Genomic studies have shown that the nomenclature for several Brucella species is not consistent if the genetic relationships among species are considered to be the gold standard for discriminating between species [20]. For example, B. ceti is divided into two separate groups, one of which is more closely related to B. pinnipedialis than to the other Selleck Go6983 group of B. ceti [20]. Additionally, B. suis biovar 5 is more related to B. ceti, B. neotomae, B. pinnipedialis and B. ovis than to the other B. suis biovars [20]. The timely detection and

rapid identification of the microorganisms involved are essential for the most-effective response to an infectious disease outbreak, regardless of whether the outbreak is natural or deliberate. This rapid identification is necessary not only to treat check details patients effectively but also to establish outbreak management, source tracing, and threat analyses. Matrix-assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI-TOF-MS) is a rapid method used to analyze biological differences

in microorganisms. selleck chemical MALDI-TOF-MS emerged as a new diagnostic tool in established microbiological laboratories [21]. The advantages of MALDI-TOF-MS over conventional techniques are that it is a fast, cost-effective, accurate method, which is suitable for the high-throughput identification of bacteria by less-skilled laboratory personnel because preliminary identification steps are unnecessary [21–24]. The bacteria are identified by comparing the obtained MS spectra to the MS spectra or profiles of MS spectra from a reference library. Hence, the reliability of the identification is based on the content and quality of this library, among other factors. Recently, a reference library to identify Brucella species was constructed using 12 Brucella strains, but using this ‘Brucella library’, the discrimination was insufficient for identification at the species level [25]. Ixazomib ic50 In contrast, reliable identification at the species level was shown for other genetically closely related species, such as Fransicella

species, Bacillus species, and species from the Burkholderia cepacia complex [26–28]. The aim of this study was to improve identification using MALDI-TOF-MS at the species level of Brucella. Therefore, a custom reference library was constructed with strains that represent the known genetic variation of Brucella at the species and biovar level according to MLVA. Subsequently, this custom reference library was evaluated using 152 Brucella isolates that were identified using MLVA. Methods Bacterial strains Seventeen of the 170 isolates included in this study are reference strains representing the classical Brucella species, and only the classical reference strain for B. suis biovar 4 is missing (Additional file 1: Table S1) [1]. The 170 isolates included in the study were all typed using MLVA [19]. The Brucella isolates originated from K.