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Novel molecular techniques for the identification of the members of Brucellaceae family

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Auteur
Papaventsis, D.; Siafakas, N.; Markoulatos, P.; Sopidou, V.; Economou, C.; Levidiotou-Stefanou, S.
Date
2006
Sujet
amikacin
aminoglycoside
ampicillin
aztreonam
beta lactam
cefepime
ceftazidime
ceftriaxone
ciprofloxacin
colistin
cotrimoxazole
gentamicin
imipenem
piperacillin
piperacillin plus tazobactam
ribosome RNA
sultamicillin
article
bacterial strain
bacterium identification
Brucellaceae
cell culture
computer program
Cyprus
gene sequence
Gram negative bacterium
nucleotide sequence
Ochrobactrum anthropi
phylogeny
polymerase chain reaction
Bacteria (microorganisms)
Negibacteria
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Résumé
An account is presented of an attempt to identify a multiresistant, gram-negative bacterium that was isolated from raw sewage in Cyprus. The API 2ONE system was initially used to identify the strain on the basis of its biochemical profile. In addition, a 16S rRNA-specific PCR was applied on genetic material extracted directly from BGM cell culture material after which the sequence of the largest part of the 16S rRNA gene (approximately 1000 nucleotides) was obtained BLAST software was used to compare the sequences obtained with corresponding sequences of other strains belonging to members of the family Brucellaceae, which were available in the GenBank database. The isolated bacterium was identified as Ochrobactrum anthropi by both its biochemical profile and its 16S rRNA sequences, which showed a 98% similarity with other O. anthropi strains. It was found to be resistant to several antibiotics, including b-lactams and aminoglycosides. Phylogenetic analysis showed that 16S rRNA gene sequencing should be used with caution for the identification of family Brucellaceae members that are genetically closely related. In conclusion, this study recorded the first isolation of an O. anthropi strain from environmental samples in Cyprus. This strain was found to be highly resistant to antibiotics. Sequencing of the 16S rRNA gene was useful for the verification of the identity of the strain. However, phylogenetic comparisons with other related bacterial strains showed that this method is perhaps not the most decisive for identification of members of the family Brucellaceae, due to the consonance between different species and genera.
URI
http://hdl.handle.net/11615/31979
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