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慢病毒载体基因导入恒河猴胎儿(猕猴):肺靶向方法

Lentiviral vector gene transfer into fetal rhesus monkeys (Macaca mulatta): lung-targeting approaches.

作者信息

Tarantal A F, Lee C I, Ekert J E, McDonald R, Kohn D B, Plopper C G, Case S S, Bunnell B A

机构信息

California Regional Primate Research Center, University of California, Davis, California 95616-8542, USA.

出版信息

Mol Ther. 2001 Dec;4(6):614-21. doi: 10.1006/mthe.2001.0497.

DOI:10.1006/mthe.2001.0497
PMID:11735346
Abstract

We previously reported the efficiency of gene transfer in fetal monkeys using retroviral vectors and an intraperitoneal (IP) approach. Here, we explored intrapulmonary administration to determine whether gene transfer can be limited to the developing lung. The HIV-1-derived lentiviral vector (VSV-G pseudotyped; 1 x 10(7) infectious particles/fetus), using the enhanced green fluorescent protein (EGFP) as a reporter, was directly injected into fetal lung with ultrasound guidance (n=4; 55 or 70 days gestation; term 165+/-10 days). Fetuses were monitored sonographically, fetal/maternal blood samples collected during gestation, and four of four healthy newborns were delivered at term. All lung lobes were positive for the transgene (< or = 1%) when assessed by PCR, and transgene expression was observed by direct fluorescence microscopy and flow cytometry. The results of this study show the following: (1) successful gene transfer in fetal monkeys using an intrapulmonary approach; (2) less transduction of non-pulmonary tissues with gene transfer at 70 days gestation compared with 55 days gestation or use of an IP approach; (3) that the pulmonary epithelium was EGFP-positive by immunohistochemistry; and (4) no evidence of transplacental transport of vector sequences or antibody responses in the dams. The results of these investigations indicate the efficiency of fetal gene transfer by intrapulmonary delivery, and emphasize the importance of the fetal monkey as a preclinical model system for exploring in utero genetic treatment strategies for pulmonary disorders.

摘要

我们之前报道了使用逆转录病毒载体和腹腔内(IP)给药方法在胎猴中进行基因转移的效率。在此,我们探索了肺内给药,以确定基因转移是否可以局限于发育中的肺。以增强型绿色荧光蛋白(EGFP)作为报告基因,将HIV-1衍生的慢病毒载体(VSV-G假型化;1×10⁷感染性颗粒/胎儿)在超声引导下直接注入胎肺(n = 4;妊娠55或70天;足月为165±10天)。对胎儿进行超声监测,在妊娠期采集胎儿/母体血样,4例中有4例健康新生儿足月分娩。通过PCR评估时,所有肺叶的转基因均呈阳性(≤1%),并且通过直接荧光显微镜和流式细胞术观察到转基因表达。本研究结果表明:(1)使用肺内给药方法在胎猴中成功进行了基因转移;(2)与妊娠55天或使用IP给药方法相比,妊娠70天时基因转移对非肺组织的转导较少;(3)通过免疫组织化学检测肺上皮细胞EGFP呈阳性;(4)没有证据表明载体序列经胎盘转运或母体内有抗体反应。这些研究结果表明了通过肺内给药进行胎儿基因转移的效率,并强调了胎猴作为探索肺部疾病宫内基因治疗策略的临床前模型系统的重要性。

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