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首页> 外文期刊>Gene therapy >Efficient gene transfer into the CNS by lentiviral vectors purified by anion exchange chromatography.
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Efficient gene transfer into the CNS by lentiviral vectors purified by anion exchange chromatography.

机译:通过阴离子交换层析纯化的慢病毒载体将基因有效转移到CNS中。

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摘要

Lentiviral vectors have been shown to stably transduce dividing and non-dividing target cells in vitro and in vivo. However, in vivo gene transfer applications with viral vectors in the central nervous system require highly efficient vector preparations, because only very small volumes can be injected stereotactically without damage to the brain tissue. Since lentiviral vectors are generated in transient co-transfection systems, viral preparations need to be purified and efficiently concentrated before injection into the brain. We describe an alternative procedure to concentrate lentiviral preparations by binding viral particles to an anion exchange column. Viral particles are eluted with sodium chloride, desalted and further concentrated by ultrafiltration. These vector preparations allowed high levels of gene transfer into terminally differentiated neuronal and glial cells and long-term transgene expression without any signs of acute and long-term toxicity or inflammation. The purification of lentiviral vectors from large-scale preparations by anion exchange chromatography allowed us to concentrate the virus to small volumes and to use these preparations to genetically modified target cells in vivo without signs of acute inflammatory responses.
机译:慢病毒载体已显示出在体内和体外稳定转导分裂和非分裂靶细胞的能力。但是,在中枢神经系统中使用病毒载体进行的体内基因转移应用需要高效的载体制备方法,因为在立体定向上只能注射很小的量而不会损坏脑组织。由于慢病毒载体是在瞬时共转染系统中产生的,因此在注射入大脑之前,需要纯化和有效浓缩病毒制剂。我们描述了通过将病毒颗粒结合到阴离子交换柱上来浓缩慢病毒制剂的替代方法。病毒颗粒用氯化钠洗脱,脱盐并通过超滤进一步浓缩。这些载体制备物允许高水平的基因转移到终末分化的神经元和神经胶质细胞中,并且可以长期转基因表达,而没有任何急性和长期毒性或炎症的迹象。通过阴离子交换色谱从大规模制剂中纯化慢病毒载体,使我们可以将病毒浓缩至小体积,并利用这些制剂在体内进行基因修饰的靶细胞,而没有急性炎症反应的迹象。

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