Fig. 1

PCR amplifications using P. mirabilis cells and non-P. mirabilis cells as templates and ureRF1 and ureRR1 as primers. Templates used were the cells of E. hormaechei Pd9 and E. cloacae V2 (lanes 1 and 2); Acinetobacter sp. HS51 and A. calcoaceticus T32 (lanes 3 and 4); Klebsiella sp. Pd2 and K. pneumoniae Pd8 (lanes 5 and 6); Vibrio sp. V134, V. harveyi T4, V. parahaemolyticus BL, V. ichthyoenteri BX (lanes 7–10), E. tarda T2 (lane 11); Pseudomonas sp. J61 and DX7, P. plecoglossicida DJ3, P. aeruginosa YK, P. putida SP1 (lanes 12–16); P. stuartii Ps1 (lane 17); Escherichia sp. HS21 and E. coli Top10 and HS11 (lanes 18–20); P. mirabilis V7, SW11 and SY2 (lanes 21–23); DNA marker (lane 24)