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潜伏感染的底特律6细胞中腺相关病毒DNA的组织形式。

Organization of adeno-associated virus DNA in latently infected Detroit 6 cells.

作者信息

Kotin R M, Berns K I

机构信息

Department of Microbiology, Cornell University Medical College, New York, New York 10021.

出版信息

Virology. 1989 Jun;170(2):460-7. doi: 10.1016/0042-6822(89)90437-6.

Abstract

The DNA of a human dependovirus, adeno-associated virus (AAV), integrates into the cellular genome under conditions nonpermissive for viral DNA replication. The AAV DNA can be rescued from the cellular genome by superinfection with a helper virus, e.g., adenovirus. To characterize the organization of the proviral DNA in greater detail, we isolated three proviral subfragments from a latently infected human cell line. Our findings, based on sequence analysis, restriction enzyme mapping, and genomic blots, demonstrate that the viral terminal repeats (trs) are present at or near the cellular/viral DNA junctions, but significant deletions of the tr sequences have occurred. One of the proviral clones has extensive rearrangements which apparently occurred by nonhomologous recombination. The tail-to-tail arrangement of one of the proviral clones is consistent with limited DNA replication prior to integration by a mechanism similar to that seen in a productive infection. Although there are BamH1 fragments in the cell line we have characterized, which are the right size to have come from a head-to-tail tandem repeat, critical double digests show no evidence for the presence of a head-to-tail tandem repeat of wild-type proviral DNA. Use of probes derived from the flanking cellular DNA enabled us to determine that in this cell line the viral DNA had integrated into a site composed of nonrepetitive sequences.

摘要

人依赖病毒——腺相关病毒(AAV)的DNA在不利于病毒DNA复制的条件下整合到细胞基因组中。通过辅助病毒(如腺病毒)的超感染,可从细胞基因组中拯救出AAV DNA。为了更详细地描述前病毒DNA的组织情况,我们从一个潜伏感染的人细胞系中分离出了三个前病毒亚片段。基于序列分析、限制性内切酶图谱分析和基因组印迹分析的结果表明,病毒末端重复序列(TRs)存在于细胞/病毒DNA连接处或其附近,但TR序列发生了显著缺失。其中一个前病毒克隆有广泛的重排,显然是通过非同源重组发生的。其中一个前病毒克隆的尾对尾排列与整合前通过类似于在生产性感染中所见机制进行的有限DNA复制一致。尽管在我们所研究的细胞系中有BamH1片段,其大小正好来自头对头串联重复序列,但关键的双酶切结果并未显示存在野生型前病毒DNA的头对头串联重复序列。使用来自侧翼细胞DNA的探针使我们能够确定,在这个细胞系中,病毒DNA已整合到一个由非重复序列组成的位点。

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