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5型腺病毒E1b基因转录的多组分顺式激活因子。

A multicomponent cis-activator of transcription of the E1b gene of adenovirus type 5.

作者信息

Spector D J, Parks C L, Knittle R A

机构信息

Department of Microbiology and Immunology, Pennsylvania State University, College of Medicine, Hershey 17033.

出版信息

Virology. 1993 May;194(1):128-36. doi: 10.1006/viro.1993.1242.

DOI:10.1006/viro.1993.1242
PMID:8480416
Abstract

We report that transcription of the adenovirus type 5 E1b gene is activated substantially in cis by sequences located between positions -362 and -49 with respect to the RNA start site. DNA fragments consisting of the -362 to -49 sequences, or subsets thereof, were inserted into a reporter plasmid containing a minimal E1b promoter (positions -48 to +14) joined to the Escherichia coli cat gene. In the presence of cotransfected E1a and E1b genes in trans, CAT enzyme synthesis in transfected KB cells was stimulated about 20-fold by sequences from -362 to -49 (XY) in cis and to a lesser extent by sequences from either -362 to -128 (X) or -127 to -49 (Y). Adenoviruses were isolated lacking the X, Y, or XY sequences and KB cells were infected with one of the mutants, as well as wild-type virus to provide E1a and E1b in trans. Deletion of both X and Y resulted in a 20-fold reduction in early E1b RNA and a 12-fold reduction in late RNA. Deletion of X or Y alone produced up to 5-fold reductions in early or late E1b RNA accumulation. In vitro DNA-protein interactions in the Y sequence were revealed by modification of the procedure used for previous detection of X region footprints. These data indicate that X and Y sequences, which include E1a protein coding and 3' untranslated DNA, also participate in DNA-protein interactions necessary for high levels of E1b promoter activity. The presence of such overlapping genetic elements raises the interesting possibility that functional E1a and E1b mRNAs must be synthesized from separate templates.

摘要

我们报道,相对于RNA起始位点,腺病毒5型E1b基因的转录在顺式作用下被位于-362至-49位之间的序列显著激活。由-362至-49序列或其亚序列组成的DNA片段被插入到一个报告质粒中,该质粒含有与大肠杆菌cat基因相连的最小E1b启动子(-48至+14位)。在共转染E1a和E1b基因反式存在的情况下,转染的KB细胞中CAT酶的合成在顺式作用下被-362至-49序列(XY)刺激约20倍,而被-362至-128序列(X)或-127至-49序列(Y)刺激的程度较小。分离出缺失X、Y或XY序列的腺病毒,并将其中一种突变体以及野生型病毒感染KB细胞以反式提供E1a和E1b。X和Y序列均缺失导致早期E1b RNA减少20倍,晚期RNA减少12倍。单独缺失X或Y导致早期或晚期E1b RNA积累最多减少5倍。通过改进先前用于检测X区域足迹的方法,揭示了Y序列中的体外DNA-蛋白质相互作用。这些数据表明,包括E1a蛋白编码区和3'非翻译DNA的X和Y序列也参与了高水平E1b启动子活性所需的DNA-蛋白质相互作用。这种重叠遗传元件的存在提出了一个有趣的可能性,即功能性E1a和E1b mRNA必须从单独的模板合成。

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