携带 Cre-loxP 的慢病毒载体介导的位点特异性基因插入。
Site-specific gene insertion mediated by a Cre-loxP-carrying lentiviral vector.
机构信息
Department of Virology, Beckman Research Institute, City of Hope National Medical Center, Duarte, California, USA.
出版信息
Mol Ther. 2010 Oct;18(10):1814-21. doi: 10.1038/mt.2010.150. Epub 2010 Jul 13.
Abstract
Retroviral vectors have been used to treat patients with the X-linked severe combined immunodeficiency disease and chronic granulomatous disease. In both cases, success has been undermined by clonal expansion of transduced cells in some patients due to insertional mutagenesis induced by random vector integration. This outcome underscores the importance of designing vectors for site-specific gene insertion to avoid unanticipated gene disruption or gene activation. In the present study, we incorporated the sequence-specific Cre protein into lentiviral virions. We demonstrated that the virion-associated Cre protein remained enzymatically active and was capable of directing site-specific insertion of a gene in the vector into a defined loxP site in the host genome. As there are loxP-like sequences throughout human genome that can be recognized by either wild-type Cre or Cre variants, our study demonstrates a new strategy of designing lentiviral-based vector for gene targeting.
摘要
逆转录病毒载体已被用于治疗 X 连锁严重联合免疫缺陷病和慢性肉芽肿病患者。在这两种情况下,由于随机载体整合诱导的插入突变,一些患者中转导细胞的克隆扩增破坏了治疗的成功。这一结果突出表明设计用于特定部位基因插入的载体的重要性,以避免意外的基因破坏或基因激活。在本研究中,我们将序列特异性 Cre 蛋白掺入慢病毒病毒粒子中。我们证明,病毒粒子相关的 Cre 蛋白仍然具有酶活性,并能够指导载体中特定基因插入到宿主基因组中的一个特定 loxP 位点。由于人类基因组中存在着可以被野生型 Cre 或 Cre 变体识别的 loxP 样序列,我们的研究展示了一种设计基于慢病毒的基因靶向载体的新策略。
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