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首页> 外文期刊>Molecular therapy: the journal of the American Society of Gene Therapy >Helper-independent and AAV-ITR-independent chromosomal integration of double-stranded linear DNA vectors in mice.
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Helper-independent and AAV-ITR-independent chromosomal integration of double-stranded linear DNA vectors in mice.

机译:小鼠中双链线性DNA载体的不依赖辅助分子和不依赖AAV-ITR的染色体整合。

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摘要

Nonviral plasmid DNA is a promising vector for achieving ex vivo and in vivo gene transfer. However, transgene expression is usually transient, especially in dividing target cells due to loss of vector genomes. Here we describe the use of naked double-stranded (ds) linear DNA as a way to insert exogenous DNA sequences into chromosomes of mouse hepatocytes in vivo, without helper components such as integrase or transposase. We constructed ds linear DNA vectors with or without adeno-associated virus inverted terminal repeats (AAV-ITRs), introduced them into mouse hepatocytes in vivo using a hydrodynamics-based transfection technique, and analyzed for vector genome integration in various ways. Surprisingly, these linear DNA molecules integrated in mouse hepatocytes in vivo at a level of 0.3-0.5 vector genome, or more, per diploid genomic equivalent irrespective of the AAV-ITR sequences. Our results establish a novel and simple way to engineer chromosomes in vivo and provide further insights into the mechanisms of recombinant AAV vector integration in vivo. In addition, they may provide a clue for developing new nonviral integrating gene delivery vector systems.
机译:非病毒质粒DNA是用于实现离体和体内基因转移的有前途的载体。但是,转基因表达通常是瞬时的,特别是在分裂靶细胞时,由于载体基因组的丢失。在这里,我们描述了使用裸双链(ds)线性DNA作为将外源DNA序列插入体内小鼠肝细胞染色体的方法,而没有诸如整合酶或转座酶的辅助成分。我们构建了带有或不带有腺相关病毒反向末端重复序列(AAV-ITR)的ds线性DNA载体,并使用基于流体动力学的转染技术将它们引入小鼠体内的小鼠肝细胞中,并以各种方式分析了载体基因组整合。令人惊讶地,这些线性DNA分子在体内以每二倍体基因组当量0.3-0.5个载体基因组水平或更高的水平整合到小鼠肝细胞中,而与AAV-ITR序列无关。我们的结果建立了一种在体内工程改造染色体的新颖且简单的方法,并提供了对体内重组AAV载体整合机制的进一步见解。此外,它们可能为开发新的非病毒整合基因递送载体系统提供线索。

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