INFECTION OF MYCOBACTERIUM SMEGMATIS WITH D29 PHAGE DNA

doi:10.1084/jem.119.1.139

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ARTICLE

INFECTION OF MYCOBACTERIUM SMEGMATIS WITH D29 PHAGE DNA

Tohru Tokunaga M.D.¹ and Margret I. Sellers Ph.D.¹

¹ From the Department of Medical Microbiology and Immunology, School of Medicine, University of California, Los Angeles

DNA extracted from D29 mycobacteriophage produced plaques whenplated on Mycobacterium smegmatis 607. The host bacterium didnot require alternation such as conversion to protoplasts; cellssusceptible to infection with intact phage were susceptibleto DNA.

The bases found in calf thymus DNA constituted the basesof D29 DNA, adenine being paired with thymine and guanine withcytosine. The dissymmetry ratio (A + T/G + C) was 0.56, andthe buoyant density in CsCl was 1.722 with a GC content of 63.77per cent.

The efficiency of plating of the DNA is very muchlower than that of intact D29, and it penetrates the host ata slower rate. As does intact phage, D29 DNA requires calciumions for productive infection of 607.

D29 DNA is significantlyinactivated by incubation with RNAase, but the inactivationprobably results from a complexing with the DNA rather thanfrom enzyme hydrolysis.

Submitted on September 16, 1963

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