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在使用未修饰和甘露糖修饰的泡囊脂质体,并结合超声处理的情况下,激活的转录过程参与了高效的基因转染。

Involvement of activated transcriptional process in efficient gene transfection using unmodified and mannose-modified bubble lipoplexes with ultrasound exposure.

机构信息

Department of Drug Delivery Research, Graduate School of Pharmaceutical Sciences, Kyoto University, 46-29 Yoshida-Shimoadachi-cho, Sakyo-ku, Kyoto 606-8501, Japan.

出版信息

J Control Release. 2011 Dec 20;156(3):355-63. doi: 10.1016/j.jconrel.2011.06.040. Epub 2011 Jul 3.

DOI:10.1016/j.jconrel.2011.06.040
PMID:21756951
Abstract

Recently, our group developed ultrasound (US)-responsive and mannose-modified gene carriers (Man-PEG(2000) bubble lipoplexes), and successfully obtained a high level of gene expression in mannose receptor-expressing cells following gene transfection using Man-PEG(2000) bubble lipoplexes and US exposure. We also reported that large amounts of plasmid DNA (pDNA) were transferred into the cytoplasm of the targeted cells in the gene transfection using this method. In the present study, we investigated the involvement of transcriptional processes on enhanced gene expression obtained by unmodified and Man-PEG(2000) bubble lipoplexes with US exposure. The transcriptional process related to activator protein-1 (AP-1) and nuclear factor-κB (NFκB) was activated by US exposure, and was founded to be involved in enhanced gene expression obtained by gene transfection using unmodified and Man-PEG(2000) bubble lipoplexes with US exposure. On the other hand, activation of AP-1 and NFκB pathways followed by US exposure was hardly involved in the inflammatory responses in the gene transfection using this method. These findings suggest that activation of AP-1 and NFκB followed by US exposure is involved in the enhanced gene expression using unmodified and Man-PEG(2000) bubble lipoplexes with US exposure, and the selection of pDNAs activated by US exposure is important in this gene transfection method.

摘要

最近,我们小组开发了超声(US)响应和甘露糖修饰的基因载体(Man-PEG(2000)泡脂质体),并成功地在用 Man-PEG(2000)泡脂质体和 US 暴露转染后,在甘露糖受体表达细胞中获得了高水平的基因表达。我们还报道了大量质粒 DNA(pDNA)通过这种方法转染到靶向细胞的细胞质中。在本研究中,我们研究了转录过程在未修饰和 Man-PEG(2000)泡脂质体与 US 暴露增强基因表达中的作用。与激活蛋白-1(AP-1)和核因子-κB(NFκB)相关的转录过程被 US 暴露激活,并被发现参与了未修饰和 Man-PEG(2000)泡脂质体与 US 暴露增强基因表达的基因转染。另一方面,US 暴露后 AP-1 和 NFκB 途径的激活在该方法的基因转染中很少涉及炎症反应。这些发现表明,US 暴露后 AP-1 和 NFκB 的激活参与了未修饰和 Man-PEG(2000)泡脂质体与 US 暴露增强基因表达,并且 US 暴露激活的 pDNA 的选择在这种基因转染方法中很重要。

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