These findings are consistent with previously published data in w

These findings are consistent with previously published data in which 7.1% of the X. bovienii-SF43 genome and 4.6% of the X. nematophila genome match with ORFs identified as phage related (Ogier et al., 2010). All of the described phage clusters BTK inhibition match with phagic modules previously identified with the RGPFinder web tool, which identifies large regions of genomic plasticity. The xbp1 cluster encodes the main tail synthesis proteins including the tail sheath (XbpS1), tube (XbpT1), and tail fiber (XbpH1) proteins. To determine whether

the xbp1 phage gene cluster encoded a mitomycin C-inducible xenorhabdicin, the xbpS1 sheath gene was inactivated. PEG-precipitated tail structures prepared from the SF43 and SF70 (xbpS1) strains were analyzed by SDS-PAGE gel electrophoresis. Figure 3 shows that the preparation from SF43 contained

43 and 98 kDa proteins that were identified by N-terminal sequence analysis as XbpS1 and XbpH1, respectively (lane 1). We were unable to resolve the identity of the 65-kDa protein by N-terminal sequencing. In the xbpS1 strain, the level of the 43-kDa protein band was dramatically reduced but not completely eliminated (lane 2). The identity of this additional 43-kDa protein could not be resolved by MALDI-TOF MS analysis. TEM analysis showed that phage tail structures were not produced CHIR 99021 in the SF70 strain (data not shown). Interestingly, inactivation of xbpS1 did not reduce XbpH1 production (Fig. 3), suggesting that xbpH1 was expressed, and XbpH1 fiber and baseplate structures were assembled in the xbpS1 strain. This result was similar to that observed with the ΔxnpS1 strain of X. nematophila (Morales-Soto & Forst, 2011). Phage tail preparations were PEG-precipitated from the SF43 and SF70 strains and assayed for antimicrobial activity against Photorhabdus luminescens enough TT01 and Xenorhabdus bovieni SF31 (Table 1). Preparations derived from the SF43 strain displayed a high level of activity against P. luminescens TT01 and X. bovienii-SF31 (Table 2), while antimicrobial activity was dramatically reduced in the preparations derived from SF70. These findings indicate

that Xbp1 xenorhabdicin was responsible for antimicrobial activity against susceptible competitors. The tail synthesis genes of xnp1 and xbp1 are highly conserved. The sequence identity for the 12 proteins encoded by the genes located between the cI and gpI genes ranges from 77% to 95%. The respective sheath proteins, XnpS1 and XbpS1, share 94% identity and the XnpT1 and XbpT1 tube proteins share 98% identity. The 5.9 kb insertion in the region neighboring fun(Z) contains 11 ORFs and is located between the tail fiber gene xbpH1 and the tail sheath gene xbpS1. It contains three truncated tail fiber ORFs (Ff–Fh) and three tandem transposase genes. As described previously, the xnp1 remnant P2 prophage encodes the tail sheath (XnpS1), tube (XnpT1), and tail fiber (XnpH1).

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