Primary neutrophils and epithelial cells were isolated from the lungs of wild type and Ormdl3 transgenic mice using magnetic bead cell selection for Ly6G‐positive or CD326 (EpCAM)‐positive cells, respectively, exactly as we previously described.18 Epithelial cells were stimulated for 20 h with vehicle or LPS (200 ng/mL), and the neutrophil attachment assay was performed as previously described.18 Transwell inserts (pore size: 5.0 μm; Sarstedt) were used to measure the migration of neutrophils and pre‐coated with laminin. 1.5 × 105 cells were seeded in the top well in serum‐free DMEM and placed on wells containing 100 nM fMLP with S1P (100 nM) or LPS (200 ng/mL) in the lower chamber. The chambers were incubated at 37°C in 5% CO2 for 1 h. Subsequently, migrated neutrophil numbers in lower chambers were determined by removing all cells from the upper chamber and filling the bottom chamber with 100 μL of cell dissociation solution containing 2 μg/mL Calcein‐AM (Life Technologies, CA). The re‐assembled chamber was incubated for an additional 1 h at 37°C. Migrated cells in the fluid of the bottom chambers were quantified by measuring fluorescence of Calcein at 485 nm excitation, 520 nm emission with a TECAN Infinite M1000 fluorescence plate reader (Männedorf, Switzerland).
Infinite m1000 fluorescence plate reader
Manufactured by Tecan
Sourced in Switzerland
The Infinite M1000 is a fluorescence plate reader from Tecan. It is designed to measure fluorescence intensity in multiwell plates. The core function of the Infinite M1000 is to quantify fluorescent signals in biological samples.
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3 protocols using infinite m1000 fluorescence plate reader
1
Neutrophil Migration Assay with Lung Cells
2
Monitoring Liposomal SR-B Leakage
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SR-B leakage from DOPC:4 (1:1) liposomes, before and after light activation, was monitored using a TECAN Infinite M1000 Fluorescence Plate Reader and were performed in 96-well plates (PP Microplate, solid F-bottom (flat), chimney well) at room temperature. Final experimental volume in each well was 200 μL. To monitor SR-B leakage (and dye de-quenching) during photoactivation, fluorescence emission (excitation: 520 nm; emission: 580 nm) was measured every 20 s for 600 s, the sample was then irradiated (20 mins, 370 ± 7 nm, 202 mW cm−2) in a quartz cuvette, with the LED mounted at a distance of 1 cm from the sample, returned to the 96-well plate and fluorescence emission measured for a further 10 mins. After this, Triton X-100 (10 μL, 1% w/v) was added to the sample well (10 s agitation) to solubilize liposomes and release any remaining encapsulated SR-B.
3
Neutrophil Migration Assay in Lung Cells
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