The housekeeping genes, 16S rDNA, ITS1 (internal transcribed spac

The housekeeping genes, 16S rDNA, ITS1 (internal transcribed spacer 1), gyrB, hsp65, rpoB and sodA, were amplified and sequenced for the 56 strains. Two genes codifying for antibiotic resistance, aphA and ermX, were also amplified and sequenced for these strains. Three other primer sets codifying for antibiotic resistances (cmx, repB and tetA) were also tested but did not produce an amplicon. The list of primers is indicated as Additional file 2: Table S2 [21–25]. PCR amplification and sequence reaction was performed as previously

described [19]. Allele diversity, nucleotide diversity and statistical analysis Allele and nucleotide diversities were calculated from the gene sequences with the DnaSP package, version 3.51 [26]. For identification purposes, distinct allele sequences were assigned arbitrary allele numbers for each locus. For each isolate, the combination of alleles obtained at each locus defined check details its allelic profile. Each allelic profile constitutes a sequence type (ST), and isolates with identical VX-680 in vivo profiles belonged to the same ST. Clustering of STs was performed with the Sequence Type Analysis and Recombinational Tests (START) program [27]. The matrix of pair-wise distances

between the allelic profiles was converted to NEXUS files, and the split decomposition was analysed with the SplitsTree software program, vs. 4 [28]. Splits tree allowed researchers to visualise clustering within the population and to detect recombination between STs. The nucleotide sequences determined in PRI-724 purchase this study for the different alleles of each locus have been deposited in the EMBL database under the accession numbers HE586270 to HE586309. Analysis by MALDI-TOF mass spectrometry Matrix-assisted linear desorption/ionisation-time-of-flight mass spectrometry (MALDI-TOF MS) analyses for all strains were performed at Anagnostec, GmbH, Germany [29], as described Scotta et al. [30]. Results Phenotypic characterisation and antibiotic susceptibility tests of the isolates All colonies were pale yellow in colour,

nonhemolytic, catalase positive and oxidase negative. The strains were identified by the RapID CB Plus® strips as C. striatum (51 strains with a confidence level between 85.54% – 99.97%), C. pseudodiphtheriticum PJ34 HCl (2 strains with a 100% of confidence level), or C. amycolatum (1 strain with a confidence level of 51.26%) [Additional file 3: Table S3]. All isolates were susceptible to vancomycin and resistant to cefotaxime and ciprofloxacin, whereas susceptibilities to other antibiotics tested were heterogeneous (Additional file 4: Table S4). The type strain of C. amycolatum was susceptible to all the antibiotics tested. The C. striatum type strain was susceptible to all of the antibiotics except cefotaxime. The two isolates that were analysed from the CCUG were sensitive to antibiotics.

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