For example, MalF, an inner membrane maltose and maltodextrin transport protein, and MalQ, a dextrinyl transferase, have been associated with the expression of cholera toxin and toxin-co-regulated pilus in Vibrio cholerae
[8], as has been LamB with cytopathic effect in enteropathogenic E. coli [9], and adhesion in enteroinvasive E. coli [10] and Aeromonas veronii [11]. Mutants of the malE and malT (transporter) genes in group A Streptococcus are attenuated in their ability to grow in human saliva and to metabolize α glucans and are significantly impaired in their ability to colonize the mouse oropharynx [12, 13]. To elucidate the role of the predicted maltose regulon in A. pleuropneumoniae, malT and lamB knockout mutants were constructed and characterized phenotypically. Since MalT is a regulatory protein, the effect of its knockout on the bacterial gene expression level was also determined using DNA microarrays. Results
Expression PF-6463922 nmr of maltose-regulon genes by the wild-type A. pleuropneumoniae CM5 in BALF Several differentially expressed genes in A. pleuropneumoniae CM5 exposed to BALF for 30 min at 37°C were first presumptively identified by RT-PCR DD studies. These included genes encoding selleck products protein synthesis and hypothetical proteins (APL_068, APL_0363, and APL_0367), in addition to a cell surface protein, LamB (Figure 1). Homologs (>99% DNA identity) of the 3 hypothetical proteins are present in all the serotypes of A. pleuropneumoniae sequenced so far, suggesting that they might have a role in persistence or pathogenesis, but their levels of expression were not confirmed by real-time PCR or other more direct Cediranib (AZD2171) methods. The level RAD001 of expression of the lamB gene was estimated by real-time PCR analysis to be 3.3-fold higher in BALF- than in BHI-exposed cells (Table 1). Genes of the maltose regulon that were also up-regulated (although some at very low levels) in BALF-exposed cells included malF and malG (encoding the intrinsic membrane proteins of maltose transport system),
malP (maltodextrin phophorylase), malQ (amylomaltase) and malK (the ATP-binding cassette of the maltodextrin transporter; Table 1). For further study, we constructed lamB and malT mutants to evaluate the possible role of these genes in the survival of A. pleuropneumoniae CM5. Table 1 Differential expression of maltose-regulon genes in BALF-exposed A. pleuropneumoniae CM5 Gene Putative function ΔΔCT ± SD Fold-change* malE (T) Periplasmic maltose binding protein -2.82 ± 0.51 7.06 (4.95-10.05) malE (R) 0 ± 0.84 1 (0.55-1.79) malF (T) Intrinsic membrane protein of maltose transport system -2.79 ± 1.01 6.91 (3.43-13.92) malF (R) 0 ± 0.39 1 (0.76-1.31) malG (T) Intrinsic membrane protein of the maltose transport system -2.6 ± 0.40 6.06 (8-4.59) malG (R) 0 ± 0.40 1(0.76-1.31) malK (T) ATP-binding protein of the maltodextrin transporter -1.10 ± 0.39 2.14 (1.6-2.8) malK (R) 0 ± 0.76 1(0.59-1.