Abstract

Mobile DNA elements function to control variable gene expression and are a major contributor to horizontal gene transfer, including the dissemination of antibiotic resistance and virulence factors. They are also being exploited as potent tools for genetic engineering. Over the years this grant has supported work on the mechanism and control of site-specific DNA recombination reactions, focusing largely on the DNA inversion reaction that regulates flagellar phase variation in Salmonella enterica. We now have a fairly detailed molecular and structural understanding of this reaction, including how the Fis/enhancer regulatory element interacts with the Hin serine recombinase to promote remodeling of Hin dimers into the active synaptic tetramer and how DNA exchange by subunit rotation within the tetramer occurs. Future studies will address two remaining important mechanistic issues: why does the Hin subunit rotation reaction pause at the ligation-competent conformer and how do Fis/enhancer-Hin contacts promote remodeling to the active Hin tetramer. Our emphasis in the next funding period will shift towards understudied recombination reactions mediated by members of the Large Serine Recombinase subfamily, which contain a large C-terminal DNA binding and regulatory domain (CTD), and the IS607-serine transposon subfamily, which have their DNA binding domain at the N-terminus. Regarding the former, we are investigating the Listeria phage A118 serine integrase and its regulatory partner Gp44. Research will be directed at mechanisms underlying the directional control of synapsis and will be influenced by a recently determined X-ray structure of the CTD of a nearly identical Listeria phage integrase by the Van Duyne lab. Regarding serine transposons, our early biochemical and structural studies provide encouragement that we will be able to decipher the novel pathway for transposition by these unusual elements. Since the discovery of the Fis nucleoid protein from our work on the Hin-catalyzed DNA inversion reaction, we have been investigating its many other regulatory roles, its expression as a function of cell growth, and how it selects and deforms it DNA binding site. Under fast growth rates Fis can be the most abundant DNA binding protein in the cell. Fis binds prolifically throughout the chromosome, and we propose is contributing to chromosome compaction through formation of dynamic DNA loops and by DNA bending. In future work we will investigate the role of DNA minor groove shape and Fis-Fis interactions in binding to the chromosome and probe for DNA loops between Fis binding tracts in vivo. We will also investigate cooperative recruitment of proteins by Fis that are primarily mediated through changes in DNA shape.

Public Health Relevance

Work on this project will elucidate mechanisms of inversion, deletion, integration, and complete transposition of DNA segments by enzymes of the serine recombinase family. Knowledge gained from these studies will help to exploit these elements as tools of genetic engineering. An additional area concerns bacterial multi-functional chromatin proteins, particularly regarding their effects on DNA structure, gene regulation, and chromosome packaging.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM038509-32
Application #
9511845
Study Section
Prokaryotic Cell and Molecular Biology Study Section (PCMB)
Program Officer
Reddy, Michael K
Project Start
1987-07-01
Project End
2019-06-30
Budget Start
2018-07-01
Budget End
2019-06-30
Support Year
32
Fiscal Year
2018
Total Cost
Indirect Cost

  Institution

Name
University of California Los Angeles
Department
Biochemistry
Type
Schools of Medicine
DUNS #
092530369
City
Los Angeles
State
CA
Country
United States
Zip Code
90095

  Publications

Chen, Wenyang; Mandali, Sridhar; Hancock, Stephen P et al. (2018) Multiple serine transposase dimers assemble the transposon-end synaptic complex during IS607-family transposition. Elife 7:
Mandali, Sridhar; Gupta, Kushol; Dawson, Anthony R et al. (2017) Control of Recombination Directionality by the Listeria Phage A118 Protein Gp44 and the Coiled-Coil Motif of Its Serine Integrase. J Bacteriol 199:
Kamar, Ramsey I; Banigan, Edward J; Erbas, Aykut et al. (2017) Facilitated dissociation of transcription factors from single DNA binding sites. Proc Natl Acad Sci U S A 114:E3251-E3257
Hadizadeh, Nastaran; Johnson, Reid C; Marko, John F (2016) Facilitated Dissociation of a Nucleoid Protein from the Bacterial Chromosome. J Bacteriol 198:1735-42
Xiao, Botao; McLean, Meghan M; Lei, Xianbin et al. (2016) Controlled rotation mechanism of DNA strand exchange by the Hin serine recombinase. Sci Rep 6:23697
Hancock, Stephen P; Stella, Stefano; Cascio, Duilio et al. (2016) DNA Sequence Determinants Controlling Affinity, Stability and Shape of DNA Complexes Bound by the Nucleoid Protein Fis. PLoS One 11:e0150189
Johnson, Reid C (2015) Site-specific DNA Inversion by Serine Recombinases. Microbiol Spectr 3:MDNA3-0047-2014
Johnson, Reid C (2015) Site-specific DNA Inversion by Serine Recombinases. Microbiol Spectr 3:1-36
Chang, Yong; Johnson, Reid C (2015) Controlling tetramer formation, subunit rotation and DNA ligation during Hin-catalyzed DNA inversion. Nucleic Acids Res 43:6459-72
Giuntoli, Rebecca D; Linzer, Nora B; Banigan, Edward J et al. (2015) DNA-Segment-Facilitated Dissociation of Fis and NHP6A from DNA Detected via Single-Molecule Mechanical Response. J Mol Biol 427:3123-36

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