However, pre-treatment with individual chemokines at 50 ng/ml or combinations of CCL3 + 19 Selleckchem PR 171 (5 : 5) or (3 : 7) did not induce antigen degradation levels that were statistically different from those seen after only LPS treatment. Upon pre-treatment with chemokines or subsequent treatment with LPS, profiles of cytokines (IL-1β, TNF-α, IL-12p70, IL-23, IL-10 and IL-4) released into the supernatants of DCs were measured by ELISA. After subsequent
LPS treatment, iDCs pre-treated with individual chemokines or chemokine combinations secreted IL-1β (Fig. 8a) and TNF-α (Fig. 8c) at levels that were statistically no different from iDCs treated only with LPS. Only the combination
of CCL3 + 19 (7 : 3) induced IL-1β secretion at a level higher (50%) than untreated iDCs before LPS treatment, whereas TNF-α was below detectable limits for all DCs before LPS treatment. Secretion levels of both IL-12p70 and IL-23 were below detectable limits for all DCs after just chemokine treatment (Fig. 8d,e). However, after subsequent LPS treatment, individual CCL3 or CCL19 AZD9668 molecular weight or a combination of CCL3 + 19 (5 : 5) induced IL-12p70 secretion at levels lower than iDCs treated only with LPS, whereas only the combination of CCL3 + 19 (7 : 3) induced IL-23 secretion at a level higher than iDCs treated only with LPS. While combinations of CCL3 + 19 (3 : 7) or (7 : 3) induced IL-10 secretion at a level higher than untreated iDCs before LPS treatment, all the treatments of iDCs exhibited IL-10 secretion levels similar to iDCs treated only with LPS after subsequent LPS treatment (Fig. 8b). In addition to these cytokines, IL-4 secretion was also measured but IL-4 secretion levels of all
DCs for both cases before and after LPS treatment were not detectable (data not shown). Results here indicate that chemokine pre-treatment can program DCs to internalize and process antigen, even after DC maturation by LPS. The pre-treatment of DCs with CCL3 + 19 (7 : 3) for 24 hr followed by subsequent LPS treatment for another 24 hr induced the endocytic capacity of DCs at levels ADP ribosylation factor 96% higher than iDCs that were only exposed to LPS. Our finding differs from that reported for the simultaneous application of antigen or dextran and chemokines, which enhanced DC endocytic capacity but only for less than an hour after treatment.[36, 49] Our results indicate that prolonged presence of chemokines in the cell culture well can modulate DC phenotypes against subsequent TLR stimulation. Chemokines are known for their role in chemotaxis; inducing DC migration to the secondary lymphoid organs to present antigens to T cells, thereby initiating the adaptive immune response.