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细胞蛋白与BK病毒DNA调控区域的结合。

Binding of cellular proteins to the regulatory region of BK virus DNA.

作者信息

Markowitz R B, Dynan W S

机构信息

Department of Chemistry and Biochemistry, University of Colorado, Boulder 80309-0215.

出版信息

J Virol. 1988 Sep;62(9):3388-98. doi: 10.1128/JVI.62.9.3388-3398.1988.

Abstract

The human papovavirus BK has a noncoding regulatory region located between the divergently transcribed early and late coding regions. Many strains of BK virus (BKV) have direct DNA sequence repeats in the regulatory region, although the number and extent of these repeats varies widely between independent isolates. Until recently, little was known about the individual functional elements within the BKV regulatory region, and the biological significance of the variable repeat structure has been unclear. To characterize the interaction between sequences in the BKV regulatory region and host cell transcription factors, we have carried out DNase I footprinting and competitive binding experiments on three strains of BKV, including one strain that does not contain direct sequence repeats. We have used relatively crude fractions from HeLa cell nuclear extracts, as well as DNA affinity-purified preparations of proteins. Our results demonstrate that BK(Dunlop), BK(WW), and BK(MM) each contain multiple binding sites for a factor, NF-BK, that is a member of the nuclear factor 1 family of transcription factors. We predict the presence of three to eight binding sites for NF-BK in the other strains of BKV for which a DNA sequence is available. This suggests that the binding of this protein is likely to be required for biological activity of the virus. In addition to NF-BK sites, BK(WW) and BK(MM) each contain a single binding site for transcription factor Sp1, and BK(Dunlop) contains two binding sites for transcription factor AP-1. The AP-1 sites in BK(Dunlop) span the junction of adjacent direct repeats, suggesting that repeat formation may be an important mechanism for de novo formation of binding sites not present in a parental strain.

摘要

人乳头多瘤空泡病毒BK在早期和晚期编码区反向转录之间有一个非编码调控区。许多BK病毒(BKV)毒株在调控区有直接的DNA序列重复,尽管这些重复的数量和范围在独立分离株之间差异很大。直到最近,人们对BKV调控区内的单个功能元件知之甚少,可变重复结构的生物学意义也不清楚。为了表征BKV调控区序列与宿主细胞转录因子之间的相互作用,我们对三株BKV进行了DNase I足迹分析和竞争性结合实验,其中包括一株不含直接序列重复的毒株。我们使用了来自HeLa细胞核提取物的相对粗提物,以及DNA亲和纯化的蛋白质制剂。我们的结果表明,BK(邓洛普)、BK(WW)和BK(MM)各自含有转录因子核因子1家族成员NF-BK的多个结合位点。我们预测在其他有DNA序列的BKV毒株中存在三到八个NF-BK结合位点。这表明该蛋白的结合可能是病毒生物学活性所必需的。除了NF-BK位点外,BK(WW)和BK(MM)各自含有转录因子Sp1的一个结合位点,BK(邓洛普)含有转录因子AP-1的两个结合位点。BK(邓洛普)中的AP-1位点跨越相邻直接重复序列的交界处,这表明重复序列的形成可能是亲本毒株中不存在的结合位点从头形成的重要机制。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b9bf/253462/e6154cc2a4a5/jvirol00088-0329-a.jpg

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