Inhibition of spontaneous induction of lambdoid prophages in Escherichia coli cultures: Simple procedures with possible biotechnological applications

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Abstract

Background: Infections of bacterial cultures by bacteriophages are serious problems in biotechnological laboratories. Apart from such infections, prophage induction in the host cells may also be dangerous. Escherichia coli is a commonly used host in biotechnological production, and many laboratory strains of this bacterium harbour lambdoid prophages. These prophages may be induced under certain conditions leading to phage lytic development. This is fatal for further cultivations as relatively low, though still significant, numbers of phages may be overlooked. Thus, subsequent cultures of non-lysogenic strains may be infected and destroyed by such phage. Results: Here we report that slow growth of bacteria decreases deleterious effects of spontaneous lambdoid prophage induction. Moreover, replacement of glucose with glycerol in a medium stimulates lysogenic development of the phage after infection of E. coli cells. A plasmid was constructed overexpressing the phage 434 cl gene, coding for the repressor of phage promoters which are necessary for lytic development. Overproduction of the cl repressor abolished spontaneous induction of the λimm434 prophage. Conclusions: Simple procedures that alleviate problems with spontaneous induction of lambdoid prophage and subsequent infection of E. coli strains by these phages are described. Low bacterial growth rate, replacement of glucose with glycerol in a medium and overproduction of the cl repressor minimise the risk of prophage induction during cultivation of lysogenic bacteria and subsequent infection of other bacterial strains. © 2001 Czyz et al, licensee BioMed Central Ltd.

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Czyz, A., Los, M., Wrobel, B., & Wegrzyn, G. (2001). Inhibition of spontaneous induction of lambdoid prophages in Escherichia coli cultures: Simple procedures with possible biotechnological applications. BMC Biotechnology, 1. https://doi.org/10.1186/1472-6750-1-1

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