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Efficient Transgene Reconstitution with Hybrid Dual AAV Vectors Carrying the Minimized Bridging Sequences

机译:带有最小化桥接序列的混合双AAV载体的高效转基因重组

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摘要

A hybrid dual-vector system was developed recently as a universal platform to double the packaging capacity of recombinant adeno-associated virus (AAV). In this system, the expression cassette is split into two independent AAV vectors. A highly recombinogenic bridging DNA sequence is engineered in both vectors to mediate target gene-independent homologous recombination between the split vector genomes. In the prototype hybrid vectors, a 0.87-kb DNA fragment from the middle portion of the human placental alkaline phosphatase (AP) gene was used as the bridging sequence. Here we report the development of the minimized bridging sequences. Five independent bridging sequences (0.26 to 0.44 kb) were evaluated in MO59K cells and/or murine skeletal muscle in the context of the AP overlapping vectors and/or the β-galactosidase (LacZ) hybrid vectors. Robust reconstitution comparable to that of the original hybrid vectors was achieved from a 0.26-kb and a 0.27-kb bridging sequence. These newly developed bridging sequences greatly expand the utility of the hybrid dual AAV vector system for delivering larger therapeutic genes/expression cassettes.
机译:最近开发了一种混合双载体系统,作为通用平台,可将重组腺相关病毒(AAV)的包装能力提高一倍。在该系统中,表达盒被分成两个独立的AAV载体。在两个载体中都设计了高度重组的桥接DNA序列,以介导分裂的载体基因组之间不依赖靶基因的同源重组。在原型杂交载体中,来自人胎盘碱性磷酸酶(AP)基因中间部分的0.87-kb DNA片段被用作桥接序列。在这里,我们报告了最小化桥接序列的发展。在AP重叠载体和/或β-半乳糖苷酶(LacZ)杂交载体的背景下,在MO59K细胞和/或鼠骨骼肌中评估了五个独立的桥接序列(0.26-0.44kb)。从0.26kb和0.27kb的桥接序列获得了与原始杂种载体相当的稳健重组。这些新开发的桥接序列极大地扩展了杂交双重AAV载体系统用于递送更大的治疗基因/表达盒的用途。

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