Discussion To further investigate the role of AI-2 in the pathogen S. Typhimurium, we evaluated a luxS mutant in a 2D-DIGE proteomics approach. Abolishment of AI-2 production does not cause a drastic change in the proteome of S. Typhimurium in our experimental set-up. Several factors should be kept in mind when interpreting this result. First, a proteome analysis is condition and time point dependent. Second, we used a 2D-DIGE approach to analyze the proteomic

differences. The fluorescent labeling prior to protein separation permits the incorporation buy JNK inhibitor of an internal standard on each gel making differential proteome analysis more accurate [34]. In addition, we chose rather strict cut-off values in our statistical analysis to minimize false positive results. This specific experimental set-up could explain differences with a previously

reported proteomic study on the effect of AI-2 in Salmonella [19]. Finally, the 2DE technique is limited both by the pI and molecular weight range of the first and second dimension, respectively, and by the low abundance of some protein spots which hampers their identification. Nevertheless, 2DE is a powerful high-throughput technique revealing distinct Selleck OSI906 posttranslational modified protein forms which are possibly relevant for the functionality of a protein. We identified two distinct protein forms of LuxS and this led us to examine this protein in more detail, more specifically considering posttranslational modification and subcellular localization.

In previous publications it was FK228 datasheet already mentioned that the exact function and regulation of the LuxS protein, occurring in a wide diversity of bacteria, are probably more complex than anticipated so far [10, 11, 21, 35]. However, apart from structural and catalytic studies, mainly in B. subtilis, the LuxS protein itself has not yet been subjected to further studies [23–26, 36, 37]. The two forms of the S. Typhimurium LuxS protein identified in this study have similar molecular weight, but differing isoelectric points. Point mutation analysis of the conserved cysteine 83 residue confirmed on the one hand its importance in the catalytic activity of S. Typhimurium LuxS and provided on the other hand see more clear evidence that the C83A mutation results in only one form of LuxS. From the latter observation, it can be concluded that the cysteine 83 residue is the subject of posttranslational modification of the wildtype LuxS protein in S. Typhimurium extending an observation previously reported for Bacillus subtilis [23–25]. This result shows that care has to be taken when interpreting putative posttranslational modifications. Although S. Typhimurium LuxS contains a semi-conserved tyrosine phosphorylation motif, our data do not support that tyrosine phosphorylation is involved. The previous study of structure and catalytic mechanism of purified LuxS from the Gram-positive B.