Figure 1 Agarose click here gel electrophoresis and Southern blot hybridization of DNA preparations of 18 STEC strains. A) plasmid preparations (left side) and Southern blot hybridization with a subAB 1 specific DNA probe (right side). Gene Ruler 1 kb DNA ladder (M), Lambda-Mix Marker 19 (Mλ) (both Fermentas), K17 (lane 1), LM25602/08 (2), CB11588 (3), CB11633 (4), TS20/08 (5), TS26/08 (6), SF16b (7) TS18/08 (8), TS30/08 (9), EDL933 (10). B) chromosomal DNA (left side) and Southern blot hybridization with a subAB 2 specific DNA probe (right side). Gene Ruler 1 kb DNA ladder

(M), Lambda DNA/HindIII Marker (MλH) (Fermentas), LM14603/08 (1), LM16092/08 (2), LM227553stx1 (3), LM227553stx2 (4), LM27564 (5), Ferrostatin-1 price LM27558 (6), LM27555 (7), LM14960 (8), LM27558 (9). EDL933 (10) was used as a negative control for hybridization. Recombinant plasmid pK18 containing subAB 1 was used as positive control for hybridization

(data not shown). PCR analysis of subAB and adjacent DNA regions All STEC strains were analyzed by PCR with specific primers directed to the subAB operon or flanking regions of the two recently described subAB alleles [8, 16] (Figure 2). PCR-products were confirmed by DNA-sequencing. For the detection of plasmid-located subAB 1, primer pair subAB-for5/subAB-rev5 (Figure 2A) was used to amplify the complete ORF, including a region 202 bp upstream and 194 bp downstream of subAB 1. The nine strains with plasmid-located subAB 1 yielded a PCR product of the expected size of 1821 bp, indicating the presence of the subAB 1 variant Rucaparib in vitro MK 1775 and complete ORFs in these strains (data not shown). Moreover, saa was present in these strains indicating a similar

genetic arrangement as previously described [8]. Figure 2 Schematic illustration of the different genomic loci of subAB . A) plasmid locus of subAB 1 of E. coli O113:H21 strain 98NK2 (GenBank Acc. No. AY258503) with three putative genes located upstream of the subAB operon and primer binding sites 202 bp upstream and 194 bp downstream of the operon. B) genomic locus of subAB 2-1 of E. coli O78:H- strain ED32 (Acc. No. JQ994271) with the tia gene of the SE-PAI located 789 bp upstream of the operon and primer binding sites 1336 bp upstream and 316 bp downstream of the operon. C) locus of the new (subAB 2-2 ) operon of E. coli O76:H- strain 1.2264 (Acc. No. AEZO02000020.1) with an outer membrane efflux protein as part of a type 1 secretion system located 1496 bp upstream of the subAB operon and primer binding sites 1235 bp upstream and 65 bp downstream of the operon. Primers subA-L and subAB2-3′out (Table 1) were used to generate a template for sequencing. Since it has been reported that the chromosomal subAB 2 variant of STEC strain ED32 was linked to the tia gene in the chromosomal island SE-PAI [16], corresponding primers were used to test the hypothesis whether the remaining 9 strains contained this particular variant (for a scheme see Figure 2B).