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Space exploration by the promoter of a long human gene during one transcription cycle.

by: Joshua D. Larkin, Argyris Papantonis, Peter R. Cook, Davide Marenduzzo
Nucleic acids research (8 January 2013), doi:10.1093/nar/gks1441  Key: citeulike:11895180

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Abstract

An RNA polymerase has been thought to transcribe by seeking out a promoter, initiating and then tracking down the template. We add tumor necrosis factor α to primary human cells, switch on transcription of a 221-kb gene and monitor promoter position during the ensuing transcription cycle (using RNA fluorescence in situ hybridization coupled to super-resolution localization, chromosome conformation capture and Monte Carlo simulations). Results are consistent with a polymerase immobilized in a 'factory' capturing a promoter and reeling in the template, as the transcript and promoter are extruded. Initially, the extruded promoter is tethered close to the factory and so likely to re-initiate; later, the tether becomes long enough to allow re-initiation in another factory. We suggest close tethering underlies enhancer function and transcriptional 'bursting'.


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