Identification of multicopy suppressors of the pcnB plasmid copy number defect in Escherichia coli

被引:0
|
作者
N. Sarkar
G.-j. Cao
C. Jain
机构
[1] Boston Biomedical Research Institute,
[2] 64 Grove Street,undefined
[3] Watertown,undefined
[4] MA 02472,undefined
[5] USA,undefined
[6] Dept. of Biological Chemistry and Molecular Pharmacology,undefined
[7] Harvard Medical School,undefined
[8] Boston,undefined
[9] MA 02115,undefined
[10] USA,undefined
[11] Department of Biochemistry and Molecular Biology,undefined
[12] University of Miami School of Medicine,undefined
[13] Miami,undefined
[14] FL 33101,undefined
[15] USA,undefined
[16] 1401 Saint Edwards Drive,undefined
[17] Apt. #174,undefined
[18] Austin,undefined
[19] TX 78704,undefined
[20] USA,undefined
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关键词
Plasmid copy number ColE1 plasmid Poly(A) polymerase Antisense RNA;
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摘要
Plasmids containing a ColE1 origin of replication are widely used for cloning purposes in Escherichia coli. Among the host factors that affect the copy number of ColE1 plasmids is the E. coli protein poly(A) polymerase I (PAP I), which regulates the intracellular level of RNA I, a ColE1-encoded negative regulator of plasmid replication. In strains that lack PAP I, RNA I levels are elevated, resulting in reduced levels of ColE1 plasmids in the cell. PAP I is encoded by the gene pcnB. We devised a genetic approach, based on the identification of multicopy suppressor clones, to identify trans-acting factors that can help offset the ColE1 plasmid copy number defect in a pcnB- genetic background. Using this strategy, we identified suppressors that mapped to two regions of the E. coli chromosome. The suppressor activity of one of the chromosomal regions was localized to the rssB gene, a response regulator gene known to be involved in the turnover of the stationary-phase sigma factor, RpoS. The second suppressor maps to min 55.4 of the E. coli chromosome, and the factor responsible for the suppressor activity appears to be a novel RNA or protein.
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页码:62 / 69
页数:7
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