However, plasmids are poorly understood in Xanthomonas spp. beyond the knowledge that they are often carriers of important virulence/avirulence genes (Vivian et al., 2001; Sundin, 2007), including avrBs1 (Stall et al., 1986; Swanson et al., 1988) and avrBs3/pthA (Bonas et al., 1989; Kim et al., 2006). Up to six avirulence genes were found clustered on a 90-kb plasmid in X. campestris pv. malvacearum strain Proteases inhibitor XcmH1005 (De Feyter & Gabriel, 1991). Plasmids in xanthomonads have been reported to carry determinants for resistance to copper or streptomycin (Stall et al., 1986; Minsavage et al., 1990), standard compounds used for bacterial plant disease control (McManus et al., 2002; Hopkins, 2004).

Indications of a 26.7-MDa plasmid were reported in the 1980s in strains of X. arboricola pv. pruni from the United States (Kado & Liu, 1981; Lazo & Gabriel, 1987; Randhawa & Civerolo, 1987), but further characterization of this plasmid stalled. We recently observed a similarly sized plasmid in the

European X. arboricola pv. pruni strain CFBP 5530. The objectives of this study were to sequence Dapagliflozin nmr and annotate this plasmid, conduct comparative genomic analysis against known Xanthomonas plasmids and complete chromosomal sequences, ascertain the prevalence among X. arboricola pv. pruni genotypes and determine whether it is unique to this pathovar, and thus may offer a means for identification at the pathovar level, discrimination that is not possible with currently available molecular diagnostic methods. Xanthomonas strains were routinely

grown on peptone yeast extract glycerol agar (NYGA) (Turner et al., 1984) and peptone yeast extract glycerol broth (NYGB) with incubation at 28 °C for 24–48 h. The presence of plasmid pXap41 was first confirmed in representative strains of X. arboricola pv. pruni with the plasmid profile determined after plasmid DNA extraction, as MRIP described in Zhou et al. (1990), and restriction with EcoRI (Fermentas SA, Mont-sur-Lausanne, Switzerland) according to the manufacturer’s instructions. Restriction products were then separated by electrophoresis on a 1% agarose gel containing ethidium bromide. For screening its presence in a larger number of strains, a pXap41-specific multiplex-PCR was established. For this purpose, primers targeting genes involved in pXap41 replication and mobilization were designed using the program fastpcr v5.4. A geographically and genetically representative collection of 35 X. arboricola pv. pruni isolates covering the full range of described genotypes (Zaccardelli et al., 1999; Boudon et al., 2005) and two strains each of six additional X. arboricola pathovars (Table 1) were screened for the presence of pXap41. The identity of all X. arboricola pv. pruni strains was confirmed using a duplex-PCR assay (Pothier et al., 2011) before screening for plasmid presence. Amplifications were carried out in a final volume of 20 μL using AccuStart PCR SuperMix (Quanta Biosciences, Gaithersburg, MD) and 0.2 μM of each primer.