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本文引用的文献

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Overcoming adeno-associated virus vector size limitation through viral DNA heterodimerization.通过病毒DNA异源二聚化克服腺相关病毒载体大小限制
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A new dual-vector approach to enhance recombinant adeno-associated virus-mediated gene expression through intermolecular cis activation.一种通过分子间顺式激活增强重组腺相关病毒介导的基因表达的新型双载体方法。
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Increasing the size of rAAV-mediated expression cassettes in vivo by intermolecular joining of two complementary vectors.通过两个互补载体的分子间连接在体内增加rAAV介导的表达盒的大小。
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Evidence for gene transfer and expression of factor IX in haemophilia B patients treated with an AAV vector.使用腺相关病毒(AAV)载体治疗的B型血友病患者中因子IX基因转移和表达的证据。
Nat Genet. 2000 Mar;24(3):257-61. doi: 10.1038/73464.
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Concatamerization of adeno-associated virus circular genomes occurs through intermolecular recombination.腺相关病毒环状基因组的串联化通过分子间重组发生。
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Structural analysis of adeno-associated virus transduction circular intermediates.腺相关病毒转导环状中间体的结构分析
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Titration of AAV-2 particles via a novel capsid ELISA: packaging of genomes can limit production of recombinant AAV-2.通过新型衣壳酶联免疫吸附测定法滴定腺相关病毒2型颗粒:基因组包装可能会限制重组腺相关病毒2型的产生。
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High-titer recombinant adeno-associated virus production utilizing a recombinant herpes simplex virus type I vector expressing AAV-2 Rep and Cap.利用表达AAV-2 Rep和Cap的重组I型单纯疱疹病毒载体进行高滴度重组腺相关病毒的生产。
Gene Ther. 1999 Jun;6(6):986-93. doi: 10.1038/sj.gt.3300937.
9
Highly purified recombinant adeno-associated virus vectors are biologically active and free of detectable helper and wild-type viruses.高度纯化的重组腺相关病毒载体具有生物活性,且不含可检测到的辅助病毒和野生型病毒。
Hum Gene Ther. 1999 Apr 10;10(6):1031-9. doi: 10.1089/10430349950018427.
10
Gene therapy vectors based on adeno-associated virus type 1.基于1型腺相关病毒的基因治疗载体。
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使用含内含子的辅助质粒生产高滴度、无野生型的重组腺相关病毒载体

High-titer, wild-type free recombinant adeno-associated virus vector production using intron-containing helper plasmids.

作者信息

Cao L, Liu Y, During M J, Xiao W

机构信息

CNS Gene Therapy Center, Department of Neurosurgery, Thomas Jefferson University, Philadelphia, Pennsylvania 19107, USA.

出版信息

J Virol. 2000 Dec;74(24):11456-63. doi: 10.1128/jvi.74.24.11456-11463.2000.

DOI:10.1128/jvi.74.24.11456-11463.2000
PMID:11090141
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC112424/
Abstract

Recombinant adeno-associated virus (rAAV) is capable of directing long-term, high-level transgene expression without destructive cell-mediated immune responses. However, traditional packaging methods for rAAV vectors are generally inefficient and contaminated with replication-competent AAV (rcAAV) particles. Although wild-type AAV is not associated with any known human diseases, contaminating rcAAV particles may affect rAAV gene expression and are an uncontrolled variable in many AAV gene transfer studies. In the current study, a novel strategy was designed to both optimize AAV rep gene expression and increase vector yield, as well as simultaneously to diminish the potential of generating rcAAV particles from the helper plasmid. The strategy is based on the insertion of an additional intron in the AAV genome. In the AAV infectious clone, the intron insertion had no effects on the properties of Rep proteins expressed. Normal levels of both Rep and Cap proteins were expressed, and the replication of the AAV genome was not impaired. However, the generation of infectious rcAAV particles using intronized AAV helper was greatly diminished, which was due to the oversized AAV genome caused by the insertion of the artificial introns. Moreover, the rAAV packaging was significantly improved with the appropriate choice of intron and insertion position. The intron is another element that can regulate the rep and cap gene expression from the helper plasmid. This study provides for a novel AAV packaging system which is highly versatile and efficient. It can not only be combined with other AAV packaging systems, including rep-containing cell lines and herpes simplex virus hybrid packaging methods, but also be used in other vector systems as well.

摘要

重组腺相关病毒(rAAV)能够实现长期、高水平的转基因表达,且不会引发具有破坏性的细胞介导免疫反应。然而,传统的rAAV载体包装方法通常效率低下,且会被具有复制能力的AAV(rcAAV)颗粒污染。尽管野生型AAV与任何已知人类疾病均无关联,但污染的rcAAV颗粒可能会影响rAAV基因表达,并且在许多AAV基因转移研究中是一个无法控制的变量。在本研究中,设计了一种新策略,既能优化AAV rep基因表达并提高载体产量,同时又能降低从辅助质粒产生rcAAV颗粒的可能性。该策略基于在AAV基因组中插入一个额外的内含子。在AAV感染性克隆中,内含子插入对所表达的Rep蛋白的特性没有影响。Rep和Cap蛋白均正常表达,且AAV基因组的复制未受损害。然而,使用内含子化的AAV辅助质粒产生感染性rcAAV颗粒的情况大大减少,这是由于人工内含子插入导致AAV基因组过大所致。此外,通过适当选择内含子和插入位置,rAAV包装得到了显著改善。内含子是另一种可调节辅助质粒中rep和cap基因表达的元件。本研究提供了一种高度通用且高效的新型AAV包装系统。它不仅可以与其他AAV包装系统相结合,包括含rep的细胞系和单纯疱疹病毒杂交包装方法,还可用于其他载体系统。