Your search keyword '"E. coli Cell cycle"' showing total 4 results

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

Author

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

Subjects

MiniR1–1 replication, DnaA-boxes, Complete genome sequence, E. coli Cell cycle, Microbiology, QR1-502

Abstract

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.

Published

2018

2. Mutations of DnaA-boxes in the oriR region increase replication frequency of the MiniR1–1 plasmid

Author

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

Published

2018

3. Mutations of DnaA-boxes in the oriR region increase replication frequency of the MiniR1–1 plasmid

Author

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

Subjects

DNA Replication, DNA, Bacterial, 0301 basic medicine, Microbiology (medical), Cell division, R1 plasmid, Genetic Vectors, genetic processes, 030106 microbiology, lcsh:QR1-502, Cloning vector, Replication Origin, Biology, medicine.disease_cause, Microbiology, lcsh:Microbiology, DnaA-boxes, 03 medical and health sciences, Plasmid, Bacterial Proteins, Escherichia coli, MiniR1–1 replication, medicine, Complete genome sequence, Gene, Mutation, Binding Sites, Base Sequence, Escherichia coli Proteins, DNA Helicases, DNA replication, DNA, Sequence Analysis, DNA, Molecular biology, DnaA, DNA-Binding Proteins, 030104 developmental biology, Copper-Transporting ATPases, Trans-Activators, health occupations, bacteria, E. coli Cell cycle, Plasmids, Research Article

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. Electronic supplementary material The online version of this article (10.1186/s12866-018-1162-3) contains supplementary material, which is available to authorized users.

Published

2018

4. 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