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Marker Rescue of Adeno-Associated Virus (AAV) Capsid Mutants: a Novel Approach for Chimeric AAV Production

机译:腺相关病毒(AAV)衣壳突变体的标记抢救:嵌合AAV生产的一种新方法。

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摘要

Marker rescue, the restoration of gene function by replacement of a defective gene with a normal one by recombination, has been utilized to produce novel adeno-associated virus (AAV) vectors. AAV serotype 2 (AAV2) clones containing wild-type terminal repeats, an intact rep gene, and a mutated cap gene, served as the template for marker rescue. When transfected alone in 293 cells, these AAV2 mutant plasmids produced noninfectious AAV virions that could not bind heparin sulfate after infection with adenovirus dl309 helper virus. However, the mutation in the cap gene was corrected after cotransfection with AAV serotype 3 (AAV3) capsid DNA fragments, resulting in the production of AAV2/AAV3 chimeric viruses. The cap genes from several independent marker rescue experiments were PCR amplified, cloned, and then sequenced. Sequencing results confirmed not only that homologous recombination occurred but, more importantly, that a mixed population of AAV chimeras carrying 16 to 2,200 bp throughout different regions of the type 3 cap gene were generated in a single marker rescue experiment. A 100% correlation was observed between infectivity and the ability of the chimeric virus to bind heparin sulfate. In addition, many of the AAV2/AAV3 chimeras examined exhibited differences at both the nucleotide and amino acid levels, suggesting that these chimeras may also exhibit unique infectious properties. Furthermore, AAV helper plasmids containing these chimeric cap genes were able to function in the triple transfection method to generate recombinant AAV. Together, the results suggest that DNA from other AAV serotypes can rescue AAV capsid mutants and that marker rescue may be a powerful, yet simple, technique to map, as well as develop, chimeric AAV capsids that display different serotype-specific properties.
机译:标记抢救,即通过重组将缺陷基因替换为正常基因来恢复基因功能,已被用于生产新型腺相关病毒(AAV)载体。包含野生型末端重复序列,完整的rep基因和突变的cap基因的AAV血清型2(AAV2)克隆用作标记物拯救的模板。当在293细胞中单独转染时,这些AAV2突变体质粒产生的非感染性AAV病毒体在感染腺病毒dl309辅助病毒后不能结合硫酸肝素。但是,在与AAV血清型3(AAV3)衣壳DNA片段共转染后,纠正了cap基因中的突变,从而产生了AAV2 / AAV3嵌合病毒。 PCR扩增,克隆并测序来自几个独立的标记物拯救实验的帽基因。测序结果不仅证实发生了同源重组,而且更重要的是,在单个标记拯救实验中产生了在3型cap基因的不同区域携带16到2,200 bp的AAV嵌合体的混合群体。在感染性和嵌合病毒结合硫酸肝素的能力之间观察到100%的相关性。此外,检查的许多AAV2 / AAV3嵌合体在核苷酸和氨基酸水平上均表现出差异,这表明这些嵌合体也可能具有独特的传染性。此外,包含这些嵌合帽基因的AAV辅助质粒能够在三重转染方法中发挥作用,以产生重组AAV。总之,结果表明来自其他AAV血清型的DNA可以拯救AAV衣壳突变体,而标志物拯救可能是一种强大而简单的技术,可定位和开发显示不同血清型特异性的嵌合AAV衣壳。

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