8% w/v glucose (M9-08% w/v glucose) All solutions were prepared

8% w/v glucose (M9-0.8% w/v glucose). All solutions were prepared using TraceSelect water (Sigma, Poole, UK), ultrapure reagents and sterile plasticware to minimize iron contamination. The culture was grown overnight at Androgen Receptor antagonist 37 °C shaking and diluted 1 : 1000 into M9-0.8% w/v glucose containing varying concentrations of iron (III) nitrate and 100 μM INP0403 or 0.1% v/v DMSO. Two hundred and fifty microlitres of culture was added per well to a 96-well flat-bottomed plate with a lid and the OD600 nm was recorded every 30 min for 24 h in

a Tecan Infinite 200 plate reader (Tecan UK Ltd, Theale, UK), heated to 37 °C. Each sample was assayed in triplicate, and at least four independent biological replicates of the assay were performed. Statistical analysis (Welch two-sample t-test) of the mean data was performed using the r statistical software package, comparing the effect of INP0403 to DMSO alone at each iron (III) nitrate concentration. P-values ≤0.05 were considered significant. To ensure that the growth conditions were strictly iron-dependent, INP0403 was incubated with Chelex100 resin (Bio-Rad, Hemel Hempstead, UK) for 1 h to remove residual iron before use. Salicylidene Ion Channel Ligand Library in vitro acylhydrazides

and related compounds have been reported to impair transcription of T3S loci in Yersinia (Nordfelth et al., 2005), enteropathogenic E. coli (Gauthier et al., 2005) and enterohaemorrhagic E. coli (Tree et al., 2009). In Salmonella, Negrea et al. (2007) proposed that inhibition of secretion via T3SS-1 is due to transcriptional silencing of SPI-1 as reduced expression of chromosomal lacZ fusions to promoters of SPI-1 genes was seen in S. Typhimurium strain TT16729. However, the authors of this report also noted that the inhibitor may impair the secretion competency of T3SS-1 because secretion, but not expression, of a SipB-β-lactamase fusion protein was inhibited, with the SPI-1-encoded fusion protein accumulating

intracellularly (Negrea et al., 2007). However transcription of a chromosomal PJ34 HCl lacZ fusion to sipC in the same operon was repressed approximately 10-fold in the presence of an inhibitor, which is at odds with the absence of effects on SipB fusion protein expression (Negrea et al., 2007). To further investigate the mechanism of salicylidene acylhydrazide-mediated inhibition of Salmonella T3SS-1, we defined the transcriptome of S. Typhimurium under T3SS-1-inducing conditions in the presence or absence of INP0403, which proved to be the most potent inhibitor of T3SS-1 in our previous studies (Hudson et al., 2007). INP0403 is also known as D4 (active against Salmonella T3S; Negrea et al., 2007), compound 11 (active against Yersinia T3S; Nordfelth et al., 2005) and ME0053 (active against E. coli O157:H7 T3S; Tree et al., 2009). The chemical structure of INP0403 has been described (Hudson et al., 2007; Negrea et al., 2007).

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