School of Pharmacy, Jilin Medical University, Jilin, Jilin, 132013, China,
Immunology Department, Laboratory Medical College, Jilin Medical University, Jilin, Jilin, 132013, China.
Int J Nanomedicine. 2018 Sep 19;13:5537-5559. doi: 10.2147/IJN.S172556. eCollection 2018.
Acceleration and improvement of penetration across cell-membrane interfaces of active targeted nanotherapeutics into tumor cells would improve tumor-therapy efficacy by overcoming the issue of poor drug penetration. Cell-penetrating peptides, especially synthetic polyarginine, have shown promise in facilitating cargo delivery. However, it is unknown whether polyarginine can work to overcome the membrane interface in an inserted pattern for cyclic peptide ligand-mediated active targeting drug delivery. Here, we conducted a study to test the hypothesis that tandem-insert nona-arginine (tiR) can act as an accelerating component for intracellular internalization, enhance cellular penetration, and promote antitumor efficacy of active targeted cyclic asparagine-glycine-arginine (cNGR)-decorated nanoliposomes.
Polyarginine was coupled with the polyethylene glycol (PEG) chain and the cNGR moiety, yielding a cNGR-tiR-PEG-distearoylphosphatidylethanolamine conjugate.
The accelerating active targeted liposome (Lip) nanocarrier (cNGR-tiR-Lip-doxorubicin [Dox]) constructed in this study held suitable physiochemical features, such as appropriate particle size of ~150 nm and sustained-release profiles. Subsequently, tiR was shown to enhance cellular drug delivery of Dox-loaded active targeted systems (cNGR-Lip-Dox) significantly. Layer-by-layer confocal microscopy indicated that the tandem-insert polyarginine accelerated active targeted system entry into deeper intracellular regions based on observations at marginal and center locations. tiR enhanced the penetration depth of cNGR-Lip-coumarin 6 through subcellular membrane barriers and caused its specific accumulation in mitochondria, endoplasmic reticulum, and Golgi apparatus. It was also obvious that cNGR-tiR-Lip-Dox induced enhanced apoptosis and activated caspase 3/7. Moreover, compared with cNGR-Lip-Dox, cNGR-tiR-Lip-Dox induced a significantly higher antiproliferative effect and markedly suppressed tumor growth in HT1080-bearing nude mice.
This active tumor-targeting nanocarrier incorporating a tandem-insert polyarginine (tiR) as an accelerating motif shows promise as an effective drug-delivery system to accelerate translocation of drugs across tumor-cell/subcellular membrane barriers to achieve improved specific tumor therapy.
加速和提高主动靶向纳米治疗剂穿过细胞膜界面进入肿瘤细胞的穿透能力,将通过克服药物穿透性差的问题来提高肿瘤治疗效果。细胞穿透肽,特别是合成多聚精氨酸,在促进货物传递方面显示出了希望。然而,目前尚不清楚多聚精氨酸是否可以以插入模式工作,以克服膜界面,用于环肽配体介导的主动靶向药物传递。在这里,我们进行了一项研究,以测试以下假设:串联插入非精氨酸(tiR)可以作为细胞内内化的加速成分,增强细胞穿透性,并促进主动靶向环天冬氨酸-甘氨酸-精氨酸(cNGR)修饰的纳米脂质体的抗肿瘤功效。
将多聚精氨酸与聚乙二醇(PEG)链和 cNGR 部分偶联,得到 cNGR-tiR-PEG-二硬脂酰基磷脂酰乙醇胺缀合物。
本研究构建的加速主动靶向脂质体(Lip)纳米载体(cNGR-tiR-Lip-阿霉素[Dox])具有合适的物理化学特性,如合适的~150nm 粒径和持续释放特性。随后,结果表明 tiR 可显著增强负载 Dox 的主动靶向系统(cNGR-Lip-Dox)的细胞内药物传递。层层共聚焦显微镜表明,串联插入的多聚精氨酸基于边缘和中心位置的观察结果,加速主动靶向系统进入更深的细胞内区域。tiR 增强了 cNGR-Lip-香豆素 6 通过亚细胞膜屏障的穿透深度,并使其特异性积聚在线粒体、内质网和高尔基体中。显然,cNGR-tiR-Lip-Dox 诱导了增强的细胞凋亡并激活了 caspase 3/7。此外,与 cNGR-Lip-Dox 相比,cNGR-tiR-Lip-Dox 在 HT1080 荷瘤裸鼠中引起了更高的抗增殖作用和明显抑制肿瘤生长。
这种包含串联插入多聚精氨酸(tiR)作为加速基序的主动肿瘤靶向纳米载体作为一种有效的药物递送系统具有很大的潜力,可以加速药物穿过肿瘤细胞/亚细胞膜屏障的转运,从而实现改善的特异性肿瘤治疗。
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