Cytospin centrifugation was performed at 600 r.p.m. for 5 min and the slides were stained with modified Wright’s stain (Hema 3® Stain Set, Fisher) according to the manufacturer’s instructions. Approximately 100 cells from several microscope fields (5–6) were counted and identified for each sample. Clodronate (kindly provided by Roche Diagnostics GmbH, Mannheim, Germany) was incorporated into liposomes from a 250 mg mL−1 solution as described previously (Van Rooijen & Sanders, 1994). Anesthetized mice were inoculated intranasally with 100 μL clodronate-containing liposomes (CL)
or PBS-containing liposomes (PL). Macrophage depletion was determined by analysis of BAL fluid cells as described above, and was routinely >90%. Neutrophil depletion was conducted in mice using 1 mg of rat monoclonal antibody RB6 administered by an intraperitoneal injection. The RB6 antibody RAD001 solubility dmso is specific for Ly-6G (Gr-1), a marker that is expressed predominantly on neutrophils. Mice were treated with antibody 1 day before intranasal Napabucasin chemical structure bacterial inoculation and every other day subsequently until euthanization.
Control mice were treated with 1 mg of purified rat immunoglobulin G (IgG; Sigma). Neutrophil depletion was confirmed by the analysis of BAL fluid cells in infected mice and was routinely >95%. The advantage that one strain has over another in a mixed infection can be measured by calculating the CI. CI is defined as the ratio between strain
A (in our case B. parapertussis) and strain B (B. pertussis) in the output, i.e. recovered from the respiratory tract, divided by the ratio of strain A and strain B in the input (the ratio in the inoculum). Dynein Comparisons between the mean bacterial loads were analyzed using a t-test, and CIs were log transformed and analyzed using a t-test (vs. a theoretical value of 1). To compare the effect of mixed infection with B. pertussis and B. parapertussis with single strain infections with either pathogen, 6-week-old Balb/c mice were inoculated intranasally with 50 μL of a suspension containing 5 × 105 CFU of B. pertussis and 5 × 105 CFU B. parapertussis (mixed infection), or with 50 μL of a suspension containing 5 × 105 CFU of either organism (single strain infection). Seven days postinoculation (near the peak of bacterial loads in single infections), mice were euthanized and the bacterial load of each pathogen in the respiratory tract was determined. As shown in Fig. 1a, B. pertussis loads were significantly lower in the mixed infection than in the single strain infection. In contrast, B. parapertussis loads were significantly higher in the mixed infection than in the single strain infection, and in the mixed infection, B. parapertussis significantly outcompeted B. pertussis, with a mean of ninefold more CFU recovered from the murine respiratory tract.