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A novel herpes simplex virus type 1 transcript (AL-RNA) antisense to the 5' end of the latency-associated transcript produces a protein in infected rabbits.一种与潜伏相关转录本5'端反义的新型单纯疱疹病毒1型转录本(AL-RNA)在受感染的兔子中产生一种蛋白质。
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High-mobility-group protein I can modulate binding of transcription factors to the U5 region of the human immunodeficiency virus type 1 proviral promoter.高迁移率族蛋白I可调节转录因子与人免疫缺陷病毒1型前病毒启动子U5区域的结合。
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本文引用的文献

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Downstream regulatory elements increase acute and latent herpes simplex virus type 2 latency-associated transcript expression but do not influence recurrence phenotype or establishment of latency.下游调控元件可增加单纯疱疹病毒2型急性和潜伏性潜伏相关转录本的表达,但不影响复发表型或潜伏的建立。
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Reversal of intrinsic DNA bends in the IFN beta gene enhancer by transcription factors and the architectural protein HMG I(Y).转录因子和结构蛋白HMG I(Y)对干扰素β基因增强子中固有DNA弯曲的逆转作用
Cell. 1995 Dec 29;83(7):1101-11. doi: 10.1016/0092-8674(95)90137-x.
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Organization and analysis of the promoter region and 5' non-coding exons of the human c-src proto-oncogene.人类c-src原癌基因启动子区域及5'非编码外显子的组织与分析
Oncogene. 1993 Jul;8(7):1973-81.
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Gene splicing by overlap extension.重叠延伸基因剪接
Methods Enzymol. 1993;217:270-9. doi: 10.1016/0076-6879(93)17067-f.
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Multiple promoters direct tissue-specific expression of the rat BDNF gene.多个启动子指导大鼠脑源性神经营养因子基因的组织特异性表达。
Neuron. 1993 Mar;10(3):475-89. doi: 10.1016/0896-6273(93)90335-o.
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T3 receptor suppression of Sp1-dependent transcription from the epidermal growth factor receptor promoter via overlapping DNA-binding sites.T3 受体通过重叠的 DNA 结合位点抑制表皮生长因子受体启动子上 Sp1 依赖性转录。
J Biol Chem. 1993 Jul 25;268(21):16065-73.
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A strong promoter element is located between alternative exons of a gene encoding the human gamma-aminobutyric acid-type A receptor beta 3 subunit (GABRB3).一个强启动子元件位于编码人类γ-氨基丁酸A型受体β3亚基(GABRB3)的基因的可变外显子之间。
J Biol Chem. 1993 Feb 25;268(6):4420-8.
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SAR-dependent mobilization of histone H1 by HMG-I/Y in vitro: HMG-I/Y is enriched in H1-depleted chromatin.体外HMG-I/Y依赖于SAR的组蛋白H1动员:HMG-I/Y在H1缺失的染色质中富集。
EMBO J. 1993 Aug;12(8):3237-47. doi: 10.1002/j.1460-2075.1993.tb05993.x.
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A novel cis-acting element controlling the rat CYP2D5 gene and requiring cooperativity between C/EBP beta and an Sp1 factor.一种控制大鼠CYP2D5基因的新型顺式作用元件,需要C/EBPβ和一个Sp1因子之间的协同作用。
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10
Decreased reporter gene expression during latent infection with HSV LAT promoter constructs.单纯疱疹病毒潜伏相关转录本(HSV LAT)启动子构建体潜伏感染期间报告基因表达降低。
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一种高迁移率族蛋白参与单纯疱疹病毒潜伏激活启动子2的转录活性

Involvement of a high-mobility-group protein in the transcriptional activity of herpes simplex virus latency-active promoter 2.

作者信息

French S W, Schmidt M C, Glorioso J C

机构信息

Department of Molecular Genetics and Biochemistry, University of Pittsburgh School of Medicine, Pennsylvania 15261, USA.

出版信息

Mol Cell Biol. 1996 Oct;16(10):5393-9. doi: 10.1128/MCB.16.10.5393.

DOI:10.1128/MCB.16.10.5393
PMID:8816451
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC231538/
Abstract

Latency-active promoter 2 (LAP 2) is a TATA-less promoter in herpes simplex virus type 1 (HSV-1) that can express genes during viral latency. Four regions of LAP2 are protected from DNase I digestion in vitro by either HeLa cell nuclear extracts or purified Sp1. Transient gene expression assays of LAP2 substitution mutants demonstrate that two of the regions protected by Sp1 and three other regions protected by nuclear extract are important for promoter function. The mutation causing the most significant reduction in expression alters a stretch of 23 thymidine residues (T23) that binds a protein with several properties common to high-mobility-group (HMG) proteins. The T23 binding activity is heat stable, can be inhibited by poly(dA-dT).poly(dA-dT), and is inhibited by minor-groove-binding drugs. Antiserum directed against HMG I(Y) blocked the formation of one of the DNA-protein complexes on the T23 oligonucleotide, suggesting that a protein antigenically related to HMG I(Y) binds to LAP2 in vitro. Direct evidence of HMG I(Y) involvement in LAP2 function is provided by the findings that recombinant HMG I(Y) protein facilitates Sp1 binding to LAP2 in mobility shift assays and that antisense HMG I(Y) RNA specifically inhibits LAP2 function in vivo. These results suggest that DNA structure may be an important determinant of the activity of a promoter that is capable of escaping the global shutoff of transcription that occurs during viral latency.

摘要

潜伏激活启动子2(LAP 2)是1型单纯疱疹病毒(HSV - 1)中的一种无TATA框启动子,它能在病毒潜伏期间表达基因。在体外,LAP2的四个区域可被HeLa细胞核提取物或纯化的Sp1保护而免受DNase I消化。对LAP2替代突变体进行的瞬时基因表达分析表明,受Sp1保护的两个区域以及受核提取物保护的其他三个区域对启动子功能很重要。导致表达最显著降低的突变改变了一段23个胸腺嘧啶残基(T23),该序列与一种具有高迁移率族(HMG)蛋白若干特性的蛋白质结合。T23结合活性具有热稳定性,可被聚(dA - dT)·聚(dA - dT)抑制,也可被小沟结合药物抑制。针对HMG I(Y)的抗血清可阻断T23寡核苷酸上一种DNA - 蛋白质复合物的形成,这表明一种与HMG I(Y)抗原相关的蛋白质在体外与LAP2结合。重组HMG I(Y)蛋白在迁移率变动分析中促进Sp1与LAP2结合,以及反义HMG I(Y)RNA在体内特异性抑制LAP2功能的研究结果,为HMG I(Y)参与LAP2功能提供了直接证据。这些结果表明,DNA结构可能是一个能够逃避病毒潜伏期间发生的全局转录关闭的启动子活性的重要决定因素。