hago cytosis, processed peptides are being cross presented to CD

hago cytosis, processed peptides are being cross presented to CD8 T cells by DCs. A recent report by Blanch��re et al. suggested in a murine model that apoptotic cells may be critical in processing Ags for cross presentation, in essence by pre selection of immunologically important antigenic determinants. In this view, our results in the human setting further support this hypothesis, since tumor dying cells can be used as a source of processed tumor determinants for DCs loading and cross presentation to CTLs. Furthermore, presenta tion by DCs of Ags generated in apoptotic melanoma cells has the potential benefit that presentation via HLA class II may generate helper epitopes that support the develop ment of specific CD4 lymphocytes that might be impor tant for antitumoral immunity.

Drug_discovery We cannot address if Ag peptides are being processed into Apo Nec cells and then taken up by DCs and presented in the HLA class I conte t or if DCs have processed them after Apo Nec phagocyto sis. Besides, tumor derived e osomes loaded onto DCs have been shown to trigger MART 1 melanoma Ag cross presentation to specific CTLs Although we used washed Apo Nec cells resuspended in fresh AIM V medium in all e periments and a differential ultracentrif ugation of culture supernatants is required to obtain tumor derived e osomes, we cannot e clude the contribu tion of e osomes that might be released by Apo Nec cells during the 48 hs co culture with DCs. Nevertheless, our main objective has been to assess if this particular mi ture of Apo Nec cells was able to be phagocytosed by iDCs, induce iDCs maturation, migration and cross pres entation of native tumor peptides to specific CD8 T cells.

We have also evaluated DC Apo Nec cells migration to MIP 3 as a measure of their potential homing to lymph nodes. Upon phagocytosis, DCs must reach the lymph nodes in response to chemokine concentration gradients such as MIP 3 in order to prime na ve T cells. It was important to asses if DC Apo Nec could respond in vitro to MIP 3?. We found that like fully mature LPS treated DCs, DC Apo Nec cells up regulated MIP 3 receptor and efficiently migrated in vitro to MIP 3 but not to MIP 1. Our results are coincident with those reported by Hirao et al, who found specific DCs migration to MIP 3 in vitro and in vivo and CCR7 induction after phagocy tosis of UV treated fibrosarcoma cells.

The production of the pro inflammatory cytokine IL 12 requires two signals IFN and a maturation signal pro vided by CD40 ligation or LPS. Recently, u et al have proposed that Toll like receptor 8 pro vides a priming signal for high production of IL 12. Pro duction of IL 12 and IL 10 influences DCs maturation and the induction of a potent immune presentation to T cells. Accordingly, we found that upon phagocyto sis of Apo Nec intracellular pro inflammatory IL 12 tran siently increased while IL 10 did not change in DC Apo Nec cells. We believe that our results complement the e isting reports about the use of apoptotic a

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