%0 Journal Article %1 darzacq2007dynamics %A Darzacq, X %A Shav-Tal, Y %A de Turris, V %A Brody, Y %A Shenoy, S M %A Phair, R D %A Singer, R H %D 2007 %J Nat Struct Mol Biol %K polymerase stochastic_transcription %N 9 %P 796-806 %R 10.1038/nsmb1280 %T In vivo dynamics of RNA polymerase II transcription %U http://www.ncbi.nlm.nih.gov/pubmed/17676063 %V 14 %X 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.

@article{darzacq2007dynamics, 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.}, added-at = {2010-05-06T20:55:39.000+0200}, author = {Darzacq, X and Shav-Tal, Y and de Turris, V and Brody, Y and Shenoy, S M and Phair, R D and Singer, R H}, biburl = {https://www.bibsonomy.org/bibtex/2452318a34040d337dcf5340cd0e2c0c7/peter.ralph}, description = {In vivo dynamics of RNA polymerase II transcriptio... [Nat Struct Mol Biol. 2007] - PubMed result}, doi = {10.1038/nsmb1280}, interhash = {d2fd73e72f500bb27b136a2e47937be2}, intrahash = {452318a34040d337dcf5340cd0e2c0c7}, journal = {Nat Struct Mol Biol}, keywords = {polymerase stochastic_transcription}, month = sep, number = 9, pages = {796-806}, pmid = {17676063}, timestamp = {2010-05-06T20:55:39.000+0200}, title = {{{\it In vivo}} dynamics of {RNA} polymerase {II} transcription}, url = {http://www.ncbi.nlm.nih.gov/pubmed/17676063}, volume = 14, year = 2007 }