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A New Hybrid System Capable of Efficient Lentiviral Vector Production and Stable Gene Transfer Mediated by a Single Helper-Dependent Adenoviral Vector

机译:一个新的能够有效生产慢病毒载体和稳定的基因转移的混合系统,该系统由单个依赖于助手的腺病毒载体介导

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摘要

To achieve efficient and sustained gene expression, we developed a new lentivirus/adenovirus hybrid vector (LA vector) that encodes sequences required for production of a human immunodeficiency virus-based lentiviral vector (i.e., a lentiviral vector, a gag/pol/rev expression cassette, a tetracycline-inducible envelope cassette, and the tetracycline-inducible transcriptional activator cassette) in a single helper-dependent adenovirus vector backbone. Via either transfection or infection, human cell lines transduced with the LA vector produced a lentiviral vector in a doxycycline-dependent manner at titers up to 105 to 106 green fluorescent protein transducing units per ml, which are comparable to the titers obtained by conventional multiple plasmid transfection methods. Efficient spread and persistent expression of the transgene were observed in cells maintained in long-term culture that had been infected with the LA vector. Furthermore, when cocultured with adherent cells infected with the LA vector, the human T-cell leukemia cell line was successfully transduced with a marker gene. This LA vector possesses the advantages of efficient gene transfer from an adenoviral vector and stable integration from a lentiviral vector; therefore, it might have potential for a variety of gene therapy applications.
机译:为了实现有效和持续的基因表达,我们开发了一种新的慢病毒/腺病毒杂交载体(LA载体),该载体编码生产基于人免疫缺陷病毒的慢病毒载体(即慢病毒载体,gag / pol / rev表达)所需的序列盒,四环素诱导的包膜盒和四环素诱导的转录激活剂盒)。通过转染或感染,用LA载体转导的人细胞系以强力霉素依赖性的方式产生了慢病毒载体,其滴度高达每毫升105至106个绿色荧光蛋白转导单位,这与常规多重质粒获得的滴度相当转染方法。在长期培养的被LA载体感染的细胞中观察到转基因的有效传播和持续表达。此外,当与感染了LA载体的贴壁细胞共培养时,成功地用标记基因转导了人类T细胞白血病细胞系。该LA载体具有从腺病毒载体有效转移基因和从慢病毒载体稳定整合的优点。因此,它可能具有多种基因治疗应用的潜力。

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