This is in accordance with a study by Fernandes et al. who showed that the liposomal incorporation of two other triacylated lipopeptides enhanced the proliferation of murine splenocytes [36], which could be attributed to improved adjuvant uptake by the DCs [20] and [21]. The prominent advantage of liposomal encapsulation of CpG correlates excellently with the cellular localisation of the PAM and CpG receptors. Whilst TLR2 is expressed on the cell surface, TLR9 is present in the endosomal compartment. Conceivably, CpG profits more from liposomal delivery than PAM. For PAM this is illustrated in vitro as liposome
encapsulation decreases its ability to stimulate HEK293-CD14/TLR2 cells, probably due to reduced interaction with the receptor. It is known that liposomal incorporation can have a profound influence Anti-diabetic Compound high throughput screening on the immunomodulatory properties of lipoproteins [37]. VX-770 order PAM’s functionality is dependent on different structural components.
The peptide segment linked to the carboxyl terminus of the palmitoyl lipopeptide, the SKKKK sequence, was shown to elevate the adjuvant activity compared to other peptide sequences [38]. Changes to the lipopeptide fatty acid chains, the O-linked fatty acids in particular, appear to have a substantial effect on the signalling through TLRs. The palmitoyl groups (C16) provide better adjuvant activity than longer and shorter fatty acids [39] and [40]. If the interaction of either of these moieties with the TLR2
is disturbed, the adjuvanticity will be diminished. Liposomal encapsulation can also have a positive effect on the adjuvanticity as it improves the solubility of PAM [41] and the DC uptake of OVA, which may improve DC maturation. However, probably due to loss of interaction with the TLR2, this did not enhance the immune response in vivo. For CpG, improved DC uptake of OVA/CpG liposomes facilitates the interaction with the endosomal TLR9 [18] and [42], thereby inducing DC maturation. STK38 The in vivo situation is more complicated. Even though the DCs will preferentially take up the liposomes, the speed and duration of antigen and immune potentiator exposure will differ between the solution and the liposomal formulations. CpG and OVA in solution will probably reach the lymph nodes faster than the liposomes, but only liposomes ensure uptake of CpG and OVA by the same DC, which was reported to influence the type of immune response generated [21]. Indeed, the enhanced DC uptake does result in a more Th1-biased response, which is most pronounced for the CpG-containing liposomes. Similar results were reported by Gursel et al., who showed that co-encapsulation of OVA and CpG in cationic liposomes induced elevated IgG2a titres and IFN-γ secretion compared to free CpG after intraperitoneal injection [43]. It has to be noted that liposome size also affects the Th1/Th2 bias; larger liposomes tend to induce a Th1 shift [44] and [45].