Abstract

The induction and maintenance of the DNA damage response (DDR) plays a central role in protecting genome integrity, allowing cells more time to repair chromosomal double-strand breaks (DSBs) or to eliminate cells that fail to accomplish repair. In budding yeast, creation of a single DSB is sufficient to activate the Mec1 (ATR) and Tel1 (ATM) checkpoint protein kinases that both modify chromatin around the DSB and trigger a cascade of phosphorylations that result in the arrest of cell cycle progression prior to anaphase. This proposal investigates three major aspects of the checkpoint response: the activation and maintenance of the checkpoint, the modification of chromatin by formation of g-H2AX and - as we have discovered - g-H2B, and a synergistic interaction of the DDR with the Spindle Assembly Checkpoint that is responsible for the prolongation of the arrested state. In the first Aim, how Mec1-dependent G2/M cell cycle arrest is maintained will be investigated by studying newly-discovered mutations of phosphorylation sites on Mec1 that are required to turn the checkpoint off; consequently cells fail to adapt and resume mitosis after 12-15 h when there is no DSB repair. How Mec1 monitors the presence of DNA damage will be examined, focusing on the relation between 5' to 3' resection of the DSB ends by exonucleases and maintenance of the checkpoint. Previous results suggest that the ability of cells to resume cell cycle progression after a DSB is repaired depends on how long cells have been arrested, which may correlate with the strength of the checkpoint signal. The strength of checkpoint signaling will be examined by augmenting the response by artificially tethering the Ddc1 and Ddc2 (ATRIP) activators of Mec1 to elicit a response independent of a DSB.
A second Aim will focus on the Mec1- and Tel1-dependent phosphorylation of the C-terminus of histone H2B (g-H2B) that resembles the well-studied g- H2AX modification but appears to have separate roles in DNA damage signaling and repair.
A third Aim will focus on the synergy between the DNA damage checkpoint and the Spindle Assembly Checkpoint, following up our findings that deleting Mad2 shortens checkpoint arrest in wild type cells and suppresses the permanent arrest of adaptation-defective mutations and that this suppression can be mimicked by deleting the centromere on the chromosome suffering an unrepaired DSB.

Public Health Relevance

The DNA damage checkpoint plays a key role in preserving genome stability, guarding against the formation of chromosomal rearrangements characteristic of cancer cells. DNA damage provokes cell cycle arrest and the induction of efficient DNA repair processes through a cascade of post-translational protein modifications triggered by the ATM and ATR kinases. In budding yeast a single site-specific double-strand chromosome break is sufficient to trigger checkpoint arrest. Genetic and molecular biological approaches are used to learn how the checkpoint is activated, maintained and turned off. The remarkable conservation of the checkpoint pathways between yeast and humans then makes it possible to point to mechanisms that regulate the checkpoint in normal and cancer cells.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
4R01GM061766-16
Application #
9130180
Study Section
Molecular Genetics B Study Section (MGB)
Program Officer
Willis, Kristine Amalee
Project Start
2001-06-01
Project End
2017-08-31
Budget Start
2016-09-01
Budget End
2017-08-31
Support Year
16
Fiscal Year
2016
Total Cost
Indirect Cost

  Institution

Name
Brandeis University
Department
Biology
Type
Schools of Arts and Sciences
DUNS #
616845814
City
Waltham
State
MA
Country
United States
Zip Code

  Publications

Gallagher, Danielle N; Haber, James E (2018) Repair of a Site-Specific DNA Cleavage: Old-School Lessons for Cas9-Mediated Gene Editing. ACS Chem Biol 13:397-405
Botchkarev Jr, Vladimir V; Haber, James E (2018) Functions and regulation of the Polo-like kinase Cdc5 in the absence and presence of DNA damage. Curr Genet 64:87-96
Roy, Kevin R; Smith, Justin D; Vonesch, Sibylle C et al. (2018) Multiplexed precision genome editing with trackable genomic barcodes in yeast. Nat Biotechnol 36:512-520
Botchkarev Jr, Vladimir V; Garabedian, Mikael V; Lemos, Brenda et al. (2017) The budding yeast Polo-like kinase localizes to distinct populations at centrosomes during mitosis. Mol Biol Cell 28:1011-1020
Eapen, Vinay V; Waterman, David P; Bernard, Amélie et al. (2017) A pathway of targeted autophagy is induced by DNA damage in budding yeast. Proc Natl Acad Sci U S A 114:E1158-E1167
Klionsky, Daniel J (see original citation for additional authors) (2016) Guidelines for the use and interpretation of assays for monitoring autophagy (3rd edition). Autophagy 12:1-222
Jain, Suvi; Sugawara, Neal; Haber, James E (2016) Role of Double-Strand Break End-Tethering during Gene Conversion in Saccharomyces cerevisiae. PLoS Genet 12:e1005976
Tsabar, Michael; Haase, Julian; Harrison, Benjamin et al. (2016) A Cohesin-Based Partitioning Mechanism Revealed upon Transcriptional Inactivation of Centromere. PLoS Genet 12:e1006021
Tsabar, Michael; Hicks, Wade M; Tsaponina, Olga et al. (2016) Re-establishment of nucleosome occupancy during double-strand break repair in budding yeast. DNA Repair (Amst) 47:21-29
Tsabar, Michael; Waterman, David P; Aguilar, Fiona et al. (2016) Asf1 facilitates dephosphorylation of Rad53 after DNA double-strand break repair. Genes Dev 30:1211-24

Showing the most recent 10 out of 59 publications