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牛腺相关病毒和禽腺相关病毒的表达谱与5型腺相关病毒的表达谱显示出显著相似性。

Expression profiles of bovine adeno-associated virus and avian adeno-associated virus display significant similarity to that of adeno-associated virus type 5.

作者信息

Qiu Jianming, Cheng Fang, Pintel David J

机构信息

Life Sciences Center, University of Missouri-Columbia, 1201 Rollins Road, Columbia, MO 65211, USA.

出版信息

J Virol. 2006 Jun;80(11):5482-93. doi: 10.1128/JVI.02735-05.

Abstract

We present the first detailed expression profiles of nonprimate-derived adeno-associated viruses, namely, bovine adeno-associated virus (B-AAV) and avian adeno-associated virus (A-AAV), which were obtained after the infection of cell lines derived from their natural hosts. In general, the profiles of B-AAV and A-AAV were quite similar to that of AAV5; however, both exhibited features found for AAV2 as well. Like adeno-associated virus type 5 (AAV5), B-AAV and A-AAV utilized an internal polyadenylation site [(pA)p]; however, it was used to greater relative levels by B-AAV than by A-AAV. Similar to AAV5, >99% of B-AAV RNAs generated from upstream promoters were polyadenylated at (pA)p and hence not spliced. In contrast, ca. 50% of the A-AAV RNAs generated from upstream promoters read through (pA)p, as seen for AAV2. However, A-AAV generated lower levels of spliced P5 and P19 products than does AAV2, suggesting that A-AAV generates lower relative levels of Rep 68 and Rep 40. An additional difference in the expression profile of these viruses was that B-AAV generated a greater level of ITR-initiated RNAs than did A-AAV or AAV5. In addition, we demonstrate that, like AAV2, transactivation of transcription of the capsid-gene promoter of B-AAV required both adenovirus and targeting of its Rep protein to the transcription template; however, expression of the capsid-gene promoter of A-AAV was, like AAV5, largely independent of both adenovirus and its Rep proteins.

摘要

我们展示了非灵长类动物源腺相关病毒,即牛腺相关病毒(B-AAV)和禽腺相关病毒(A-AAV)的首个详细表达谱,这些表达谱是在感染源自其天然宿主的细胞系后获得的。总体而言,B-AAV和A-AAV的表达谱与AAV5相当相似;然而,它们也都表现出AAV2所具有的特征。与5型腺相关病毒(AAV5)一样,B-AAV和A-AAV利用一个内部聚腺苷酸化位点[(pA)p];不过,B-AAV对其的相对利用水平高于A-AAV。与AAV5类似,从上游启动子产生的B-AAV RNA中>99%在(pA)p处进行了聚腺苷酸化,因此没有发生剪接。相比之下,从上游启动子产生的A-AAV RNA中约50%如AAV2那样通读了(pA)p。然而,A-AAV产生的剪接P5和P19产物水平低于AAV2,这表明A-AAV产生的Rep 68和Rep 40相对水平较低。这些病毒表达谱的另一个差异在于,B-AAV产生的ITR起始RNA水平高于A-AAV或AAV5。此外,我们证明,与AAV2一样,B-AAV衣壳基因启动子的转录反式激活既需要腺病毒,也需要将其Rep蛋白靶向转录模板;然而,A-AAV衣壳基因启动子的表达与AAV5一样,在很大程度上独立于腺病毒及其Rep蛋白。

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