Dakwar George R, Braeckmans Kevin, Ceelen Wim, De Smedt Stefaan C, Remaut Katrien
Ghent Research Group on Nanomedicines, Laboratory for General Biochemistry and Physical Pharmacy, Faculty of Pharmaceutical Sciences, Ghent University, Ottergemsesteenweg 460, 9000, Ghent, Belgium.
Centre for Nano- and Biophotonics, Ghent University, 9000, Ghent, Belgium.
Drug Deliv Transl Res. 2017 Apr;7(2):241-251. doi: 10.1007/s13346-016-0329-4.
Delivery of small interfering RNA (siRNA) is recently gaining tremendous attention for the treatment of ovarian cancer. The present study investigated the potential of different liposomal formulations composed of (2,3-dioleoyloxy-propyl)-trimethylammonium (DOTAP) and 1,2-dioleoyl-sn-glycero-3-phosphoethanolamine (DOPE) encapsulating siRNA (hydration method) for their ability to knockdown luciferase (Luc) activity in human ovarian cancer SKOV-3 cells. Fluorescence single particle tracking (fSPT) and fluorescence correlation spectroscopy (FCS) in human-undiluted ascites fluid obtained from a peritoneal carcinomatosis patient revealed that cationic hydra-lipoplexes (HYDRA-LPXs) and HYDRA-LPXs decorated with stable DSPE-PEG (DSPE HYDRA-LPXs) showed high stability during at least 24 h. HYDRA-LPXs decorated with sheddable C8 and C16 PEG-Ceramides (Cer HYDRA-LPXs) resulted in rapid and premature release of siRNA already in the first hours. Despite their role in preventing aggregation in vivo, liposomes decorated with stable PEG residues resulted in a poor transfection compared to the ones decorated with sheddable PEG residues in reduced serum conditions. Yet, the transfection efficiency of both Cer HYDRA-LPXs significantly decreased following 1 h of incubation in ascites fluid due to a drastic drop in the cellular uptake, while DSPE HYDRA-LPXs are still taken up by cells, but too stable to induce efficient gene silencing.
小干扰RNA(siRNA)递送在卵巢癌治疗中最近备受关注。本研究调查了由(2,3-二油酰氧基丙基)三甲基氯化铵(DOTAP)和1,2-二油酰基-sn-甘油-3-磷酸乙醇胺(DOPE)组成的不同脂质体制剂(水合方法)包裹siRNA后在人卵巢癌SKOV-3细胞中敲低荧光素酶(Luc)活性的能力。对从一名腹膜癌患者获得的未稀释人腹水进行荧光单粒子追踪(fSPT)和荧光相关光谱(FCS)分析发现,阳离子水合脂质复合物(HYDRA-LPXs)和用稳定的二硬脂酰基聚乙二醇(DSPE-PEG)修饰的HYDRA-LPXs(DSPE HYDRA-LPXs)在至少24小时内表现出高稳定性。用可脱落的C8和C16聚乙二醇神经酰胺修饰的HYDRA-LPXs(Cer HYDRA-LPXs)在最初几小时内就导致siRNA快速过早释放。尽管稳定的聚乙二醇残基修饰的脂质体在体内具有防止聚集的作用,但在血清减少的条件下,与可脱落聚乙二醇残基修饰的脂质体相比,其转染效果较差。然而,由于细胞摄取急剧下降,在腹水中孵育1小时后,Cer HYDRA-LPXs的转染效率均显著降低,而DSPE HYDRA-LPXs仍被细胞摄取,但稳定性过高,无法诱导有效的基因沉默。