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壳聚糖/透明质酸纳米粒的体内外基因传递:透明质酸分子量和冻干对转染效率的影响。

In vitro and in vivo gene delivery using chitosan/hyaluronic acid nanoparticles: Influences of molecular mass of hyaluronic acid and lyophilization on transfection efficiency.

机构信息

Department of Biosciences and Informatics, Keio University, Yokohama, Kanagawa, Japan.

Research Support Center, Dokkyo Medical University, Shimotsuga, Tochigi, Japan.

出版信息

J Gene Med. 2017 Aug;19(8). doi: 10.1002/jgm.2968.

DOI:10.1002/jgm.2968
PMID:28667693
Abstract

BACKGROUND

Lyophilization is an effective method for preserving nonviral gene vectors. To improve the stability and transgene expression of lyophilized plasmid DNA (pDNA) complexes, we coated the surfaces of pDNA/chitosan complexes with hyaluronic acid (HA) of varying molecular masses. The transgene expression of pDNA/chitosan/HA ternary complexes was characterized in vitro and in vivo.

METHODS

pDNA complexes were lyophilized overnight and the resultant products with spongy, porous consistencies were stored at -30, 4 or 25°C for 2 weeks. Rehydrated complexes were characterized using gel retardation assays, aiming to confirm complex formation, measure particle size and evaluate zeta potential, as well as conduct luciferase gene reporter assays. The anti-tumor effects of pDNA ternary complexes were evaluated using suicide gene (pTK) coding thymidine kinase in Huh7-implanted mice.

RESULTS

Transfection efficiencies of pDNA/chitosan/HA ternary complexes were dependent on the average molecular masses of HA. The coating of pDNA/chitosan complexes with HA maintained the cellular transfection efficiencies of lyophilized pDNA ternary complexes. Furthermore, intratumoral injection of lyophilized, rehydrated pDNA ternary complexes into tumor-bearing mice showed a significant suppression of tumor growth.

CONCLUSIONS

The coating of pDNA/chitosan complexes with high-molecular-weight HA augmented the stability and cellular transfection ability of the complexes after lyophilization-rehydration.

摘要

背景

冷冻干燥是保存非病毒基因载体的有效方法。为了提高冷冻干燥质粒 DNA(pDNA)复合物的稳定性和转基因表达,我们用不同分子量的透明质酸(HA)对 pDNA/壳聚糖复合物进行表面涂层。在体外和体内对 pDNA/壳聚糖/HA 三元复合物的转基因表达进行了表征。

方法

pDNA 复合物经过夜冷冻干燥,所得具有海绵状、多孔结构的产物在-30、4 或 25°C 下储存 2 周。通过凝胶阻滞实验对复溶复合物进行表征,以确认复合物的形成、测量粒径和评估zeta 电位,并进行荧光素酶基因报告基因实验。通过自杀基因(pTK)编码胸苷激酶在 Huh7 植入小鼠中评估 pDNA 三元复合物的抗肿瘤作用。

结果

pDNA/壳聚糖/HA 三元复合物的转染效率取决于 HA 的平均分子量。用 HA 对 pDNA/壳聚糖复合物进行涂层可保持冷冻干燥 pDNA 三元复合物的细胞转染效率。此外,向荷瘤小鼠瘤内注射冷冻干燥、复溶的 pDNA 三元复合物可显著抑制肿瘤生长。

结论

用高分子量的 HA 对 pDNA/壳聚糖复合物进行涂层可提高复合物在冷冻干燥-复水后的稳定性和细胞转染能力。

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