Breakfast Club Seminar Series

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Event Details
Contact

Colly Mitchell

Summaries

Summary Sentence: ""Mechanisms of RNA-driven DNA Modification and Repair"" - Francesca Storici, PhD - Assistant Professor, School of Biology

Full Summary: The IBB Breakfast Club seminar series was started with the spirit of the Institute's interdisciplinary mission in mind and started to feature local IBB faculty member's research in a seminar format. Faculty are often asked to speak at other universities and conferences, but rarely present at their home institution, this seminar series is an attempt to close that gap. The IBB Breakfast Club is open to anyone in the bio-community.

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  • Francesca Storici, PhD - Assistant Professor, School of Biology Francesca Storici, PhD - Assistant Professor, School of Biology
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  • Breakfast Club Seminar Series Breakfast Club Seminar Series
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"Mechanisms of RNA-driven DNA Modification and Repair"

Francesca Storici, PhD

Assistant Professor
School of Biology

As we have recently demonstrated in yeast Saccharomyces cerevisiae cells, short ribonucleoside monophosphate (rNMP) tracts carried within DNA oligonucleotides (oligos) can serve as templates for DNA synthesis at the chromosomal level and transfer a genetic change. The capacity of RNA to directly modify genomic DNA was also found in the bacterium Escherichia coli and in human embryonic kidney (HEK-293) cells, thus suggesting that the phenomenon is conserved. These findings stimulated two major avenues of research: i) to study how scattered ribonucleotides embedded in DNA can affect genome stability, and ii) how endogenous RNA transcripts can directly drive DNA modifications in cells.

With the goal of understanding to what extent rNMPs embedded in DNA may alter genome integrity and what factors affect their stability we developed oligo-driven gene correction assays in E. coli and S. cerevisiae. We showed that mispaired rNMPs embedded into genomic DNA, if not removed, serve as templates for DNA synthesis and can produce a genetic change. We demonstrated that RNase H type 2 can recognize single mispaired rNMPs embedded in DNA at the chromosomal level in both E. coli and S. cerevisiae cells. We found that the mismatch repair (MMR) system can remove mispairs of scattered rNMPs embedded in DNA both in yeast and E. coli cells and that instead a mismatch within an RNA-DNA heteroduplex region required RNase H type 1 for removal. Our data revealed overlapping activity between the MMR system and RNase H type 2 in processing the RNA/DNA mispairs. In the absence of mismatch repair and RNases H, ribonucleotide-driven gene modification increased by a factor of ~50 in yeast and 77,000 in E. coli.

In order to determine the capacity of an RNA transcript to directly serve as a template for chromosomal DNA modifications, we developed two assays in yeast. An RNA transcript was tested to repair a chromosomal double-strand break (DSB) generated either in the DNA from which the transcript itself originated or in an ectopic DNA locus homologous to the transcript. Data will be shown revealing the capacity of an RNA transcript to efficiently repair a DSB in its own DNA.
 



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Additional Information

In Campus Calendar
Yes
Groups

Parker H. Petit Institute for Bioengineering and Bioscience (IBB)

Invited Audience
No audiences were selected.
Categories
Seminar/Lecture/Colloquium
Keywords
BK Club, Breakfast Club Seminar Series, Francesca Storici, IBB, Mechanisms of RNA-driven DNA Modification and Repair
Status
  • Created By: Colly Mitchell
  • Workflow Status: Published
  • Created On: Jul 16, 2012 - 6:11am
  • Last Updated: Oct 7, 2016 - 9:59pm