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      In vivo dynamics of RNA polymerase II transcription.

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          Abstract

          We imaged transcription in living cells using a locus-specific reporter system, which allowed precise, single-cell kinetic measurements of promoter binding, initiation and elongation. Photobleaching of fluorescent RNA polymerase II revealed several kinetically distinct populations of the enzyme interacting with a specific gene. Photobleaching and photoactivation of fluorescent MS2 proteins used to label nascent messenger RNAs provided sensitive elongation measurements. A mechanistic kinetic model that fits our data was validated using specific inhibitors. Polymerases elongated at 4.3 kilobases min(-1), much faster than previously documented, and entered a paused state for unexpectedly long times. Transcription onset was inefficient, with only 1% of polymerase-gene interactions leading to completion of an mRNA. Our systems approach, quantifying both polymerase and mRNA kinetics on a defined DNA template in vivo with high temporal resolution, opens new avenues for studying regulation of transcriptional processes in vivo.

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          Author and article information

          Journal
          Nat Struct Mol Biol
          Nature structural & molecular biology
          Springer Science and Business Media LLC
          1545-9993
          1545-9985
          Sep 2007
          : 14
          : 9
          Affiliations
          [1 ] Department of Anatomy and Structural Biology, Albert Einstein College of Medicine, Bronx, New York 10461, USA.
          Article
          nsmb1280 NIHMS799959
          10.1038/nsmb1280
          4942130
          17676063
          5daad802-ab3d-4efd-b2b9-85c1d1ba9c31
          History

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