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体外非病毒介导的小鼠原神经营养因子3基因转入大鼠骨髓基质细胞

In vitro non-viral murine pro-neurotrophin 3 gene transfer into rat bone marrow stromal cells.

作者信息

Darabi Shahram, Tiraihi Taki, Delshad AliReza, Sadeghizadeh Majid, Khalil Wisam, Taheri Taher

机构信息

Cellular and Molecular Research Center, Qazvin University of Medical Science, Qazvin, Iran.

Department of Anatomical Sciences, School of Medical Sciences, Tarbiat Modares University, Tehran, Iran.

出版信息

J Neurol Sci. 2017 Apr 15;375:137-145. doi: 10.1016/j.jns.2017.01.058. Epub 2017 Jan 21.

DOI:10.1016/j.jns.2017.01.058
PMID:28320116
Abstract

Neurotrophin 3 (NT-3) is an important factor for promoting prenatal neural development, as well as regeneration, axogenesis and plasticity in postnatal life. Therapy with NT-3 was reported to improve the condition of patients suffering from degenerative diseases and traumatic injuries, however, the disadvantage of NT-3 protein delivery is its short half-life, thus our alternative approach is the use of NT-3 gene therapy. In this study, the bone marrow stromal cells (BMSCs) were isolated from adult rats, cultured for 4 passages and transfected with either pEGFP-N1 or a constructed vector containing murine proNT-3 (pSecTag2/HygroB-murine proNT-3) using Lipofectamine 2000 followed by Hygromycin B (200mg/kg). The transfection efficiency of the transiently transfected BMSCs was evaluated using the green fluorescence protein containing vector (pEGFP-N1). A quantitative evaluation of the NT-3 expression of mRNA using real time qRT-PCR shows that there was double fold increase in NT-3 gene expression compared with non-transfected BMSCs, also, the culture supernatant yielded double fold increase in NT-3 using ELISA technique, the data were supported by immunoblotting technique. This suggests that the use of this transfection technique can be useful for gene therapy in different neurological disorders with neurodegenerative or traumatic origins.

摘要

神经营养因子3(NT-3)是促进产前神经发育以及出生后生活中的再生、轴突形成和可塑性的重要因素。据报道,用NT-3进行治疗可改善患有退行性疾病和创伤性损伤患者的病情,然而,NT-3蛋白递送的缺点是其半衰期短,因此我们的替代方法是使用NT-3基因疗法。在本研究中,从成年大鼠中分离出骨髓基质细胞(BMSC),培养4代,并用Lipofectamine 2000将其转染pEGFP-N1或含有小鼠proNT-3的构建载体(pSecTag2/HygroB-小鼠proNT-3),随后用潮霉素B(200mg/kg)处理。使用含有绿色荧光蛋白的载体(pEGFP-N1)评估瞬时转染的BMSC的转染效率。使用实时qRT-PCR对NT-3 mRNA表达进行定量评估表明,与未转染的BMSC相比,NT-3基因表达增加了两倍,同样,使用ELISA技术,培养上清液中NT-3增加了两倍,数据得到免疫印迹技术的支持。这表明这种转染技术可用于治疗不同起源的神经退行性或创伤性神经系统疾病的基因治疗。

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