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Silenced yeast chromatin is maintained by Sir2 in preference to permitting histone acetylations for efficient NER

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journal contribution
posted on 2015-10-28, 11:41 authored by A. Irizar, Y. Yu, S. H. Reed, Edward John Louis, R. Waters
Very little is currently known about how nucleotide excision repair (NER) functions at the ends of chromosomes. To examine this, we introduced the URA3 gene into either transcriptionally active or repressed subtelomeric regions of the yeast genome. This enabled us to examine the repair of ultraviolet (UV)-induced cyclobutane pyrimidine dimers (CPDs) in identical sequences under both circumstances. We found that NER is significantly more efficient in the non-repressed subtelomere than the repressed one. At the non-repressed subtelomere, UV radiation stimulates both histones H3 and H4 acetylation in a similar fashion to that seen at other regions of the yeast genome. These modifications occur regardless of the presence of the Sir2 histone deacetylase. On the other hand, at the repressed subtelomere, where repair is much less efficient, UV radiation is unable to stimulate histone H4 or H3 acetylation in the presence of Sir2. In the absence of Sir2 both of these UV-induced modifications are detected, resulting in a significant increase in NER efficiency in the region. Our experiments reveal that there are instances in the yeast genome where the maintenance of the existing chromatin structures dominates over the action of chromatin modifications associated with efficient NER.

History

Citation

Nucleic Acids Res, 2010, 38 (14), pp. 4675-4686

Author affiliation

/Organisation/COLLEGE OF MEDICINE, BIOLOGICAL SCIENCES AND PSYCHOLOGY/MBSP Non-Medical Departments/Department of Genetics

Version

  • VoR (Version of Record)

Published in

Nucleic Acids Res

Publisher

Oxford University Press (OUP)

eissn

1362-4962

Acceptance date

2010-03-24

Copyright date

2010

Available date

2015-10-28

Publisher version

http://nar.oxfordjournals.org/content/38/14/4675

Language

en