Yamashita Toshifumi, Sonoda Shozo, Suzuki Ryo, Arimura Noboru, Tachibana Katsuo, Maruyama Kazuo, Sakamoto Taiji
Department of Ophthalmology, Kagoshima University Graduate School of Medical and Dental Science, Sakuragaoka, Kagoshima, Kagoshima 890-8520, Japan.
Exp Eye Res. 2007 Dec;85(6):741-8. doi: 10.1016/j.exer.2007.08.006. Epub 2007 Aug 19.
Gene therapy is a promising method; however, a potential risk of viral vector or low gene transfer efficacy of non-viral vector prevents it from clinical application for common diseases. The major obstacle in the clinical application of gene therapy is not due to the lack of an ideal gene, but rather the lack of a clinically safe and efficient gene transfer method. To complete a safe and effective gene transfer, we developed a novel bubble liposome (BL) with ultrasound (US) method. BL is composed of polyethylenglycol (PEG) modified liposome (PEGylated liposome) containing perfluoropropane gas, each of which independently has been used safely in human treatment and a PEGylated liposome is quite stable in vivo. Plasmids containing green fluorescent protein (GFP) cDNA were added to cultured rabbit corneal epithelial cells (RC-1, 2x10(5)cell/well and 5microl of a plasmid solution) followed by US exposure with BL (BL-US group). Similar experiments were conducted for US exposure-only (US-only group) and US exposure and conventional micro-bubble (MB-US group). Gene transfer efficacy was evaluated by immunofluorescent microscopy and the cell damage was analyzed by MTS assay. In an in vivo study, BL and plasmid were injected into rat subconjunctiva followed by US exposure (BLUS group, 1.2W/cm(2), 20s, duty cycle 50%) and GFP expression was evaluated by imaging (maximum +5 to minimum 0) for 8 days. Rats undergoing subconjunctival plasmid injection alone (injection group), plasmid injection and US exposure (US group), MB and plasmid injection and US exposure (MBUS group) were used as controls. Histological examination was conducted. BL and US exposure significantly increased gene transfer efficacy in cultured RC-1 cells (BL-US group, 27%; US-only group, 1%; MB-US group, 11%; P<0.05: ANOVA). Gene transfer was most prominent under the condition of US intensity of 1.2W/cm(2) with 21microg/well BL, duration 20s. No apparent cell damage was found in the BL-US group by MTS assay. In rat eyes, strong GFP staining was seen in conjunctiva of BLUS group (average: 3.6). It was significantly higher than in any of the following groups, injection group (average: 2.3), US group (average: 2.1), or MBUS group (average: 2.0; P=0.001, ANOVA). GFP-positive cells were mainly in the conjunctiva and no tissue damage was seen histologically. BL with US method effectively transfers genes to cultured corneal epithelial cells and rat subconjunctival tissue without causing any apparently adverse effect. This method would have a great advantage for gene therapy in ocular surface disease.
基因治疗是一种很有前景的方法;然而,病毒载体的潜在风险或非病毒载体的低基因转移效率阻碍了其在常见疾病临床应用中的发展。基因治疗临床应用的主要障碍并非在于缺乏理想的基因,而是缺乏临床安全且高效的基因转移方法。为了实现安全有效的基因转移,我们开发了一种新型的超声介导气泡脂质体(BL)方法。BL由含有全氟丙烷气体的聚乙二醇(PEG)修饰脂质体(聚乙二醇化脂质体)组成,其中每种成分都已在人体治疗中安全使用,并且聚乙二醇化脂质体在体内相当稳定。将含有绿色荧光蛋白(GFP)cDNA的质粒添加到培养的兔角膜上皮细胞(RC-1,2×10⁵细胞/孔和5微升质粒溶液)中,随后用BL进行超声照射(BL-US组)。对仅进行超声照射(仅超声组)和超声照射及传统微泡(MB-US组)进行了类似实验。通过免疫荧光显微镜评估基因转移效率,并通过MTS测定法分析细胞损伤。在一项体内研究中,将BL和质粒注入大鼠结膜下,随后进行超声照射(BLUS组,1.2W/cm²,20秒,占空比50%),并通过成像(最大值+5至最小值0)评估8天内的GFP表达。单独进行结膜下质粒注射的大鼠(注射组)、质粒注射并超声照射的大鼠(超声组)、微泡和质粒注射并超声照射的大鼠(MBUS组)用作对照。进行了组织学检查。BL和超声照射显著提高了培养的RC-1细胞中的基因转移效率(BL-US组为27%;仅超声组为1%;MB-US组为11%;P<0.05:方差分析)。在超声强度为1.2W/cm²、每孔21微克BL、持续时间20秒的条件下,基因转移最为显著。通过MTS测定法在BL-US组中未发现明显的细胞损伤。在大鼠眼中,BLUS组的结膜中可见强烈的GFP染色(平均值:3.6)。它显著高于以下任何一组,注射组(平均值:2.3)、超声组(平均值:2.1)或MBUS组(平均值:2.0;P = 0.001,方差分析)。GFP阳性细胞主要位于结膜中,组织学检查未发现组织损伤。超声介导气泡脂质体方法能有效地将基因转移到培养的角膜上皮细胞和大鼠结膜下组织,且不会引起任何明显的不良反应。该方法在眼表疾病的基因治疗中具有很大优势。
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