Abstract

Site-specific recombination systems are important in controlling such diverse processes such as plasmid maintenance, DNA amplification, chromosome segregation, movement of conjugative transposons and integration of genes in integrons. A long-range goal of this research is to understand how bacteriophage Lambda Int performs site-specific recombination. The findings will have a significant impact on other site-specific recombination systems that are members of the diverse Lambda Int family. Biochemical and genetic approaches will be used to characterize the protein-protein and protein-DNA interactions that occur both during the assembly of recombination complexes (intasomes) and the processes of strand cleavage and ligation. Int mutants will be characterized in assays that are designed to determine the defects of individual proteins in the recombination pathway. The host-encoded integration host factor (IHF) also participates in formation of intasomes by inducing bends in the DNA. We will crystallize mutant proteins that have expanded recognition specificities in order to understand how interactions of amino acids within the protein mediate recognition of DNA. Site-specific excision reactions are important for the spread of elements from one genome to another. We will analyze interactions of the excisionase (Xis) protein with INt and DNA. With the exception of phage Lambda (Xis) protein, little is known about how Xis proteins function during the excision reaction. In order to expand our understanding of excision reaction complexes and reactions, we plan to analyze the molecular mechanism of Xis function of page P22 Xis protein. Finally, we will initiate a project on the conjugative transposon CTnDOT. Our preliminary work indicates that although CTnDOT has an integrase that is related to the Lambda Int, it appears to have some mechanistic differences. We plan to develop an in vitro system to study the mechanism of strand exchange and the excision reaction catalyzed by the CTnDOT Int protein.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM028717-22
Application #
6519029
Study Section
Microbial Physiology and Genetics Subcommittee 2 (MBC)
Program Officer
Anderson, Richard A
Project Start
1980-12-01
Project End
2005-06-30
Budget Start
2002-07-01
Budget End
2003-06-30
Support Year
22
Fiscal Year
2002
Total Cost
$277,651
Indirect Cost

  Institution

Name
University of Illinois Urbana-Champaign
Department
Microbiology/Immun/Virology
Type
Schools of Arts and Sciences
DUNS #
041544081
City
Champaign
State
IL
Country
United States
Zip Code
61820

  Publications

Kolakowski, Adam J; Gardner, Jeffrey F (2016) The N-terminus of IntDOT forms hydrophobic interactions during Holliday Junction resolution. Plasmid 87-88:10-16
Wood, Margaret M; Gardner, Jeffrey F (2015) The Integration and Excision of CTnDOT. Microbiol Spectr 3:MDNA3-0020-2014
Ringwald, Kenneth; Gardner, Jeffrey (2015) The Bacteroides thetaiotaomicron protein Bacteroides host factor A participates in integration of the integrative conjugative element CTnDOT into the chromosome. J Bacteriol 197:1339-49
Hopp, Crystal M; Gardner, Jeffrey F; Salyers, Abigail A (2015) The Xis2d protein of CTnDOT binds to the intergenic region between the mob and tra operons. Plasmid 81:63-71
Keeton, Carolyn M; Park, Jiyeon; Wang, Gui-Rong et al. (2013) The excision proteins of CTnDOT positively regulate the transfer operon. Plasmid 69:172-9
Laprise, Jennifer; Yoneji, Sumiko; Gardner, Jeffrey F (2013) IntDOT interactions with core sites during integrative recombination. J Bacteriol 195:1883-91
Keeton, Carolyn M; Hopp, Crystal M; Yoneji, Sumiko et al. (2013) Interactions of the excision proteins of CTnDOT in the attR intasome. Plasmid 70:190-200
Keeton, Carolyn M; Gardner, Jeffrey F (2012) Roles of Exc protein and DNA homology in the CTnDOT excision reaction. J Bacteriol 194:3368-76
Kim, Seyeun; Gardner, Jeffrey F (2011) Resolution of Holliday junction recombination intermediates by wild-type and mutant IntDOT proteins. J Bacteriol 193:1351-8
Kim, Seyeun; Swalla, Brian M; Gardner, Jeffrey F (2010) Structure-function analysis of IntDOT. J Bacteriol 192:575-86

Showing the most recent 10 out of 66 publications