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一种新的165个碱基对的末端重复序列是腺相关病毒生命周期唯一的顺式作用元件需求。

A novel 165-base-pair terminal repeat sequence is the sole cis requirement for the adeno-associated virus life cycle.

作者信息

Xiao X, Xiao W, Li J, Samulski R J

机构信息

Gene Therapy Center and Department of Pharmacology, University of North Carolina at Chapel Hill, 27599, USA.

出版信息

J Virol. 1997 Feb;71(2):941-8. doi: 10.1128/JVI.71.2.941-948.1997.

Abstract

Adeno-associated virus (AAV) replication is dependent on two copies of a 145-bp inverted terminal repeat (ITR) that flank the AAV genome. This is the primary cis-acting element required for productive infection and the generation of recombinant AAV (rAAV) vectors. We have engineered a plasmid (pDD-2) containing only 165 bp of AAV sequence: two copies of the D element, a unique sequence adjacent to the AAV nicking site, flanking a single ITR. When assayed in vivo, this modified hairpin was sufficient for the replication of the plasmid vector when Rep and adenovirus (Ad) helper functions were supplied in trans. pDD-2 replication intermediates were characteristic of the AAV replication scheme in which linear monomer, dimer, and other higher-molecular-weight replicative intermediates are generated. Compared to infectious AAV clones for replication, the modified hairpin vector replicated more efficiently independent of size. Further analysis demonstrated conversion of the input circular plasmid to a linear substrate with AAV terminal repeat elements at either end as an initial step for replication. This conversion was independent of both Rep and Ad helper genes, suggesting the role of host factors in the production of these molecules. The generation of these substrates suggested resolution of the modified terminal repeat through a Holliday-like structure rather than replication as a mechanism for rescue. Production of replicative intermediates via this plasmid substrate were competent not only for AAV DNA replication but also for encapsidation, infection, integration, and subsequent rescue from the chromosome when superinfected with Ad and wild-type AAV. These studies demonstrate that this novel 165-bp ITR substrate is sufficient in cis for the AAV life cycle and should provide a valuable reagent for further dissecting the cis sequences involved in AAV replication, packaging, and integration. In addition, this novel plasmid vector can be used as a substrate for both rAAV vector production and synthetic plasmid vector delivery.

摘要

腺相关病毒(AAV)的复制依赖于位于AAV基因组两侧的两个145bp的反向末端重复序列(ITR)拷贝。这是有效感染和产生重组AAV(rAAV)载体所需的主要顺式作用元件。我们构建了一个仅包含165bp AAV序列的质粒(pDD - 2):两个D元件拷贝,这是一个与AAV切口位点相邻的独特序列,两侧各有一个ITR。在体内检测时,当反式提供Rep和腺病毒(Ad)辅助功能时,这种修饰的发夹结构足以使质粒载体进行复制。pDD - 2复制中间体具有AAV复制模式的特征,即产生线性单体、二聚体和其他高分子量的复制中间体。与用于复制的感染性AAV克隆相比,修饰的发夹载体复制效率更高,且与大小无关。进一步分析表明,输入的环状质粒首先转化为两端带有AAV末端重复元件的线性底物作为复制的起始步骤。这种转化与Rep和Ad辅助基因均无关,表明宿主因子在这些分子产生中的作用。这些底物的产生表明修饰的末端重复序列是通过类Holliday结构进行解析,而不是通过复制作为拯救机制。通过这种质粒底物产生的复制中间体不仅能够进行AAV DNA复制,还能够进行衣壳化、感染、整合,并且当被Ad和野生型AAV超感染时能够从染色体中随后拯救出来。这些研究表明,这种新型的165bp ITR底物在顺式作用下足以支持AAV生命周期,并且应该为进一步剖析AAV复制、包装和整合中涉及的顺式序列提供有价值的试剂。此外,这种新型质粒载体既可以用作rAAV载体生产的底物,也可以用作合成质粒载体递送的底物。

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