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多瘤病毒DNA整合到转化大鼠细胞的染色体DNA中会导致侧翼细胞序列的缺失。

Integration of polyoma virus DNA into chromosomal DNA in transformed rat cells causes deletion of flanking cell sequences.

作者信息

Neer A, Baran N, Manor H

出版信息

J Gen Virol. 1983 Jan;64 (Pt 1):69-82. doi: 10.1099/0022-1317-64-1-69.

Abstract

In order to find out whether polyoma virus (Py) integration into chromosomes causes rearrangements in the cell DNA flanking the integration site, we have mapped the flanking sequences in the inducible LPT line of Py-transformed rat cells and the corresponding sequences in normal rat fibroblasts, and then compared the two maps. To carry out this study we have cloned a segment including Py DNA and flanking sequences in the bacteriophage vector lambda gt WES and subcloned the flanking cell DNA in a bacterial plasmid. We performed a Southern blot analysis of LPT and rat fibroblast DNA digested with various restriction enzymes and used the cloned flanking cell DNA and Py DNA as hybridization probes. Autoradiography of the LPT DNA blots revealed two sets of fragments. One set includes fragments containing both Py and cell DNA sequences; the second set consists of fragments which contain no virus DNA sequences, and are identical to the fragments observed in the corresponding normal rat DNA digests. These data indicate that LPT cells are heterozygous with respect to the Py inserts. The same data were used to map the flanking sequences in the two types of cells. A comparison between the two maps revealed that a 3.0 kb cell DNA segment, which is located next to the unoccupied integration site in the normal rat chromosomes, has been deleted from the LPT chromosome which carries Py DNA, but not from the LPT chromosome which does not carry the virus DNA. The implications for papovavirus integration are discussed.

摘要

为了弄清楚多瘤病毒(Py)整合到染色体中是否会导致整合位点侧翼的细胞DNA发生重排,我们绘制了Py转化的大鼠细胞的可诱导LPT系中的侧翼序列图谱以及正常大鼠成纤维细胞中的相应序列图谱,然后比较了这两张图谱。为了开展这项研究,我们在噬菌体载体λgt WES中克隆了一个包含Py DNA和侧翼序列的片段,并将侧翼细胞DNA亚克隆到一个细菌质粒中。我们对用各种限制酶消化的LPT和大鼠成纤维细胞DNA进行了Southern印迹分析,并使用克隆的侧翼细胞DNA和Py DNA作为杂交探针。LPT DNA印迹的放射自显影显示出两组片段。一组包括同时含有Py和细胞DNA序列的片段;第二组由不包含病毒DNA序列的片段组成,这些片段与在相应的正常大鼠DNA消化物中观察到的片段相同。这些数据表明LPT细胞对于Py插入片段是杂合的。相同的数据被用于绘制两种细胞类型中的侧翼序列图谱。两张图谱的比较显示,在正常大鼠染色体中位于未占据整合位点旁边的一个3.0 kb细胞DNA片段,已从携带Py DNA的LPT染色体中缺失,但未从不携带病毒DNA的LPT染色体中缺失。文中讨论了乳头瘤病毒整合的意义。

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