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J. Bacteriol., 11 1995, 6100-6105, Vol 177, No. 21
BI Marklund, DP Speert and RW Stokes
Mycobacterium intracellulare is a slow-growing pathogenic mycobacterium
closely related to Mycobacterium avium. In contrast to Mycobacterium
tuberculosis and Mycobacterium bovis BCG, M. intracellulare has received
little attention as a model species for studies of mycobacterial molecular
biology and genetics. This study shows that M. intracellulare 1403 (ATCC
35761) can be transformed by electroporation with high frequencies (up to
10(6) transformants per microgram of DNA), using plasmids pYT937 and pMH94
as replicative and integrative vectors, respectively. We also describe an
experimental system that we used to study DNA recombination in M.
intracellulare. First, an integrative plasmid was introduced into M.
intracellulare 1403. A nonreplicative, nonintegrative plasmid having
homology with the integrated plasmid was then introduced, and the resultant
recombinants were analyzed to distinguish between events of homologous and
illegitimate recombination. No illegitimate recombination occurred; in all
recombinants, a single crossover between homologous regions of the two
plasmids was noted. During subsequent growth of a recombinant clone, a
spontaneous deletion occurred that resulted in a gene replacement on the
chromosome of M. intracellulare 1403. The ability to construct site-
specific mutations in M. intracellulare will provide novel insights into
the biology of slow-growing mycobacteria.
Copyright © 1995, American Society for Microbiology
Gene replacement through homologous recombination in Mycobacterium intracellulare
Division of Infectious and Immunological Diseases, British Columbia's Children's Hospital, Vancouver, Canada.
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