Pol II, which formed more stable chromatin interactions. Fluorescence correlation spectroscopy analyses revealed that the mobile pool of the two co‐activators, as well as that of TFIID and TFIIB, can be subdivided into “fast” (free) and “slow” (chromatin‐interacting) populations. Inhibiting transcription elongation decreased H3K4 trimethylation and reduced the “slow” population of SAGA, ATAC, TFIIB and TFIID. In addition, inhibiting histone H3K4 trimethylation also reduced the “slow” populations of SAGA and ATAC. Thus, our results demonstrate that in the nuclei of live cells the equilibrium between fast and slow population of SAGA or ATAC complexes is regulated by active transcription via changes in the abundance of H3K4me3 on chromatin.

show abstract

Section: Resultsmentioning

confidence: 99%

Coactivators and general transcription factors have two distinct dynamic populations dependent on transcription

et al. 2017

View full text Add to dashboard Cite

show abstract

“…A major conclusion of this study is that cleavage/polyadenylation factors are maximally recruited at the 3′ pause 0.5-1.5 kb downstream of poly (A) sites. This downstream pause detected by ChIP may correspond to the pause in live cells detected by FRAP in the 3′ portion of a reporter gene 47 . The 3′ pause was normally followed by termination (Figs.…”

Section: Pausing Termination and Recruitment Of 3′ End Processing Fmentioning

confidence: 87%

RNA polymerase II pauses and associates with pre-mRNA processing factors at both ends of genes

Glover-Cutter

Kim

Espinosa

et al. 2007

Nat Struct Mol Biol

291

336

View full text Add to dashboard Cite

We investigated co-transcriptional recruitment of pre-mRNA processing factors to human genes. Capping factors associate with paused RNA pol II at the 5′ ends of quiescent genes. They also track throughout actively transcribed genes, and accumulate with paused polymerase in the 3′ flanking region. 3′ processing factors CstF and CPSF are maximally recruited 0.5-1.5 kb downstream of poly (A) sites where they coincide with capping factors, Spt5, and Ser2 hyperphosphorylated, paused pol II. 3′ end processing factors also localize at transcription start sites, and this early recruitment is enhanced after polymerase arrest with DRB. These results suggest that promoters may help specify recruitment of 3′ end processing factors. We propose a dual pausing model where elongation arrests near the transcription start site and in the 3′ flank to allow co-transcriptional processing by factors recruited to the pol II ternary complex.

show abstract

“…During transcriptional activation, the rate of oscillations is further reduced (“S” R1 converts into “ES”, (t/12 > 50 sec), possibly reflecting FGFR1 and RSK1 binding events and the formation of productive elongating complexes. The kinetics of RNA Polymerase II (RPII) are based on the methods of (Darzacq et al, 2007) and are similar to FGFR1. Close co‐localization of nFGFR1 and RNA Pol II is illustrated by immunostaining and super‐resolution microscopy in Video—Supplemental Material (collaborative experiment with Dr. Hari Shroff, NIH) l (Video 1).…”

Section: Nuclear Fgf Receptor‐1 and Creb Binding Protein—an Integratimentioning

confidence: 99%

Evidence‐Based Theory for Integrated Genome Regulation of Ontogeny—An Unprecedented Role of Nuclear FGFR1 Signaling

Stachowiak

2016

Journal Cellular Physiology

View full text Add to dashboard Cite

Genetic experiments have positioned the fgfr1 gene at the top of the gene hierarchy that governs gastrulation, as well as the subsequent development of the major body axes, nervous system, muscles, and bones, by affecting downstream genes that control the cell cycle, pluripotency, and differentiation, as well as microRNAs. Studies show that this regulation is executed by a single protein, the nuclear isoform of FGFR1 (nFGFR1), which integrates signals from development‐initiating factors, such as retinoic acid (RA), and operates at the interface of genomic and epigenomic information. nFGFR1 cooperates with a multitude of transcriptional factors (TFs), and targets thousands of genes encoding for mRNAs, as well as miRNAs in top ontogenic networks. nFGFR1 binds to the promoters of ancient proto‐oncogenes and tumor suppressor genes, in addition to binding to metazoan morphogens that delineate body axes, and construct the nervous system, as well as mesodermal and endodermal tissues. The discovery of pan‐ontogenic gene programming by integrative nuclear FGFR1 signaling (INFS) impacts our understanding of ontogeny, as well as developmental pathologies, and holds new promise for reconstructive medicine, and cancer therapy. J. Cell. Physiol. 231: 1199–1218, 2016. © 2016 The Authors. Journal of Cellular Physiology published by Wiley Periodicals, Inc.

show abstract

In vivo dynamics of RNA polymerase II transcription

Cited by 613 publications

References 61 publications

Coactivators and general transcription factors have two distinct dynamic populations dependent on transcription

Coactivators and general transcription factors have two distinct dynamic populations dependent on transcription

RNA polymerase II pauses and associates with pre-mRNA processing factors at both ends of genes

Evidence‐Based Theory for Integrated Genome Regulation of Ontogeny—An Unprecedented Role of Nuclear FGFR1 Signaling

Contact Info

Product

Resources

About