suis persister cells in bacterial colonization of host tissues, general antibiotic tolerance, and recurrent infections. Methods Bacterial strains, media, and growth conditions All bacterial strains investigated in this study (listed in Table 1) were grown in complex Todd Hewitt Broth (THB,

Becton Dickinson Diagnostics) medium at 37°C. If not stated otherwise cryo-conserved bacterial stocks were used in the experiments. Preliminary experiments with see more cryo-conserved and freshly prepared bacterial cultures had revealed no significant differences in persister cell formation assays (data not shown), similar to what has been reported for E. coli[6]. For the preparation of bacterial stocks, overnight cultures were diluted to an optical density at 600 nm (OD600) of 0.02 in fresh THB medium and selleck chemicals further incubated until bacteria reached either the early exponential (exp) or stationary (stat) growth phase as depicted in Additional file 2: Figure S1. Then 19 ml of exponential grown or 4 ml of stationary grown bacterial cultures were collected and centrifuged at 4000 × g for 10 min C59 wnt manufacturer at 4°C. Bacterial pellets were washed once in phosphate-buffered saline, resuspended in THB medium containing 15% glycerol (v/v), and aliquots were immediately shock frozen in liquid nitrogen. Frozen cultures were kept at −80°C until

use and numbers of viable cells were determined by serial plating on sheep blood Columbia agar plates. All antibiotic treatments were performed in chemically defined medium, RPMI 1640 (Life Technologies), which is routinely used in cell culture. Table 1 Bacterial strains used in this study Strain Description Reference S. suis       10 Virulent serotype 2 strain, porcine isolate [56]   10ΔccpA Strain 10 ccpA

mutant; ccpA::EmR [39]   10ΔAD Strain 10 arginine deiminase operon mutant; arcA::SpcR [38]   05ZYH33 Virulent serotype 2 strain, isolate from human outbreak in China [40]   A3286/94 Virulent serotype 9 strain, porcine isolate [41] S. agalactiae       6313 A clinical isolate belonging to serotype III [57] S. gordonii       30   [58] S. pyogenes       A40 A clinical isolate belonging to M type 12 [59] Antibiotics and determination Casein kinase 1 of minimal inhibitory concentration (MIC) Daptomycin (commercial Cubicin®) analytic grade powder was purchased from Novartis Pharma. Penicillin G, ciprofloxacin, amoxicillin, and rifampicin were purchased from Sigma, and gentamicin from Roth. The antimicrobial solutions were prepared freshly prior to each application according to the manufacturers’ recommendations. The MIC of each antibiotic was determined in duplicate by the microdilution technique in 96-well plates. Serial two-fold dilutions of different antibiotics prepared in RPMI 1640 medium were inoculated each with 5 × 105 colony forming units (CFU) of exponential grown cryo-conserved bacteria per well.