aureus strains and the daptomycin susceptible parent (when available and confirmed isogenic by PFGE). Strains were grown to early exponential phase in 20 mL of SMHB, pelleted, washed twice with HEPES buffer (pH 7.2, containing 50 mg/L Ca2+) and then re-suspended in HEPES (OD600 = 0.2). Aliquots were transferred to a cuvette containing a stir
bar, then KCl (100 mM) was added and the cuvette was placed in the heated chamber of a FluoroMax-3 spectrofluorometer (λ ex = 622 nm and λ em 670 nm at 37 °C) (Horiba Jobin–Yvon Inc., Edison, NJ, USA). Cells were incubated with the membrane potential-sensitive dye DiSC3 (0.1 mg/mL) for 10 min. Conditions included no antibiotic, nisin (25 mg/L) and daptomycin (8 mg/L). The selleck products membrane-depolarizing Momelotinib supplier activity of daptomycin over 60 min was calculated as follows: % depolarization = [(F d − F c)/(F n − F c)] × 100, where F d, F c and F n are fluorescence measurements with daptomycin, no antibiotic and nisin, respectively. Results are expressed as the mean of two independent experiments. This article does not contain any studies with human or animal subjects performed
by any of the authors. Results MICs as determined by both Microscan and BMD for the twelve DNS S. aureus isolates are displayed in Table 1. As can be seen, all isolates had the Microscan MICs confirmed by BMD (within 1 tube dilution standard error). The spread for MIC values was as follows: three isolates with 2 mg/L (Microscan) and 1 mg/L (BMD), three isolates with 2 mg/L (Microscan/BMD), three isolates with 4 mg/L (Microscan) and 2 mg/L (BMD), and three isolates with 4 mg/L (Microscan/BMD). All isolates were stable over five NVP-BGJ398 mw serial passages on drug free TSA. Etest MICs confirmed the daptomycin MIC value within 1 tube dilution. Examination
of the twelve isolates by daptomycin population analysis revealed both left-shift and right-shift profiles within the 4 MIC value groups (Fig. 1a–d). Additionally, Thymidylate synthase the daptomycin AUC values (Table 1) increase as the MIC values increase (Table 1). Retesting of the isolate’s daptomycin MIC values by BMD after greater than 2 years of storage at −80 °C revealed that the MIC values were stable (±1 tube dilution standard error) for 11/12 isolates (Table 1). One isolate, R6827, displayed a daptomycin MIC decrease from 4 to 0.5 mg/L on retesting after storage. Table 1 Minimum inhibitory concentration values, daptomycin population analysis area under curve (AUC) values and molecular characteristics Isolate MIC value (mg/L) DAP AUC SCCmec USA PVL AGR Initial Storage Microscan BMD BMD Type Function R6297 2 1 1 14.01 2 − − 2 − R6515 2 1 1 16.87 2 − − 2 − R6738 2 1 1 18.08 4 300 + 1 − R6212 2 2 2 18.45 2 − − 2 + R6737 2 2 2 20.03 2 − − 2 − R6516a 2 2 2 22.09 4 − − 1 − R6003 4 2 4 22.14 2 − − 2 − R6253 4 2 2 23.66 4 300 + 1 + R6747 4 2 2 22.28 2 − − 2 − R6219 4 4 2 20.68 4 300 − 1 + R6255 4 4 4 26.85 2 − + 2 − R6827 4 4 0.5 21.