They have been assayed with moderate success in different therape

They have been assayed with moderate success in different therapeutic settings to treat colorectal carcinoma [29], melanoma [20], gastric [30], bladder [31], ovarian, and breast cancer [32-34]. Viral dsRNA is normally recognized by TLR3 and RLRs in a cell-type and pathogen-type specific manner. TLR3 has been shown to be expressed on human selleck lung carcinoma cells [35] and in lung epithelial cells [36]. Besides, functional expression of TLR3 has been detected in

human prostate cancer cell lines and in murine models of prostate cancer [37-39]. Also, it has been published that TLR3 is intracellularly localized in melanoma cells, where it can deliver proapoptotic and antiproliferative signaling. Poly IC activates the TLR3 pathway leading to suppression of the viability of melanoma cells [20, 40]. The murine melanoma B16 cells have also

been reported to respond to poly AU [29]. We chose the human lung carcinoma cell line A549, the human prostate carcinoma cell line DU145, and the murine melanoma cell line B16 because they were all reported to express TLR3 and to respond to dsRNA therapy. However, the fact that the levels of IFN-β induction upon poly I:C or poly A:U stimulation were capable of improving DC function had not been reported AUY-922 before. dsRNA from engulfed apoptotic infected cells is recognized by TLR3 in endosomes, triggering a MyD88-independent response whereas activation of RLRs by viral dsRNA occurs in cytosol and engages a different set of molecular adaptors [1-3]. However, triggering any of these receptors Diflunisal ends in activation of the transcription factors IRF3 and NF-κB and the production of type I IFNs and pro-inflammatory cytokines. A549 cells and DU145 cells (data not shown) upregulate the expression levels of both TLR3 and RLRs. DU145 and A549 human cancer cells respond to dsRNA analogs, inducing an important IFN response and pro-inflammatory cytokines. Phosphorylation of IRF3 was readily observed as well as phosphorylation of STAT1 24 h after the initial stimulus. The latter indicates that type I IFNs are acting in an autocrine fashion on tumor

cells, as previously described [8, 9]. Interestingly, the expression of type I IFN receptor has been shown in different epithelial tumors but not in sarcomas, lymphomas, and endocrine tumors [41]. We cannot exclude the possibility of a heterogeneous expression of IFNAR among the tumor cell population, which could promote an in vivo selection of tumor cells refractory to type I IFN stimulation. Our results show that IFN-β produced by dsRNA-activated tumor cells can also act in a paracrine fashion, as determined by the presence of pSTAT1 after incubation of MoDCs and BMDCs with dsRNA-CM (Fig. 2 and Supporting Information Fig. 1). PIC-CM by itself was capable of inducing the upregulation of CXCL10 mRNA, CD40, and CD86 expression levels on MoDCs, but not the secretion of IL-12p70.

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