Excess production of phage λ delayed early proteins under conditions supporting high Escherichia coli growth rates

Author:

Gabig Magdalena1,Obuchowski Michal1,WeLgrzyn Alicja2,Szalewska-Palasz Agnieszka1,Thomas Mark S.3,WeLgrzyn Grzegorz1

Affiliation:

1. Laboratory of Molecular Genetics, Department of Molecular Biology, University of GdańskKładki 24, 80-822 GdańskPoland

2. Institute of Biochemistry and Biophysics, Polish Academy of Sciences, Laboratory of Molecular Biology affiliated to the University of GdańskK&lstroke;adki 24, 80-822 GdańskPoland

3. Division of Molecular and Genetic Medicine, University of Sheffield Medical SchoolBeech Hill Road, Sheffield S10 2RXUK

Abstract

Bacteriophage λ is unable to lysogenize Escherichia coli hosts harbouring the rpoA341 mutation due to a drastic reduction in transcription from CII-activated lysogenic promoters (p E, p 1 and p aQ). In addition, the level of early transcripts involved in the lytic pathway of λ development is also decreased in this genetic background due to impaired N-dependent antitermination. Here, it is demonstrated that despite the reduced level of early lytic p L- and p R-derived transcripts, lytic growth of bacteriophage λ is not affected in rich media. The level of the late lytic, p R-derived transcripts also remains unaffected by the rpoA341 mutation under these conditions. However, it was found that whilst there is no significant difference in the phage burst size in rpoA + and rpoA341 hosts growing in rich media, phage λ is not able to produce progeny in the rpoA341 mutant growing in minimal medium, in contrast to otherwise isogenic rpoA + bacteria. Provision of an excess of the phage replication proteins O and P in trans or overproduction of the antitermination protein N restore the ability of phage λ to produce progeny in the rpoA341 mutant under the latter conditions. These results suggest that in rich media phage λ produces some early proteins in excess of that needed for its effective propagation and indicate that replication proteins may be limiting factors for phage lytic growth in poor media.

Publisher

Microbiology Society

Subject

Microbiology

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