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基于电穿孔的基因转移用于神经前体细胞的高效转染。

Electroporation-based gene transfer for efficient transfection of neural precursor cells.

作者信息

Richard Ines, Ader Marius, Sytnyk Vladimir, Dityatev Alexander, Richard Gisbert, Schachner Melitta, Bartsch Udo

机构信息

Kopf-und Hautzentrum, Klinik und Poliklinik für Augenheilkunde, Universitätsklinikum Hamburg-Eppendorf, Martinistr. 52, D-20246 Hamburg, Germany.

出版信息

Brain Res Mol Brain Res. 2005 Aug 18;138(2):182-90. doi: 10.1016/j.molbrainres.2005.04.010.

Abstract

Transplantation of neural precursor cells (NPCs) is a potential tool to replace dysfunctional or degenerated neuronal or glial cell types in the central nervous system. Furthermore, transplantation of genetically engineered neural precursor cells might provide a strategy to target therapeutic gene products to the diseased nervous system. Here, we describe a novel and highly efficient electroporation-based transfection protocol for mitogen-expanded mouse NPCs. Transfection of NPCs with the reporter gene enhanced green fluorescent protein (EGFP) or the neural adhesion molecule L1 revealed transfection efficacies of more than 70% as estimated by the number of EGFP-positive or L1-immunoreactive cells 1 day after transfection in vitro. The percentage of EGFP- or L1-positive cells decreased with increasing time in culture. Positive cells were detectable for up to 3 weeks after transfection. When EGFP- or L1-transfected NPCs were grafted into the retina of adult wild-type or L1-deficient mice, they differentiated into glial cells some of which expressed EGFP and L1 for up to 2 and 3 weeks, respectively, the longest post-transplantation periods investigated.

摘要

神经前体细胞(NPCs)移植是一种潜在的工具,可用于替代中枢神经系统中功能失调或退化的神经元或神经胶质细胞类型。此外,基因工程神经前体细胞的移植可能提供一种将治疗性基因产物靶向患病神经系统的策略。在此,我们描述了一种针对有丝分裂原扩增的小鼠神经前体细胞的基于电穿孔的新型高效转染方案。用报告基因增强型绿色荧光蛋白(EGFP)或神经粘附分子L1转染神经前体细胞,体外转染1天后,根据EGFP阳性或L1免疫反应性细胞的数量估计,转染效率超过70%。随着培养时间的增加,EGFP或L1阳性细胞的百分比下降。转染后长达3周均可检测到阳性细胞。当将EGFP或L1转染的神经前体细胞移植到成年野生型或L1缺陷型小鼠的视网膜中时,它们分化为神经胶质细胞,其中一些分别在长达2周和3周的时间内表达EGFP和L1,这是所研究的最长移植后时期。

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