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1. Mutations of DnaA-boxes in the <italic>oriR</italic> region increase replication frequency of the MiniR1–1 plasmid.

Author

Yao, Yuan, Enkhtsetseg, Sukhbold, Odsbu, Ingvild, Fan, Lifei, and Morigen, Morigen

Subjects

*PLASMIDS, *DNA replication, *NUCLEOTIDE sequence, *ESCHERICHIA coli, *GENES

Abstract

Background: The MiniR1–1 plasmid is a derivative of the R1 plasmid, a low copy cloning vector. Results: Nucleotide sequencing analysis shows that the MiniR1–1 plasmid is a 6316 bp circular double-stranded DNA molecule with an oriR1 (origin for replication). The plasmid carries the repA, tap, copA and bla genes, and genes for ORF1 and ORF2. MiniR1–1 contains eight DnaA-binding sites (DnaA-boxes). DnaA-box1 is in the oriR1 region and fully matched to the DnaA-box consensus sequence, and DnaA-box8, with one mismatch, is close to the copA gene. The presence of the MiniR1–1 plasmid leads to an accumulation of the D-period cells and an increase in cell size of slowly growing Escherichia coli cells, suggesting that the presence of MiniR1–1 delays cell division. Mutations in the MiniR1–1 DnaA-box1 and DnaA-box8 significantly increase the copy number of the plasmid and the mutations in DnaA-box1 also affect cell size. It is likely that titration of DnaA to DnaA-boxes negatively controls replication of the MiniR1–1 plasmid and delays cell division. Interestingly, DnaA weakly interacts with the initiator protein RepA in vivo. Conclusion: DnaA regulates the copy number of MiniR1–1 as a negative factor through interacting with the RepA protein. [ABSTRACT FROM AUTHOR]

Published

2018