Abstract

I propose to study the mechanism of genetic recombination in E. coli using plasmid DNAs as recombination substrates. There are two pathways of plasmid recombination in E. coli. One pathway is blocked by mutations in the recA, recF andtopoisomerase I genes and is partially blocked by recB recC mutations. Recombination by this pathway can be stimulated when the plasmid substrates contain either of two classes of cloned DNA segments: one of which only act in cis and the other of which acts in trans. The second pathway is induced in recB recC strains by the sbcA mutation and is independent of recA or recF function. Derivatives of plasmids containing mutations which modify restriction endonuclease cleavage sites and inactivate either tetracycline resistance or ampicillin resistance genes have been constructed. These plasmids will be used in in vivo experiments to measure the rate of recombination, to study the mechanism of recombination and to assess the effects of recombination-deficient mutations on recombination. New recombination-deficient mutations affecting plasmid recombination will be isolated using a new screening procedure and mapped. The effect of these mutations on recombination will be determined. The recombination genes will be cloned to identify, overproduce and purify their gene products. The mechanism by which DNA sequences can stimulate plasmid recombination in cis will be studied and the active nucleotide sequence of these recombination hotspots will be determined. The mechanism by which some cloned DNA segments can stimulate plasmid recombination in trans will also be studied. Assays using plasmids to detect intragenic recombination and the recombination interconversion of plasmids and their circular oligomeric forms in vitro have been developed. Previously unidentified proteins involved in the plasmid recombination pathways will be purified and characterized using in vitro complementation assays and in vitro reconstitution assays. Studies on the mechanism of action of exonuclease VIII, a protein required for the sbcA-induced pathway, will be continued. The recombination pathways will be reconstituted with purified proteins to study the mechanism of plasmid recombination. The interaction between the purified recombination proteins and recombination hotspots will be studied in detail.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM026017-08
Application #
3273493
Study Section
(MG)
Project Start
1978-12-01
Project End
1986-11-30
Budget Start
1985-12-01
Budget End
1986-11-30
Support Year
8
Fiscal Year
1986
Total Cost
Indirect Cost

  Institution

Name
Dana-Farber Cancer Institute
Department
Type
DUNS #
149617367
City
Boston
State
MA
Country
United States
Zip Code
02115

  Publications

Liang, Jason; Li, Bin-Zhong; Tan, Alexander P et al. (2018) SUMO E3 ligase Mms21 prevents spontaneous DNA damage induced genome rearrangements. PLoS Genet 14:e1007250
Srivatsan, Anjana; Putnam, Christopher D; Kolodner, Richard D (2018) Analyzing Genome Rearrangements in Saccharomyces cerevisiae. Methods Mol Biol 1672:43-61
Nene, Rahul V; Putnam, Christopher D; Li, Bin-Zhong et al. (2018) Cdc73 suppresses genome instability by mediating telomere homeostasis. PLoS Genet 14:e1007170
Putnam, Christopher D; Kolodner, Richard D (2017) Pathways and Mechanisms that Prevent Genome Instability in Saccharomyces cerevisiae. Genetics 206:1187-1225
Putnam, Christopher D; Srivatsan, Anjana; Nene, Rahul V et al. (2016) A genetic network that suppresses genome rearrangements in Saccharomyces cerevisiae and contains defects in cancers. Nat Commun 7:11256
de Souza, Jorge E S; Fonseca, André F; Valieris, Renan et al. (2014) S-score: a scoring system for the identification and prioritization of predicted cancer genes. PLoS One 9:e94147
Putnam, Christopher D; Pallis, Katielee; Hayes, Tikvah K et al. (2014) DNA repair pathway selection caused by defects in TEL1, SAE2, and de novo telomere addition generates specific chromosomal rearrangement signatures. PLoS Genet 10:e1004277
Ragu, Sandrine; Dardalhon, Michèle; Sharma, Sushma et al. (2014) Loss of the thioredoxin reductase Trr1 suppresses the genomic instability of peroxiredoxin tsa1 mutants. PLoS One 9:e108123
Allen-Soltero, Stephanie; Martinez, Sandra L; Putnam, Christopher D et al. (2014) A saccharomyces cerevisiae RNase H2 interaction network functions to suppress genome instability. Mol Cell Biol 34:1521-34
Albuquerque, Claudio P; Wang, Guoliang; Lee, Nancy S et al. (2013) Distinct SUMO ligases cooperate with Esc2 and Slx5 to suppress duplication-mediated genome rearrangements. PLoS Genet 9:e1003670

Showing the most recent 10 out of 84 publications