Transformation of Streptococcus mutans with chromosomal and shuttle plasmid (pYA629) DNAs.

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Infect Immun. 1986 November; 54(2): 273-282

Transformation of Streptococcus mutans with chromosomal and shuttle plasmid (pYA629) DNAs.

H H Murchison, J F Barrett, G A Cardineau and R Curtiss 3rd

ABSTRACT

Transformation (i.e., DNase-sensitive genetic transfer) of strainsof Streptococcus mutans representing serotypes c and e was accomplishedby using chromosomal DNA from a Rifr Strr Spcr isolate of strainGS5 (UAB525) and a chimeric plasmid, pYA629. Shuttle plasmidpYA629 comprises the S. mutans plasmid pVA318, an inducibleerythromycin resistance determinant originally isolated froma group A streptococcal strain, the tetracycline resistancegene and replication region of the Escherichia coli plasmidpBR322, and the promoter region of the S. mutans gene for aspartatebeta-semialdehyde dehydrogenase. The strains examined for recipientability included those known to lack a cryptic plasmid (GS5,UA130, UA159, and MT8148) and those known to contain a widelydisseminated 5.8-kilobase cryptic plasmid (LM7, V318, UA101,UA174, and 3098791). The transformation frequencies in GS5 forGS5 chromosomal antibiotic resistance markers were comparableto those reported by others, but UA101, UA130, UA159 and UA174were transformed with both chromosomal and plasmid markers atmuch higher efficiencies. In a larger strain survey, strainscontaining the 5.8-kilobase cryptic plasmid were more frequentlytransformable with both chromosomal and pYA629 DNAs than werestrains lacking this cryptic plasmid. All plasmid-containingstrains except LM7 lost their resident cryptic plasmids whentransformed with pYA629. LM7 transformed with pYA629 retainedpLM7. There are therefore at least two incompatibility groupsamong S. mutans cryptic plasmids. yPA629 DNA isolated from eitherE. coli or S. mutans transformed S. mutans with equal efficiency.pYA629 DNA isolated from S. mutans transformed both restriction-deficientand restriction-proficient E. coli recipients. Therefore, thestrains of S. mutans used lack a restriction-modification systemfor pYA629 DNA sequences. S. mutans strains that are readilytransformable, display maximal cariogenicity in gnotobioticrats, and give high scores for in vitro measures of importantvirulence attributes have been identified to facilitate studieson the genetic basis and control of virulence.

Infect Immun. 1986 November; 54(2): 273-282

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