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未整合的逆转录病毒DNA重排很复杂,是多种遗传决定因素的结果。

Rearrangements in unintegrated retroviral DNA are complex and are the result of multiple genetic determinants.

作者信息

Olsen J C, Bova-Hill C, Grandgenett D P, Quinn T P, Manfredi J P, Swanstrom R

机构信息

Department of Biochemistry, University of North Carolina, Chapel Hill 27599.

出版信息

J Virol. 1990 Nov;64(11):5475-84. doi: 10.1128/JVI.64.11.5475-5484.1990.

Abstract

We used a replication-competent retrovirus shuttle vector based on a DNA clone of the Schmidt-Ruppin A strain of Rous sarcoma virus to characterize rearrangements in circular viral DNA. In this system, circular molecules of viral DNA present after acute infection of cultured cells were cloned as plasmids directly into bacteria. The use of a replication-competent shuttle vector permitted convenient isolation of a large number of viral DNA clones; in this study, over 1,000 clones were analyzed. The circular DNA molecules could be placed into a limited number of categories. Approximately one-third of the rescued molecules had deletions in which one boundary was very near the edge of a long terminal repeat (LTR) unit. Subtle differences in the patterns of deletions in circular DNAs with one versus two copies of the LTR sequence were observed, and differences between deletions emanating from the right and left boundaries of the LTR were seen. A virus with a missense mutation in the region of the pol gene responsible for integration and exhibiting a temperature sensitivity phenotype for replication had a marked decrease in the number of rescued molecules with LTR-associated deletions when infection was performed at the nonpermissive temperature. This result suggests that determinants in the pol gene, possibly in the integration protein, play a role in the generation of LTR-associated deletions. Sequences in a second region of the genome, probably within the viral gag gene, were also found to affect the types of circular viral DNA molecules present after infection. Sequences in this region from different strains of avian sarcoma-leukosis viruses influenced the fraction of circular molecules with LTR-associated deletions, as well as the relative proportion of circular molecules with either one or two copies of the LTR. Thus, the profile of rearrangements in unintegrated viral DNA is complex and dependent upon the nature of sequences in the gag and pol regions.

摘要

我们使用了一种基于劳斯肉瘤病毒施密特 - 鲁平A株DNA克隆的具有复制能力的逆转录病毒穿梭载体,来表征环状病毒DNA中的重排。在这个系统中,培养细胞急性感染后出现的病毒DNA环状分子被直接作为质粒克隆到细菌中。使用具有复制能力的穿梭载体便于大量分离病毒DNA克隆;在本研究中,分析了超过1000个克隆。环状DNA分子可分为有限的几类。大约三分之一的拯救分子存在缺失,其中一个边界非常靠近长末端重复序列(LTR)单元的边缘。观察到具有一个与两个LTR序列拷贝的环状DNA中缺失模式的细微差异,并且还发现了源自LTR右边界和左边界的缺失之间的差异。当在非允许温度下进行感染时,在负责整合的pol基因区域具有错义突变且复制表现出温度敏感性表型的病毒,其具有LTR相关缺失的拯救分子数量显著减少。这一结果表明,pol基因中的决定因素,可能是整合蛋白中的决定因素,在LTR相关缺失的产生中起作用。基因组第二个区域的序列,可能在病毒gag基因内,也被发现会影响感染后存在的环状病毒DNA分子的类型。来自不同禽肉瘤 - 白血病病毒株的该区域序列影响具有LTR相关缺失的环状分子的比例,以及具有一个或两个LTR拷贝的环状分子的相对比例。因此,未整合病毒DNA中的重排情况很复杂,并且取决于gag和pol区域中序列的性质。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/eba6/248599/a175b3ad001d/jvirol00066-0254-a.jpg

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