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在小鼠中使用腺相关病毒和慢病毒载体进行子宫内肺基因转移。

In utero lung gene transfer using adeno-associated viral and lentiviral vectors in mice.

作者信息

Joyeux Luc, Danzer Enrico, Limberis Maria P, Zoltick Philip W, Radu Antoneta, Flake Alan W, Davey Marcus G

机构信息

1 Children's Center for Fetal Research, Children's Hospital of Philadelphia , Philadelphia, PA 19104.

出版信息

Hum Gene Ther Methods. 2014 Jun;25(3):197-205. doi: 10.1089/hgtb.2013.143. Epub 2014 Apr 21.

Abstract

Virus-mediated gene transfer to the fetal lung epithelium holds considerable promise for the therapeutic management of prenatally diagnosed, potentially life-threatening inherited lung diseases. In this study we hypothesized that efficient and life-long lung transduction can be achieved by in utero gene therapy, using viral vectors. To facilitate diffuse entry into the lung, viral vector was injected into the amniotic sac of C57BL/6 mice on embryonic day 16 (term, ∼ 20 days) in a volume of 10 μl. Vectors investigated included those based on adeno-associated virus (AAV) (serotypes 5, 6.2, 9, rh.64R1) and vesicular stomatitis virus G glycoprotein (VSV-G)-pseudotyped HIV-1-based lentivirus (LV). All vectors expressed green fluorescent protein (GFP) under the transcriptional control of various promoters including chicken β-actin (CB) or cytomegalovirus (CMV) for AAV and CMV or MND (myeloproliferative sarcoma virus enhancer, negative control region deleted) for LV. Pulmonary GFP gene expression was detected by fluorescence stereoscopic microscopy and immunohistochemistry for up to 9 months after birth. At equivalent vector doses (mean, 12 × 10(10) genome copies per fetus) three AAV vectors resulted in long-term (up to 9 months) pulmonary epithelium transduction. AAV2/6.2 transduced predominantly cells of the conducting airway epithelium, although transduction decreased 2 months after vector delivery. AAV2/9-transduced cells of the alveolar epithelium with a type 1 pneumocyte phenotype for up to 6 months. Although minimal levels of GFP expression were observed with AAV2/5 up to 9 months, the transduced cells immunostained positive for F480 and were retrievable by bronchoalveolar lavage, confirming an alveolar macrophage phenotype. No GFP expression was observed in lung epithelial cells after AAV2/rh.64R1 and VSV-G-LV vector-mediated gene transfer. We conclude that these experiments demonstrate that prenatal lung gene transfer with AAV vectors engineered to target pulmonary epithelial cells may provide sustained long-term levels of transgene expression, supporting the therapeutic potential of prenatal gene transfer for the treatment of congenital lung diseases.

摘要

病毒介导的基因转移至胎儿肺上皮细胞,对于产前诊断的、可能危及生命的遗传性肺部疾病的治疗管理具有巨大潜力。在本研究中,我们假设通过子宫内基因治疗,使用病毒载体可以实现高效且终身的肺部转导。为促进病毒载体扩散进入肺部,于胚胎第16天(足月约20天)将10 μl病毒载体注射到C57BL/6小鼠的羊膜囊中。所研究的载体包括基于腺相关病毒(AAV)的载体(血清型5、6.2、9、rh.64R1)以及水泡性口炎病毒G糖蛋白(VSV-G)假型化的基于HIV-1的慢病毒(LV)。所有载体在包括鸡β-肌动蛋白(CB)或巨细胞病毒(CMV)(用于AAV)以及CMV或MND(骨髓增殖性肉瘤病毒增强子,缺失负调控区)(用于LV)等各种启动子的转录控制下表达绿色荧光蛋白(GFP)。通过荧光立体显微镜和免疫组织化学检测出生后长达9个月的肺部GFP基因表达。在等效载体剂量下(平均每胎儿12×10¹⁰个基因组拷贝),三种AAV载体导致长期(长达9个月)的肺上皮细胞转导。AAV2/6.2主要转导传导气道上皮细胞,尽管在载体递送2个月后转导减少。AAV2/9转导具有I型肺细胞表型的肺泡上皮细胞长达6个月。尽管AAV2/5在长达9个月时观察到最低水平的GFP表达,但转导细胞对F480免疫染色呈阳性,并且可通过支气管肺泡灌洗回收,证实为肺泡巨噬细胞表型。在AAV2/rh.64R1和VSV-G-LV载体介导的基因转移后,未在肺上皮细胞中观察到GFP表达。我们得出结论,这些实验表明,用经工程改造以靶向肺上皮细胞的AAV载体进行产前肺基因转移可提供持续的长期转基因表达水平,支持产前基因转移治疗先天性肺部疾病的治疗潜力。

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