based on 15-loci multi locus VNTR analysis. BMC Microbiol 2009, 9:66.PubMedCrossRef 31. Kattar MM, Jaafar RF, Araj GF, Le Fleche P, Matar GM, Abi RR, Khalife S, Vergnaud G: Evaluation of a multilocus variable-number tandem-repeat analysis scheme for typing human Brucella isolates in a region of brucellosis endemicity. J Clin Microbiol 2008, 46:3935–3940.PubMedCrossRef 32. Foster JT, Beckstrom-Sternberg SM, Pearson T, Beckstrom-Sternberg JS, Chain PS, Roberto FF, Hnath J, Brettin T, Keim P: Whole-genome-based phylogeny and divergence of the genus Brucella . J Bacteriol 2009, 191:2864–2870.PubMedCrossRef 33. Whatmore AM, Perrett LL, MacMillan Q VD Oph AP: Characterisation of the genetic diversity

of Brucella by multilocus sequencing. BMC Microbiol 2007, 7:34.PubMedCrossRef 34. Weynants V, Gilson D, Cloeckaert A, Tibor A, Denoel PA, Godfroid F, Limet JN, Letesson JJ: Characterization of smooth lipopolysaccharides and O polysaccharides of Brucell species by competition binding assays with monoclonal antibodies. Infect Immun 1997, 65:1939–1943.PubMed Authors’ contributions FL participated in the design of the study and coordinated the MLVA

work; FR participated in the design of the study and critically revised the manuscript; RDS executed the MLVA experiments, analyzed the data and drafted the manuscript; RP participated in the analysis of the MALDI-TOF-MS data; AdJ executed the MALDI-TOF-MS experiments and participated in the MALDI-TOF-MS data analysis; JK Microtubule Associated inhibitor participated in the design of the study; AvdL executed the MALDI-TOF-MS experiments; IVV executed the MALDI-TOF-MS experiments; SF executed the MLVA experiments; HJJ participated in the design of the study and critically revised the manuscript; JVdP participated in the design of the study and critically revised the manuscript; and AP participated in the design of the study, performed data analysis on the MLVA and MALDI-TOF-MS data, coordinated the MALDI-TOF-MS experiments,

and drafted the CP-690550 price manuscript. All authors read and approved the final manuscript.”
“Background Botrytis cinerea is a haploid necrotrophic ascomycete which is known as a major pathogen responsible ID-8 for ‘grey mold’ disease in more than 200 plant species [1–3]. It attacks aboveground plant organs, and is a major pathogen during post-harvest storage due to its exceptional ability to grow, develop and attack produce at low temperatures. The high impact of diseases caused by B. cinerea has triggered a wide scope of molecular research in recent years, resulting in the sequencing of two B. cinerea strains. This has generated a wealth of information on the genome of this fungus (http://​www.​broadinstitute.​org/​annotation/​genome/​botrytis_​cinerea/​Home.​html; http://​urgi.​versailles.​inra.​fr/​index.​php/​urgi/​Species/​Botrytis)[4].