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Integrase-defective Lentiviral Vectors as a Delivery Platform for Targeted Modification of Adenosine Deaminase Locus

机译:整合酶缺陷型慢病毒载体作为靶向修饰腺苷脱氨酶基因座的传递平台。

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摘要

We investigated the use of integrase-defective lentiviral vectors (IDLVs) for transient delivery of zinc finger nucleases (ZFNs) and donor templates for site-specific modification of the human adenosine deaminase (hADA) gene. Initially, we constructed IDLVs carrying ZFN monomers (Single-IDLVs) and found them to be able to deliver their gene-editing payload to K562 cells successfully upon cotransduction, with minimal cytotoxicity. To simplify delivery, we designed an IDLV construct to deliver both ZFN monomers from the same vector (Double-IDLV). However, this construct in its original state was prone to rearrangements of the vector genome, resulting in greatly reduced functionality; this was due to recombination between highly similar ZFN monomers arranged in tandem. We modified the Double-IDLV constructs to reduce recombination and restored simultaneous delivery of both ZFNs. We also tested an IDLV construct for delivery of donor templates and demonstrated its efficacy for gene modification. In summary, we highlighted the importance of modifying vector design for co-delivery of highly similar sequences inherent to genome-editing nucleases, and demonstrated significant improvement in the use of IDLVs for delivery of ZFNs and donor templates for genome modification.
机译:我们调查了整合酶缺陷型慢病毒载体(IDLV)用于瞬时递送锌指核酸酶(ZFNs)和供体模板的人腺苷脱氨酶(hADA)基因的位点特异性修饰的用途。最初,我们构建了携带ZFN单体的IDLV(Single-IDLV),发现它们能够通过共转导成功地将其基因编辑有效载荷传递给K562细胞,且细胞毒性最小。为了简化传递,我们设计了IDLV构造,以从同一载体(Double-IDLV)传递两种ZFN单体。然而,这种构建体在其原始状态下易于对载体基因组进行重排,从而导致功能大大降低。这是由于串联排列的高度相似的ZFN单体之间发生重组。我们修改了Double-IDLV结构,以减少重组并恢复了两个ZFN的同时传递。我们还测试了IDLV构建体用于递送供体模板,并证明了其对基因修饰的功效。总之,我们强调了修饰载体设计对于共同传递基因组编辑核酸酶固有的高度相似序列的重要性,并证明了IDLV用于ZFN传递和供体模板用于基因组修饰的显着改善。

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