No change of the promoter activity of the ampOP operon was observed in the PAOampG mutant. Discussion Members of the Pseudomonadaceae family are intrinsically resistant to β-lactam antibiotics. Earlier reports successfully identified ampC, ampR, ampD, and ampE as genes involved in the β-lactamase

induction mechanism. However, the question of how chromosomal β-lactamase is induced remains elusive. This study examines the role of two previously uncharacterized P. aeruginosa putative permeases. P. aeruginosa harbors two distinct and independent AmpG orthologues In Enterobacteriaceae, besides AmpR, AmpD and AmpE, AmpG has also been implicated www.selleckchem.com/products/ve-821.html in the ampC-encoded β-lactamase induction, acting as a membrane permease that see more transports 1,6-anhMurNAc-tripeptide and 1,6-anhMurNAc-pentapeptide [17]. In P. aeruginosa, two paralogs, PA4393/ampG and PA4218/ampP, were found (Figure 1) [28]. Both ampG and ampP appear to be one member of

two independent two-gene operons (Figures 2 and 3). PFAM analysis of AmpP identifies a Major Facilitator Superfamily (MFS1) domain between amino acids 14 and 346, in agreement with a role in transport [23, 29, 30]. Upstream from ampP is PA4219/ampO, a gene that has seven putative transmembrane domains [23, 31]. Together, these genes form an operon (Figure 3) that is conserved in P. aeruginosa PA14, LES, PACS2, and PA2192 [23, 32]. In contrast, PFAM analysis of AmpG does not reveal any significant hits, however, there was an insignificant match to the MFS1 domain Selleckchem CH5183284 (E = .00018) [29, 30]. The ampG gene is downstream from PA4392/ampF, which encodes a protein with a putative 6-O-methylguanine-DNA methyltransferase domain [23, 33]. These two genes also form an operon (Figure 3) that is conserved in P. aeruginosa PA14, LES, and PA7 [23]. The topology of the E. coli AmpG permease has Morin Hydrate been analyzed using β-lactamase fusion proteins [15]. It was shown that AmpG has ten transmembrane domains with the

amino- and carboxyl-termini localized to the cytoplasm [15]. In accordance with roles as transporters, AmpG and AmpP have 14 or 16 (depending upon the algorithm used) and 10, respectively predicted TM domains. PhoA and LacZ fusion analysis corroborates the existence of 14 and 10 TM domains in AmpG and AmpP, respectively (Figure 4). In AmpG, the predicted transmembrane helices between amino acids 440 and 460 and either 525 and 545 or 555 to 575 of PA4393 are likely false positives. AmpG fusions at amino acids 438, 468 and 495 indicate that these amino acids are cytoplasmic (Figure 4), suggesting that if the region between amino acids 440 and 460 is membrane associated, it may be an integral monotopic domain. Similarly, AmpG fusions at residues 495 and 594 are cytoplasmic, while that at 540 is periplasmic, suggesting that if the region between amino acids 525 and 545 is membrane associated, it may be an integral monotopic domain.