| Literature DB >> 26820519 |
Shota Warashina1, Takashi Nakamura1, Yusuke Sato1, Yuki Fujiwara1, Mamoru Hyodo2, Hiroto Hatakeyama3, Hideyoshi Harashima4.
Abstract
Applying small interfering RNA (siRNA) to dendritic cell (DC) based therapy represents a potential candidate for cancer immunotherapy. However, delivering siRNA to DCs is a challenging issue for non-viral vectors. To date, only viral vectors have achieved efficient gene silencing in DCs. We report herein that a novel cationic lipid, YSK12-C4, when loaded in a nanoparticle with siRNA (YSK12-C4 multifunctional envelope type nano device [YSK12-MEND]), greatly facilitated gene silencing in mouse DCs. The use of the YSK12-MEND resulted in a gene silencing efficiency in excess of 90%, with a median effective dose (ED50) of 1.5nM, whereas the maximum gene silencing efficiency of Lipofectamine RNAiMAX was less than 60% and the ED50 was 25nM. Furthermore, suppressor of cytokine signaling 1, an immune suppressive molecule in DCs, silenced in the mouse DC by the YSK12-MEND showed a drastic enhancement in cytokine production, resulting in the significant suppression of tumor growth when it was applied to DC-based therapy against a mouse lymphoma. These results clearly indicate that YSK12-MEND overcomes the obstacle associated with non-viral vectors and can be considered to be a promising non-viral vector for siRNA delivery to DCs, thus accelerating DC-based therapies with siRNA.Entities:
Keywords: Cancer immunotherapy; Dendritic cell; Dendritic cell-based vaccine; Endosomal escape; SOCS1; siRNA nanoparticle
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Year: 2016 PMID: 26820519 DOI: 10.1016/j.jconrel.2016.01.042
Source DB: PubMed Journal: J Control Release ISSN: 0168-3659 Impact factor: 9.776