The distribution of active RNA polymerase II along the transcribed region is gene-specific and controlled by elongation factors

Rodríguez-Gil A, García-Martínez J, Pelechano V, Muñoz-Centeno MdlC, Geli V, Pérez-Ortín JE, Chávez S

Nucleic Acids Res. 38 (14) 4651-4664 [2010-08-00; online 2010-04-10]

In order to study the intragenic profiles of active transcription, we determined the relative levels of active RNA polymerase II present at the 3'- and 5'-ends of 261 yeast genes by run-on. The results obtained indicate that the 3'/5' run-on ratio varies among the genes studied by over 12 log(2) units. This ratio seems to be an intrinsic characteristic of each transcriptional unit and does not significantly correlate with gene length, G + C content or level of expression. The correlation between the 3'/5' RNA polymerase II ratios measured by run-on and those obtained by chromatin immunoprecipitation is poor, although the genes encoding ribosomal proteins present exceptionally low ratios in both cases. We detected a subset of elongation-related factors that are important for maintaining the wild-type profiles of active transcription, including DSIF, Mediator, factors related to the methylation of histone H3-lysine 4, the Bur CDK and the RNA polymerase II subunit Rpb9. We conducted a more detailed investigation of the alterations caused by rpb9Delta to find that Rpb9 contributes to the intragenic profiles of active transcription by influencing the probability of arrest of RNA polymerase II.

SciLifeLab Fellow

Vicent Pelechano

PubMed 20385590

DOI 10.1093/nar/gkq215

Crossref 10.1093/nar/gkq215


Publications 9.5.1