Abstract

H2B ubiquitylation is carried out by Bre1p, an E3 ligase, along with an E2 conjugase, Rad6p. H2B ubiquitylation has been previously implicated in promoting the association of RNA polymerase II with the coding sequence of the active GAL1 gene, and hence transcriptional elongation. Intriguingly, we find here that the association of RNA polymerase II with the active GAL1 coding sequence is not decreased in Δbre1, although it is required for H2B ubiquitylation. In contrast, the loss of Rad6p significantly impairs the association of RNA polymerase II with GAL1. Likewise, the point mutation of lysine 123 (ubiquitylation site) to arginine of H2B (H2B-K123R) also lowers the association of RNA polymerase II with GAL1, consistent with the role of H2B ubiquitylation in promoting RNA polymerase II association. Surprisingly, unlike the Δrad6 and H2B-K123R strains, complete deletion of BRE1 does not impair the association of RNA polymerase II with GAL1. However, deletion of the RING domain of Bre1p (that is essential for H2B ubiquitylation) impairs RNA polymerase II association with GAL1. These results imply that a non-RING domain of Bre1p counteracts the stimulatory role of the RING domain in regulating the association of RNA polymerase II with GAL1, and hence RNA polymerase II occupancy is not impaired in Δbre1. Consistently, GAL1 transcription is impaired in the absence of the RING domain of Bre1p, but not in Δbre1. Similar results are also obtained at other genes. Collectively, our results implicate both the stimulatory and repressive roles of Bre1p in regulation of RNA polymerase II association with active genes (and hence transcription) in vivo.

Highlights

  • Bre1p is required for H2B ubiquitylation that promotes RNA polymerase II association with active genes, and transcription

  • We find that deletion of RAD6 significantly decreased the association of RNA polymerase II with the coding sequence of the GAL1 gene following transcriptional induction in galactose-containing growth medium (Fig. 1, A and B), consistent with the role of histone H2B ubiquitylation in transcriptional elongation (8 –12)

  • Because Bre1p is essential for histone H2B ubiquitylation [15, 16, 19], the association of RNA polymerase II with GAL1 would be impaired in the ⌬bre1 strain, similar to the results obtained in the ⌬rad6 and H2B-K123R mutant strains (Fig. 1, B and C)

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Summary

Background

Bre1p is required for H2B ubiquitylation that promotes RNA polymerase II association with active genes, and transcription. Deletion of the RING domain of Bre1p (that is essential for H2B ubiquitylation) impairs RNA polymerase II association with GAL1. Our results implicate both the stimulatory and repressive roles of Bre1p in regulation of RNA polymerase II association with active genes (and transcription) in vivo. We have demonstrated that the absence of histone H2B ubiquitylation in the histone H2B-K123R point mutant strain significantly impaired the association of RNA polymerase II with the coding sequence of the GAL1 gene following transcriptional induction [8]. Deletion of the RING domain of Bre1p significantly impairs the association of RNA polymerase II with GAL1, consistent with the role of histone H2B ubiquitylation in association of RNA polymerase II and transcription. This study unravels a hidden function of Bre1p in gene regulation

EXPERIMENTAL PROCEDURES
The abbreviations used are
RESULTS
DISCUSSION

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