For co-encapsulation of a TLR ligand, after hydration either PAM

For co-encapsulation of a TLR ligand, after hydration either PAM or CpG was added to a final concentration of 2 mg/ml. The dispersions were dehydrated by freeze-drying and subsequently rehydrated in the same buffer solution to encapsulate the TLR ligands [27]. Extrusion was Libraries performed as described above. The size and zetapotential of the liposomes were determined by dynamic light scattering and laser Doppler velocimetry, respectively,

using a Zetasizer® Nano ZS (Malvern Instruments, UK). The amount of OVA, PAM and CpG present in the liposomes was determined by using their fluorescently INCB024360 labelled analogues (10% of used OVA, PAM or CpG were labelled). The free antigen and TLR ligand were separated from the liposomes by filtration using a Vivaspin this website 2 centrifugal concentrator (PES membrane, MWCO 300 kDa, Sartorius Stedim, Nieuwegein, The

Netherlands) and quantified using a FS920 fluorimeter (Edinburgh Instruments, Campus Livingston, UK). The stability of the OVA-loaded liposomes and OVA release from the liposomes was determined in PBS pH 7.4. Liposomes containing OVAFITC were diluted to a 0.5% lipid concentration and stored at 37 °C under constant stirring. Samples were taken at selected time intervals and the size of the liposomes and antigen encapsulation were measured after filtration. HEK293 cells, stably transfected with human CD14/TLR2 or TLR9 and a NF-κB inducible IL-8 (TLR2) or luciferase (TLR9) plasmid [28] and [29], were maintained in Dulbecco’s Modified Eagle Medium (DMEM), supplemented with 10% fetal calf serum (FCS), others 1 mM sodium pyruvate and 10 μg/ml ciprofloxacin. To the HEK293-CD14/TLR2 cells 5 μg/ml puromycin and to the HEK293/TLR9 cells 700 μg/ml Geneticin (G418) was added as a selection marker. For stimulation experiments, both cell types were seeded at a density of 4.0 × 104 cells/well in 96-well flat bottom plates and stimulated the next day. The cells were stimulated with the formulations containing different concentrations of PAM (maximum

450 ng/ml) or CpG (maximum 10 μg/ml). Medium was used as a negative control. TLR2 stimulation was measured by determining the IL-8 production in supernatants after 24 h using a commercial kit (Sanquin, Amsterdam, The Netherlands), following the manufacturer’s recommendations. The HEK-293/TLR9 cells were stimulated for 6 h with the formulations. The luciferase expression was determined with a luciferase assay kit (Promega, Leiden, The Netherlands) according to the manufacturer’s manual, using a DLReady Berthold Centro XS luminometer (Berthold Detection Systems, Germany). Monocytes were isolated from human donor blood before each experiment by Ficoll and Percoll density centrifugation and depletion of platelets was performed by surface adherence of the monocytes in 24-well plates (Corning, Schiphol, The Netherlands) as described previously [30]. The monocytes were cultured for 6 days at 37 °C and 5% CO2 after seeding at a density of 0.

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