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Global analysis of the relationship between the binding of the Bas1p transcription factor and meiosis-specific double-strand DNA breaks in Saccharomyces cerevisiae

  • Piotr A. Mieczkowski
  • , Margaret Dominska
  • , Michael J. Buck
  • , Jennifer L. Gerton
  • , Jason D. Lieb
  • , Thomas D. Petes
  • University of North Carolina at Chapel Hill
  • Duke University
  • Stowers Institute for Medical Research

Research output: Contribution to journalArticlepeer-review

56 Scopus citations

Abstract

In the yeast Saccharomyces cerevisiae, certain genomic regions have very high levels of meiotic recombination (hot spots). The hot spot activity associated with the HIS4 gene requires the Bas1p transcription factor. To determine whether this relationship between transcription factor binding and hot spot activity is general, we used DNA microarrays to map all genomic Bas1p binding sites and to map the frequency of meiosis-specific double-strand DNA breaks (as an estimate of the recombination activity) of all genes in both wild-type and bas1 strains. We identified sites of Bas1p-DNA interactions upstream of 71 genes, many of which are involved in histidine and purine biosynthesis. Our analysis of recombination activity in wild-type and bas1 strains showed that the recombination activities of some genes with Bas1p binding sites were dependent on Bas1p (as observed for HIS4), whereas the activities of other genes with Bas1p binding sites were unaffected or were repressed by Bas1p. These data demonstrate that the effect of transcription factors on meiotic recombination activity is strongly context dependent. In wild-type and bas1 strains, meiotic recombination was strongly suppressed in large (25- to 150-kb) chromosomal regions near the telomeres and centromeres and in the region lanking the rRNA genes. These results argue that both local and regional factors affect the level of meiotic recombination.

Original languageEnglish
Pages (from-to)1014-1027
Number of pages14
JournalMolecular and Cellular Biology
Volume26
Issue number3
DOIs
StatePublished - Feb 2006

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