Abstract

The process of genetic transposition has revolutionized ideas about evolution and the formation of chromosomes in eukaryotes and prokaryotes alike. While the genetic impact of transposons is becoming evident, the enzymes that splice genes and the regulatory mechanisms controlling their expression and activity in the cell are unknown. Only a few systems are currently available which permit genetic and biochemical analysis of these problems. Our long range objective is to dissect the biochemical mechanisms that regulate Mu transcription and replication. Phage Mu uses transposition to integrate and replicate its DNA. It is the most active natural transposable element known: during the lytic cycle Mu uses the E. coli replication machinery to transpose to 100 sites in the chromosome within an hour. The principle elements controlling virus development are located near the left genetic end. We are developing a technology based on anti-sense RNA production that allows the characterization of phage transcription patterns in vitro as well as in vivo. Mu utilizes converging promoters to synthesixe either lytic functions or Mu repressor. This operator is interactive wiht host enzymes. Supercoiling stimulates lytic transcription and decreases repressor transcription; thus, the virus is sensitive to DNA gyrase activity of the host. A binding site for a type II DNA binding protein of E. coli (IHF) is located in the promoter near a DDNA site containing a sequence induced bend. IHF enhances supercoil-modulation of promoter strength in vitro. This type of enhancer controls 50-fold regulation. Mu transposition is efficient also because a set of accessory proteins is encoded by a dispensible region of the virus. One protein from this region, an unusual DNA binding protein encoded by the Mu gam gene, has been purified in large amounts. pgam blocks exonucleases and aggregates supercoiled DNA. In vitro and in vivo experiments are outlined to define the biochemical mechanisms by which this protein modifies the Mu transposition process.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM033143-08
Application #
3282499
Study Section
Microbial Physiology and Genetics Subcommittee 2 (MBC)
Project Start
1983-07-01
Project End
1991-06-30
Budget Start
1990-07-01
Budget End
1991-06-30
Support Year
8
Fiscal Year
1990
Total Cost
Indirect Cost

  Institution

Name
University of Alabama Birmingham
Department
Type
Schools of Dentistry
DUNS #
004514360
City
Birmingham
State
AL
Country
United States
Zip Code
35294

  Publications

Higgins, N Patrick (2016) Species-specific supercoil dynamics of the bacterial nucleoid. Biophys Rev 8:113-121
Higgins, N Patrick; Vologodskii, Alexander V (2015) Topological Behavior of Plasmid DNA. Microbiol Spectr 3:
Higgins, N Patrick (2014) RNA polymerase: chromosome domain boundary maker and regulator of supercoil density. Curr Opin Microbiol 22:138-43
Higgins, N Patrick (2012) A human TOP2A core DNA binding X-ray structure reveals topoisomerase subunit dynamics and a potential mechanism for SUMO modulation of decatenation. J Mol Biol 424:105-8
Rovinskiy, Nikolay; Agbleke, Andrews Akwasi; Chesnokova, Olga et al. (2012) Rates of gyrase supercoiling and transcription elongation control supercoil density in a bacterial chromosome. PLoS Genet 8:e1002845
Booker, Betty M; Deng, Shuang; Higgins, N Patrick (2010) DNA topology of highly transcribed operons in Salmonella enterica serovar Typhimurium. Mol Microbiol 78:1348-64
Higgins, N Patrick (2007) Mutational bias suggests that replication termination occurs near the dif site, not at Ter sites: what's the Dif? Mol Microbiol 64:1-4
Manna, Dipankar; Porwollik, Steffen; McClelland, Michael et al. (2007) Microarray analysis of Mu transposition in Salmonella enterica, serovar Typhimurium: transposon exclusion by high-density DNA binding proteins. Mol Microbiol 66:315-28
Champion, Keith; Higgins, N Patrick (2007) Growth rate toxicity phenotypes and homeostatic supercoil control differentiate Escherichia coli from Salmonella enterica serovar Typhimurium. J Bacteriol 189:5839-49
Higgins, N Patrick (2007) Under DNA stress, gyrase makes the sign of the cross. Nat Struct Mol Biol 14:256-8

Showing the most recent 10 out of 34 publications