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骨骼肌转导后腺相关病毒载体DNA的结构

Structure of adeno-associated virus vector DNA following transduction of the skeletal muscle.

作者信息

Vincent-Lacaze N, Snyder R O, Gluzman R, Bohl D, Lagarde C, Danos O

机构信息

Gene Therapy Program, Genethon III, CNRS URA 1922, Evry, France.

出版信息

J Virol. 1999 Mar;73(3):1949-55. doi: 10.1128/JVI.73.3.1949-1955.1999.

Abstract

The skeletal muscle provides a very permissive physiological environment for adeno-associated virus (AAV) type 2-mediated gene transfer. We have studied the early steps leading to the establishment of permanent transgene expression, after injection of recombinant AAV (rAAV) particles in the quadriceps muscle of mice. The animals received an rAAV encoding a secreted protein, murine erythropoietin (mEpo), under the control of the human cytomegalovirus major immediate-early promoter and were sacrificed between 1 and 60 days after injection. The measurement of plasma Epo levels and of hematocrits indicated a progressive increase of transgene expression over the first 2 weeks, followed by a stabilization at maximal plateau values. The rAAV sequences were analyzed by Southern blotting following neutral or alkaline gel electrophoresis of total DNA from injected muscles. While a high number of rAAV sequences were detected during the first 5 days following the injection, only a few percent of these sequences was retained in the animals analyzed after 2 weeks, in which transgene expression was maximal. Double-stranded DNA molecules resulting from de novo second-strand synthesis were detected as early as day 1, indicating that this crucial step of AAV-mediated gene transfer is readily accomplished in the muscle. The templates driving stable gene expression at later time points are low in copy number and structured as high-molecular-weight concatemers or interlocked circles. The presence of the circular form of the rAAV genomes at early time points suggests that the molecular transformations involved in the formation of stable concatemers may involve a rolling-circle type of DNA replication.

摘要

骨骼肌为2型腺相关病毒(AAV)介导的基因转移提供了一个非常宽松的生理环境。我们研究了在小鼠股四头肌中注射重组AAV(rAAV)颗粒后导致永久性转基因表达建立的早期步骤。这些动物接受了一种在人巨细胞病毒主要立即早期启动子控制下编码分泌蛋白小鼠促红细胞生成素(mEpo)的rAAV,并在注射后1至60天之间处死。血浆Epo水平和血细胞比容的测量表明,转基因表达在最初2周内逐渐增加,随后稳定在最大平台值。在对注射肌肉的总DNA进行中性或碱性凝胶电泳后,通过Southern印迹分析rAAV序列。虽然在注射后的前5天检测到大量rAAV序列,但在2周后分析的动物中,只有百分之几的这些序列被保留下来,此时转基因表达最高。早在第1天就检测到了由从头合成第二链产生的双链DNA分子,这表明AAV介导的基因转移的这一关键步骤在肌肉中很容易完成。在后期驱动稳定基因表达的模板拷贝数低,并且结构为高分子量串联体或互锁环。rAAV基因组环状形式在早期时间点的存在表明,参与稳定串联体形成的分子转化可能涉及滚环型DNA复制。

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本文引用的文献

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Adeno-associated virus vector integration junctions.腺相关病毒载体整合连接点。
J Virol. 1997 Nov;71(11):8429-36. doi: 10.1128/JVI.71.11.8429-8436.1997.

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