Fig. (5) qRT-PCR analysis to determine LSMMG-induced alterations of gene expression in Enterobacteriaceae. Total RNA harvested from LSMMG and control cultures was converted to single-stranded cDNA and used as template in qPCR analysis with primers hybridizing to the indicated genes as described previously [3, 18]. PCR product levels were normalized to both the 16S rRNA and lpxC genes [3, 34], and a ratio of each gene level for LSMMG to control was calculated to give a fold-difference in expression between the two samples as previously described [3]. Differences in expression between LSMMG and control samples were significant at p-value < 0.05. The data was obtained from at least four qPCR reactions using RNA from at least two independent cultures for each condition, and the data is plotted as the average and standard deviation.