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education, concentration and efficient transfer of vsv g pseudotypisierten retroviral vectors

机译:vsv g伪型反转录病毒载体的教育,集中和有效转移

摘要

The present application discloses retrovirus-derived vectors in which the retroviral envelope glycoprotein has been replaced by the G glycoprotein of vesicular stomatitis virus, and the use of these vectors in the transfer of exogenous genes into the cells of a wide variety of non-mammalian organisms. Also disclosed is a method for the generation of retroviral vectors in high titers, wherein a recombinant, stable host cell line is provided which harbors the retroviral vector of interest without envelope protein. High-titer retroviral vector production is initiated by introducing nucleic acid encoding a functional membrane-associated protein into the cell line. The vectors disclosed in the present application can be concentrated by ultracentrifugation to titers greater than 109 cfu/ml which are especially useful in human gene therapy trials, and can also infect cells, such as hamster and fish cells, that are ordinarily resistant to infection with vectors containing the retroviral envelope protein.
机译:本申请公开了其中逆转录病毒包膜糖蛋白已被水泡性口炎病毒的G糖蛋白替代的逆转录病毒来源的载体,以及这些载体在将外源基因转移到多种非哺乳动物生物的细胞中的用途。 。还公开了一种以高滴度产生逆转录病毒载体的方法,其中提供了重组的稳定宿主细胞系,其携带感兴趣的逆转录病毒载体而没有包膜蛋白。通过将编码功能性膜相关蛋白的核酸引入细胞系来启动高滴度逆转录病毒载体的生产。可将本申请中公开的载体通过超速离心浓缩至大于109 cfu / ml的滴度,这在人类基因疗法试验中特别有用,并且还可以感染通常抵抗感染的细胞,例如仓鼠和鱼细胞。含有逆转录病毒包膜蛋白的载体。

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