Plasmid and chromosomal genes encode determinants of virulence for (Perry & Fetherston 1997, Parkhill et al. 2001, Deng et al. 2002. A 102-kb, unstable chromosomal area (locus pgm) is essential for Y. pestis virulence (Fetherston et al. 1992, Hinnebusch et al. 1996, Buchrieser et al. 1998.Typical strains of Y. pestis harbour three plasmids: pPst (9.5kb), encoding a plasminogen activator protease (Pla) (Sodeinde & Goguen, 1988; pFra (90kb), encoding a capsular protein Fraction 1 (F1) with antiphagocytic activities (Du et al. 2002) and murine toxin (Ymt), required for survival in the flea (Hinnebusch et al. 2002); pYV (70kb), encoding the Yop virulon which comprises both the Yop effectors proteins and the proteins necessary for injecting them into host cells. The Yop virulon enables the bacteria to survive and multiply in the lymphoid tissues of the host (Cornelis 2002). Several insertion sequences (IS100, IS200, IS285) present in the three plasmids favour recombination events and genetic plasticity (Filippov et al. 1995, Parkhill et al. 2001, Deng et al. 2002.However, atypical strains lacking some plasmids have been found in several foci around the world. On the other hand, strains containing extra DNA bands or additional cryptic plasmids have also been found (Filippov et al. 1990, Chu et al. 1998. In vitro, Y. pestis genome is very plastic and several changes have been described: emergence of additional DNA-bands, increasing of plasmid molecular mass, and integration of plasmids into the bacterial chromosome with or without loss of functions (Zsigray et al. 1985, Protsenko et al. 1991. Furthermore, the typical plasmids may be eliminated spontaneously at a high frequency during storage in the laboratory or through successive subcultures (Protsenko et al. 1991).The study of the plasmid content of Y. pestis isolates from the plague foci of Northeast Brazil, stored in the laboratory for several decades, showed that some of them displayed an atypical plasmid profile characterized by the absence of some plasmids or by the presence of extra DNA bands (Leal et al. 1997a, Leal & Almeida 1999, Cavalcanti et al. 2002. The absence of plasmids and the emergence of extra-DNA bands in the Brazilian isolates could also have been produced during storage or handling in the laboratory.To observe possible alterations in plasmids of the cultures in vitro and the impact of the alterations to their pathogenicity, three low subcultured and highly pathogenic Y. pestis isolates were submitted to serial subcultures. Colonies selected after subcultures were analyzed for their plasmid content and the presence of some characteristic genes of each plasmid. LD 50 in mice of the parental strains and derived cultures displaying different plasmid contents were compared. MATERIALS AND METHODSBacteria and culture conditions -The study involved two Brazilian isolates: one old (P. Exu 340, originating from a finger bone marrow in a fatal human case in 1969), and the most recent Brazilian isolate (P. CE 882, originating from a hemoculture from a plagu...
We report the ability of Yersinia pestis to survive up to 47 years in agar stabs, in rubber-stoppered tubes, under refrigeration (+4 to +10°C), although overall subculture recovery rates were poor and inversely related to the length of time stored. Genetic characterization of virulence gene presence among these subcultures was suggestive of significant variation in the genomic stability of Y. pestis subcultures stored under these conditions. This variation, together with all of the inherent temporal, geographic and other genetic variation represented by all of the recoverable strains in the historical 'Collection of Yersinia pestis' (Fiocruz-CYP) maintained by the SRP of FIOCRUZ-PE in Brazil was preserved in new frozen culture stocks stored at -70°C as a result of this study. These frozen culture stocks represent a valuable resource for future comparative studies of Y. pestis.
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