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« Previous AbstractCloning and genetic organization of the bacteriocin 31 determinant encoded on the Enterococcus faecalis pheromone-responsive conjugative plasmid pYI17    Next AbstractGenetic analysis of transfer-related regions of the vancomycin resistance Enterococcus conjugative plasmid pHTbeta: identification of oriT and a putative relaxase gene »

J Bacteriol


Title:Cloning and genetic and sequence analyses of the bacteriocin 21 determinant encoded on the Enterococcus faecalis pheromone-responsive conjugative plasmid pPD1
Author(s):Tomita H; Fujimoto S; Tanimoto K; Ike Y;
Address:"Department of Microbiology, Gunma University School of Medicine, Maebashi, Japan"
Journal Title:J Bacteriol
Year:1997
Volume:179
Issue:24
Page Number:7843 - 7855
DOI: 10.1128/jb.179.24.7843-7855.1997
ISSN/ISBN:0021-9193 (Print) 1098-5530 (Electronic) 0021-9193 (Linking)
Abstract:"The pheromone-responsive conjugative plasmid pPD1 (59 kb) of Enterococcus faecalis encodes the bacteriocin 21 (bac21) determinant. Cloning, transposon insertion mutagenesis and sequence analysis of the bac21 determinant showed that an 8.5-kb fragment lying between kb 27.1 and 35.6 of the pPD1 map is required for complete expression of the bacteriocin. The 8.5-kb fragment contained nine open reading frames (ORFs), bacA to bac1, which were oriented in the same (upstream-to-downstream) direction. Transposon insertions into the bacA to bacE ORFs, which are located in the proximal half of bac21, resulted in defective bacteriocin expression. Insertions into the bacF to bac1 ORFs, which are located in the distal half of bac21, resulted in reduced bacteriocin expression. Deletion mutant analysis of the cloned 8.5-kb fragment revealed that the deletion of segments between kb 31.6 and 35.6 of the pPD1 map, which contained the distal region of the determinant encoding bacF to bac1, resulted in reduced bacteriocin expression. The smallest fragment (4.5 kb) retaining some degree of bacteriocin expression contained the bacA to bacE sequences located in the proximal half of the determinant. The cloned fragment encoding the 4.5-kb proximal region and a Tn916 insertion mutant into pPD1 bacB trans-complemented intracellularly to give complete expression of the bacteriocin. bacA encoded a 105-residue sequence with a molecular mass of 11.1 kDa. The deduced BacA protein showed 100% homology to the broad-spectrum antibiotic peptide AS-48, which is encoded on the E. faecalis conjugative plasmid pMB2 (58 kb). bacH encoded a 195-residue sequence with a molecular mass of 21.9 kDa. The deduced amino acid sequence showed significant homology to the C-terminal region of HlyB (31.1% identical residues), a protein located in the Escherichia coli alpha-hemolysin operon that is a representative bacterial ATP-binding cassette export protein"
Keywords:"Amino Acid Sequence Anti-Bacterial Agents/*pharmacology *Bacterial Proteins Base Sequence Cloning, Molecular Conjugation, Genetic DNA Transposable Elements Enterococcus faecalis/*genetics Genetic Complementation Test Molecular Sequence Data Mutagenesis, I;"
Notes:"MedlineTomita, H Fujimoto, S Tanimoto, K Ike, Y eng Comparative Study Research Support, Non-U.S. Gov't 1997/12/24 J Bacteriol. 1997 Dec; 179(24):7843-55. doi: 10.1128/jb.179.24.7843-7855.1997"

 
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