Murine
IL-23 cDNA was subcloned into the vector so as to construct the eukaryotic dual-gene repression vector pcDNA3-IL-23. Bone-derived DCs were obtained from the long bones of extremities of normal C(57)BL/6 mice and were transfected with pcDNA3-IL-23. DCs cultured routinely and IL-23-transfected DCs were co-cultured with apoptotic
tumor cells for 24 h so as to collect sensitized DCs acquiring the
antigen of the apoptotic cells. Primary
pancreatic carcinoma models were created in C(57)BL/6 mice with dimethyl-
benzanthracene so as to obtain
suspension of
tumor cells. Thirty C(57)BL/6 mice were randomly divided into 5 groups: Group I (IL-23-transfected DC
vaccine group, to be injected subcutaneously with IL-23 and apoptotic cells-modified DC
vaccine twice with an interval of 7 d), Group II (apoptotic cells-sensitized DC
vaccine group, to be injected subcutaneously with apoptotic cells-modified DC
vaccine), Group III (IL-23 transfected DC group, to be injected with IL-23 transfected DCs), Group IV (un-modified DC group, to be injected with un-modified DCs), and Group V (control group, injected with
normal saline). Seven days after the second injection
suspension of
tumor cells was injected subcutaneously, and then
tumorigenesis was observed every other day. Another 30 C(57)BL/6 mice were divided into 5 groups as above-mentioned (Groups I - V(1)) and were killed 1 week after the inoculation of
tumor cell
suspension. Their spleens were taken out. The cytotoxic lymphocytes (CTLs) were isolated, co-cultured with IL-25 and apoptotic cells, and then tested for the secretion of
interferon (IFN)-gamma and
IL-4 by ELISA. Thirty C(57)BL/6 mice loading
pancreatic carcinoma were randomly divided into 5 groups as above-mentioned (Groups I - V(2)) so as to observe the survival time.
RESULTS: ELISA showed that the IFN-gamma expression in the supernatant of culture fluid of
IL-23 transfected DCs in Groups I(1) was significantly up-regulated (P < 0.01), and the
IL-4 secretion of Group I(1) and Groups III(1) were both significantly lower than that of Group II(1) (both P < 0.05). The CTL civilities of Group I(1) and II(1) were both significantly higher than those of the other 3 groups (all P < 0.05). Four weeks after the inoculation
tumorigenesis was not seen in Group I and was seen in Groups III and IV with an incidence of 33% - 50%.
Tumorigenesis occurred only 1 week later in Group V. The
tumor sizes of Groups I(2) and II(2) were both significantly smaller than those of the other 3 groups and the survival times of Groups I(2) and II(2) were both significantly lower than those of the other 3 groups (all P < 0.01).
CONCLUSION:
IL-23 helps enhance the presenting ability of DC
antigen.
IL-23 modified
vaccine strengthens the immune response of CTLs against specific
tumor, thus inducing defensive immune response in the host and strengthening their active immune ability.