The binding energies of the wild-type and L138P lactamases toward penicillin and ampicillin were calculated using Calculate Binding Energies protocol with default parameters except that ligand minimization were performed to consider the flexibility of residues within binding sites and implicit solvent model was set to Generalized Born method. Figure 1 Structures of penicillin G (A) and ampicillin (B). Results Antimicrobial resistance phenotype and genotype E. coli 485 exhibited resistance to the commonly used antimicrobial find more agents on farms. The Disk diffusion test showed reduced inhibition zone diameter to cefotaxime (CTX), ceftazidime(CAZ), ceftiofur (CEF) but not to
cefoxitin (FOX). This strain exhibited >5 mm increase in inhibition zone diameter of both cefotaxime and ceftazidime in the presence of amoxicillin/clavulanic acid (AMC) in contrast to when the antibiotics were tested alone. RG E. coli cells carrying bla SHV-1, blaSHV-(L138P), bla this website SHV-33 and bla SHV-33(L138P) exhibited variable zone diameter to penicillin and ampicillin in the disk diffusion test. No decrease in zone diameter
was noticed for cefotaxime (CTX), ceftazidime(CAZ), ceftiofur (CEF) and cefoxitin (FOX). The MIC values for all E. coli strains are listed in table 2. Genotype analysis of E. coli isolate showed TEM and SHV β-lactamase genes showed 100% identity to bla TEM-20 and bla SHV-1 genes except at position 138 where leucine (L) to proline (P) polymorphism was detected. Table 2 Phenotype and genotype of β-lactamases for the E. coli field isolate and mutants included HDAC inhibitor in the study Inhibition Zone diameter (mm)/MICs (mg/L)a β-lactamases Strains AM PEN CEF FOX CAZ CTX SHV TEM E. coli ≤1/640 ≤1/640 8/320 15/20 11/160 12/320 SHV-1(L138P) TEM-20 RG E. coli-M1 12/160 1/40 – - – - SHV-1 RG E. coli-M2 28/40 14/40 – - – - L138P RG E. coli-M3 11/160 1/160 – - – - P226S RG
E. coli-M4 28/20 12/2 – - – - L138P P226S aAmpicillin (AM), penicillin (PEN), ceftiofur (CEF), cefoxitin (FOX), ceftazidime (CAZ), cefotaxime (CTX) Site directed mutagenesis of blaSHV-1 Depsipeptide mw genes After cloning and confirmation of bla SHV-1 genes in the pET 200 cloning and expression vector, reverse mutation at single point (L138P) was successfully performed by site directed mutagenesis to generate bla SHV-(L138P). Plasmid carrying bla SHV-1 gene was used to generate another mutation (S226P) that showed complete identity to bla SHV-33 gene. Sequence analysis also showed that the final site directed mutagenesis on the plasmid carrying bla SHV-33 gene, gave rise to the bla SHV-33(L138P). Cloning, expression and β-lactamase activity assay All four pET 200 cloning and expression vectors carrying bla SHV-1, bla SHV-1(L138P), bla SHV-33 and bla SHV-33(L138P) genes expressed in Rossetta-gami E. coli cells.