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Relationship Between Chloramphenicol Acetyltransferase Activity and the Number of Resistance Genes
Author(s) -
Shizuko Iyobe,
Megumi Kono,
Koji Ohara,
Hajime Hashimoto,
Susumu Mitsuhashi
Publication year - 1974
Publication title -
antimicrobial agents and chemotherapy
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 2.07
H-Index - 259
eISSN - 1070-6283
pISSN - 0066-4804
DOI - 10.1128/aac.5.1.68
Subject(s) - chloramphenicol acetyltransferase , gene , biology , chromosome , genetics , gene duplication , acetyltransferase , chloramphenicol , microbiology and biotechnology , escherichia coli , mutant , strain (injury) , gene expression , reporter gene , antibiotics , anatomy , acetylation
Various mutants of anEscherichia coli K-12 strain were prepared, in which a chloramphenicol (CM) resistance gene (cml ) derived from an R factor, R100-1, was integrated into the chromosome. The CM acetyltransferase (CATase) activity of these strains and the strain carrying R100-1 were determined during exponential growth with the following results. (i) The CATase activity varied, depending upon the site of integration of thecml gene on the chromosome. Activity was found to be higher when thecml gene was integrated nearer the replication origin of the chromosome, the total enzyme activity found was the sum of activities coded by each gene separately. (iii) When thecml gene was in a cytoplasmic state on an R factor, R100-1, the expressed enzyme activity was four-to eightfold higher than that in the chromosomal state, suggesting the existence of about four to eight copies of R factor per chromosome. The CATase activity returned to the level of that expressed by R100-1 when the chromosomalcml gene was detached and picked up by an R factor.

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