One hundred microliters of heparinized blood in the presence or absence of E. coli (3*108/ml) were incubated for 1 h at 37°C. Then, an anti-human FITC-MPO antibody (20 µl/test) and SYTOX Red (10 nmol/L; Biolegend, USA) were added and incubated for 30 min at room temperature. Images were acquired on an ImageStream Multispectral Imaging Flow Cytometer (Amnis, part of EMD Millipore, USA) using the 40× magnification objective, which provides a numerical aperture (NA) of 0.75 and a pixel dimension of 0.5 m × 0.5 m.
A core diameter of 7 μm was used to maximize in-focus events. The 488 nm and 642 nm excitation laser were used at an output power of 150 mW. Objects with a minimum cross-sectional area of 50 m2 and a maximum of 600 m2 were collected to avoid acquiring debris or cellular aggregates. Typical files contained images of 20,000 cells. Cell images were analysed using IDEAS software, version 6.2. Cells in best focus were selected using the feature Brightfield (BF) Gradient RMS, a measurement of image contrast that excludes out-of-focus events. Doublets, aggregates, dead cells, and debris were excluded using SSC intensity and Syto intensity, and all analyses were restricted to single cells.
A core diameter of 7 μm was used to maximize in-focus events. The 488 nm and 642 nm excitation laser were used at an output power of 150 mW. Objects with a minimum cross-sectional area of 50 m2 and a maximum of 600 m2 were collected to avoid acquiring debris or cellular aggregates. Typical files contained images of 20,000 cells. Cell images were analysed using IDEAS software, version 6.2. Cells in best focus were selected using the feature Brightfield (BF) Gradient RMS, a measurement of image contrast that excludes out-of-focus events. Doublets, aggregates, dead cells, and debris were excluded using SSC intensity and Syto intensity, and all analyses were restricted to single cells.