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Spontaneous Excision of the Salmonella enterica Serovar Enteritidis-Specific Defective Prophage-Like Element SE14

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2010-04
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Santiviago Cid, Carlos
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Spontaneous Excision of the Salmonella enterica Serovar Enteritidis-Specific Defective Prophage-Like Element SE14
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Author
  • Santiviago Cid, Carlos;
  • Blondel, Carlos;
  • Quezada, Carolina P.;
  • Silva, Cecilia A.;
  • Tobar, Pia M.;
  • Porwollik, Steffen;
  • McClelland, Michael;
  • Andrews Polymenis, Helene L.;
  • Toro, Cecilia S.;
  • Zaldívar San Román, María Mercedes;
  • Contreras, Inés;
Abstract
Salmonella enterica serovar Enteritidis has emerged as a major health problem worldwide in the last few decades. DNA loci unique to S. Enteritidis can provide markers for detection of this pathogen and may reveal pathogenic mechanisms restricted to this serovar. An in silico comparison of 16 Salmonella genomic sequences revealed the presence of an 12.5-kb genomic island (GEI) specific to the sequenced S. Enteritidis strain NCTC13349. The GEI is inserted at the 5 end of gene ydaO (SEN1377), is flanked by 308-bp imperfect direct repeats (attL and attR), and includes 21 open reading frames (SEN1378 to SEN1398), encoding primarily phage-related proteins. Accordingly, this GEI has been annotated as the defective prophage SE14 in the genome of strain NCTC13349. The genetic structure and location of SE14 are conserved in 99 of 103 wild-type strains of S. Enteritidis studied here, including reference strains NCTC13349 and LK5. Notably, an extrachromosomal circular form of SE14 was detected in every strain carrying this island. The presence of attP sites in the circular forms detected in NCTC13349 and LK5 was confirmed. In addition, we observed spontaneous loss of a tetRA-tagged version of SE14, leaving an empty attB site in the genome of strain NCTC13349. Collectively, these results demonstrate that SE14 is an unstable genetic element that undergoes spontaneous excision under standard growth conditions. An internal fragment of SE14 designated Sdf I has been used as a serovar-specific genetic marker in PCR-based detection systems and as a tool to determine S. Enteritidis levels in experimental infections. The instability of this region may require a reassessment of its suitability for such applications.
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This work was supported by grant ADI-08/2006 to I.C. from CONICYT (Chile) and the World Bank. C.J.B. and C.A.S. were supported by fellowships from CONICYT (Chile). M.M. and S.P. were supported partly by NIH grants R01AI073971 and R01AI052237. H.L.A.-P. was supported by NIH grants R21AI083964, R01AI083646, and R56AI077645.
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URI: https://repositorio.uchile.cl/handle/2250/121017
DOI: doi:10.1128/JB.00270-09
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JOURNAL OF BACTERIOLOGY, Vol. 192, No. 8, Apr. 2010, p. 2246–2254
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