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基于聚乙二醇-聚(二硫键-赖氨酸)的氧化还原响应性阳离子聚合物用于高效基因转染。

A PEG-b-poly(disulfide-l-lysine) based redox-responsive cationic polymer for efficient gene transfection.

机构信息

School of Chemical Engineering and Technology, Tianjin University, Yaguan Road 135, Tianjin 300350, China.

出版信息

J Mater Chem B. 2019 Mar 21;7(11):1893-1905. doi: 10.1039/c8tb03226b. Epub 2019 Feb 14.

DOI:10.1039/c8tb03226b
PMID:32255052
Abstract

Gene therapy is concerned with the transfer of complement genes to functionally defective cells in a safe and directed manner for the treatment of the most challenging diseases. But safety issues and low transfection efficiency of the gene vectors are the major challenges, which need to be overcome. Recently, redox-responsive bioreducible polymers containing disulfide linkages have been considered as efficient gene vectors, owing to the selective degradation of the disulfide bond in the reducing environment of the cells. This enables spatiotemporal release of pDNA with no or minimum toxicity. Herein, we reported a bioreducible poly(ethyleneglycol)-b-poly(disulfide-l-lysine) cationic polymer (denoted as PEG-SSL) via a Michael addition reaction of poly(ethyleneglycol)tetraacrylate PEG(Ac) and the terminal amine group of poly(disulfide-l-lysine). PEG-SSL efficiently condensed the plasmid ZNF580 gene (pZNF580) forming nano-sized polyplexes (155 ± 4 to 285 ± 3 nm) with zeta potentials of 1.9 ± 0.1 to 26.7 ± 0.4 mV. PEG-SSL successfully retarded pZNF580 at a small polymer/pDNA weight ratio of 10/1 and higher. When exposed to a reducing environment of 5 mM DTT, it rapidly released genes even at higher weight ratios of the PEG-SSL polymer in the PEG-SSL/pDNA complexes. The PEG-SSL/pZNF580 complexes exhibited good stability when exposed to DNase I and efficiently protected pDNA from degradation. In vitro transfection and cytotoxicity were investigated in EA.hy926 cells. The results showed that PEG-SSL successfully delivered pZNF580 into the cells with less cytotoxicity compared to PEI25kDa. The flow cytometry and confocal scanning laser microscopy results indicated that PEG-SSL polyplexes exhibited good cellular uptake and nuclear co-localization rates. All these results implied that PEG-SSL had the potential as a non-viral vector for gene transfection.

摘要

基因治疗涉及以安全和定向的方式将补体基因转移到功能缺陷细胞中,以治疗最具挑战性的疾病。但是,基因载体的安全性问题和转染效率低是主要挑战,需要克服。最近,含有二硫键的氧化还原响应性生物可还原聚合物已被认为是有效的基因载体,因为在细胞的还原环境中二硫键选择性降解。这使得 pDNA 能够以最小的毒性或无毒性进行时空释放。在此,我们通过聚乙二醇四丙烯酸酯 PEG(Ac)的末端丙烯酰基与聚(二硫键-l-赖氨酸)的末端氨基之间的迈克尔加成反应,报道了一种生物可还原的聚乙二醇-b-聚(二硫键-l-赖氨酸)阳离子聚合物(表示为 PEG-SSL)。PEG-SSL 有效地缩合了质粒 ZNF580 基因(pZNF580),形成了纳米级的聚轮烷(155±4 至 285±3nm),其 ζ 电位为 1.9±0.1 至 26.7±0.4mV。PEG-SSL 可以在聚合物/DNA 重量比为 10/1 及更高的情况下成功地延迟 pZNF580。当暴露于 5mM DTT 的还原环境中时,即使在 PEG-SSL/DNA 复合物中 PEG-SSL 聚合物的重量比更高,它也能迅速释放基因。PEG-SSL/pZNF580 复合物在暴露于 DNase I 时表现出良好的稳定性,并能有效地保护 pDNA 免受降解。在 EA.hy926 细胞中进行了 PEG-SSL/pZNF580 复合物的体外转染和细胞毒性研究。结果表明,与 PEI25kDa 相比,PEG-SSL 成功地将 pZNF580 递送到细胞中,细胞毒性较低。流式细胞术和共聚焦扫描激光显微镜结果表明,PEG-SSL 聚轮烷具有良好的细胞摄取率和核共定位率。所有这些结果表明,PEG-SSL 具有作为非病毒基因转染载体的潜力。

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