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葡糖基葡糖苷基-β-环糊精/树枝状聚合物缀合物(G2)作为一种 DNA 载体在体外和体内的潜在应用。

Potential use of glucuronylglucosyl-β-cyclodextrin/dendrimer conjugate (G2) as a DNA carrier in vitro and in vivo.

机构信息

Graduate School of Pharmaceutical Sciences, Kumamoto University, Kumamoto, Japan.

出版信息

J Drug Target. 2012 Apr;20(3):272-80. doi: 10.3109/1061186X.2011.645163. Epub 2011 Dec 28.

DOI:10.3109/1061186X.2011.645163
PMID:22201459
Abstract

In this study, we evaluated the polyamidoamine starburst dendrimer (dendrimer, generation 2: G2) conjugate with 6-O-α-(4-O-α-D-glucuronyl)-D-glucosyl-β-cyclodextrin (GUG-β-CDE (G2)) as a gene transfer carrier. The in vitro gene transfer activity of GUG-β-CDE (G2, degree of substitution (DS) of cyclodextrin (CyD) 1.8) was remarkably higher than that of dendrimer (G2) conjugate with α-CyD (α-CDE (G2, DS 1.2)) and that with β-CyD(β-CDE (G2, DS 1.3)) in A549 and RAW264.7 cells. The particle size, ζ-potential, DNase I-catalyzed degradation, and cellular association of plasmid DNA (pDNA) complex with GUG-β-CDE (G2, DS 1.8) were almost the same as those of the other CDEs. Fluorescent-labeled GUG-β-CDE (G2, DS 1.8) localized in the nucleus 6 h after transfection of its pDNA complex in A549 cells, suggesting that nuclear localization of pDNA complex with GUG-β-CDE (G2, DS 1.8), at least in part, contributes to its high gene transfer activity. GUG-β-CDE (G2, DS 1.8) provided higher gene transfer activity than α-CDE (G2, DS 1.2) and β-CDE (G2, DS 1.3) in kidney with negligible changes in blood chemistry values 12 h after intravenous injection of pDNA complexes with GUG-β-CDE (G2, DS 1.8) in mice. In conclusion, the present findings suggest that GUG-β-CDE (G2, DS 1.8) has the potential for a novel polymeric pDNA carrier in vitro and in vivo.

摘要

在这项研究中,我们评估了聚酰胺胺星型树枝状大分子(树枝状大分子,第 2 代:G2)与 6-O-α-(4-O-α-D-葡糖醛酸基)-D-葡萄糖基-β-环糊精(GUG-β-CDE(G2))的缀合物作为基因转移载体。GUG-β-CDE(G2,环糊精(CyD)取代度(DS)1.8)的体外基因转移活性明显高于 G2 与α-CyD(α-CDE(G2,DS 1.2))和 G2 与β-CyD(β-CDE(G2,DS 1.3))的缀合物,在 A549 和 RAW264.7 细胞中。与其他 CDE 相比,GUG-β-CDE(G2,DS 1.8)与质粒 DNA(pDNA)复合物的粒径、ζ-电位、DNase I 催化降解和细胞相关性几乎相同。荧光标记的 GUG-β-CDE(G2,DS 1.8)在 A549 细胞转染其 pDNA 复合物 6 小时后定位于细胞核中,表明 GUG-β-CDE(G2,DS 1.8)的 pDNA 复合物的核定位至少部分有助于其高基因转移活性。与 G2 与 α-CyD(G2,DS 1.2)和 G2 与 β-CyD(G2,DS 1.3)相比,GUG-β-CDE(G2,DS 1.8)在肾组织中提供了更高的基因转移活性,并且在小鼠静脉注射 GUG-β-CDE(G2,DS 1.8)的 pDNA 复合物 12 小时后,血液化学值几乎没有变化。综上所述,本研究结果表明,GUG-β-CDE(G2,DS 1.8)在体外和体内具有新型聚合物 pDNA 载体的潜力。

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