The reaction mixture was stirred at room temperature for 3 h then

The reaction mixture was stirred at room temperature for 3 h then purified on silica coated preparative thin-layer chromatography. Selleckchem CYC202 After removal of the p-methoxybenzyl protection group, Reversed Phase-High Performance

Liquid Chromatography was performed to yield β-LEAF in high purity (>95%). Concentrated stocks were prepared in 100% DMSO and stored at −20°C. β-LEAF- antibiotic fluorescence assay Bacterial strains were cultured on BHI agar plates in the presence of a penicillin disk (10U) overnight. For each bacterial isolate, colonies closest to the penicillin disk were transferred to PBS to make a homogenous suspension [~109 Colony Forming Units (CFU)/ml]. Bacterial O.D. was measured at 600 nm. 100 mM antibiotic solution (4X stock) was prepared by dissolving the antibiotic powder in PBS, and 20 μM β-LEAF probe solution (2X stock) was prepared in 40% DMSO in PBS. The assays were phosphatase inhibitor performed in 96-well white clear-bottom plates in a total volume of 100 μl respectively, to include bacteria and 10 μM β-LEAF probe, with or without 25 mM antibiotic (cefazolin). Each reaction was set up as follows: 25 μl bacterial suspension, 25 μl antibiotic 4X stock solution or PBS only and 50 μl probe 2X stock solution, with Alisertib resultant buffer concentration as 20% DMSO in PBS in each 100 μl reaction. For each isolate, reactions

were performed in triplicate in the absence and presence of test antibiotic respectively. Time course assays were carried out, monitoring β-LEAF cleavage by measuring fluorescence for 60 min, at 1 min intervals (Spectramax M5 Plate Reader, Molecular Devices). selleck screening library Instrument settings were kept as excitation 640 nm, emission 700 nm and temperature was maintained at 37°C throughout. β-LEAF cleavage rate in each case was determined as slope i.e. fluorescence change as a function of time (obtained from instrument software – SoftMax Pro5), normalized by bacterial

O.D. For multiple antibiotic testing, reactions were similarly set up with β-LEAF only, and with β-LEAF and cefazolin, cefoxitin or cefepime in separate reactions. S. aureus ATCC strains with established β-lactamase status, β-lactamase producing strain 29213 (#1), and β-lactamase negative strain 25923 (#2), were used as positive and negative control strains respectively in all assay sets. Bacteria-free controls (PBS only) were also included in each assay set. For ‘un-induced’ growth cultures, bacterial strains/isolates were cultured on non-selective BHI agar plates, with the rest of the protocol remaining unchanged. Nitrocefin disk test for detection of β-lactamase The experiments were performed using cefinase disks (nitrocefin disks) as per manufacturer’s recommendations. Briefly, S. aureus isolates grown on agar plates in the presence of penicillin disks (to induce and enhance β-lactamase production) respectively were used.

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