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一种混合载体系统以不依赖转基因的方式扩展了腺相关病毒载体的包装能力。

A hybrid vector system expands adeno-associated viral vector packaging capacity in a transgene-independent manner.

作者信息

Ghosh Arkasubhra, Yue Yongping, Lai Yi, Duan Dongsheng

机构信息

Department of Molecular Microbiology and Immunology, The University of Missouri-Columbia, School of Medicine, Columbia, Missouri, USA.

出版信息

Mol Ther. 2008 Jan;16(1):124-30. doi: 10.1038/sj.mt.6300322. Epub 2007 Nov 6.

Abstract

The trans-splicing (ts) and overlapping (ov) vectors expand the packaging capacity of adeno-associated virus (AAV). But their application depends on the inherent properties of the target gene. The ts vectors require an optimal gene-splitting site and the ov vectors require a highly recombinogenic domain. In order to overcome these limitations, we developed a hybrid dual (hd) vector system. In the hd vectors, we inserted a highly recombinogenic alkaline phosphatase (AP) sequence in the ts vectors to allow for transgene-independent reconstitution through homologous recombination of the AP sequences. We first tested the hybrid system with the LacZ gene. Both in the cell line (in vitro) and in the mouse muscle (in vivo), the hd vectors significantly outperformed the ts and ov vectors. In muscle, the transduction efficiency of the hybrid vectors reached 80% of that from the single intact vector. Southern blot confirmed AP sequence-mediated transgene reconstitution. In order to validate the hybrid system, we split the 6 kilobase (kb) mini-dystrophin gene at the exon 55/56 junction, a predicted poor site for the ts approach. In dystrophic mdx mouse muscle, the hd vectors yielded 5.6-fold higher transduction than the ts vectors did. Taken together, these data suggest that the hybrid system efficiently expresses large therapeutic genes that are poor candidates for the ts and ov approaches.

摘要

反式剪接(ts)和重叠(ov)载体扩大了腺相关病毒(AAV)的包装容量。但其应用取决于靶基因的固有特性。ts载体需要一个最佳的基因切割位点,而ov载体需要一个高度重组的结构域。为了克服这些限制,我们开发了一种杂交双功能(hd)载体系统。在hd载体中,我们在ts载体中插入了一个高度重组的碱性磷酸酶(AP)序列,以允许通过AP序列的同源重组实现不依赖转基因的重组。我们首先用LacZ基因测试了该杂交系统。在细胞系(体外)和小鼠肌肉(体内)中,hd载体的表现均显著优于ts和ov载体。在肌肉中,杂交载体的转导效率达到了单个完整载体的80%。Southern印迹证实了AP序列介导的转基因重组。为了验证该杂交系统,我们在第55/56外显子连接处切割了6千碱基(kb)的微型肌营养不良蛋白基因,这是ts方法预测的不佳位点。在营养不良的mdx小鼠肌肉中,hd载体产生的转导比ts载体高5.6倍。综上所述,这些数据表明该杂交系统能有效表达对ts和ov方法来说不适合的大型治疗性基因。

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