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双生病毒外壳蛋白启动子受AL2蛋白(TrAP)调控:激活和去抑制机制的证据

Regulation of a geminivirus coat protein promoter by AL2 protein (TrAP): evidence for activation and derepression mechanisms.

作者信息

Sunter G, Bisaro D M

机构信息

Plant Biotechnology Center, Ohio State University, Columbus 43210-1002, USA.

出版信息

Virology. 1997 Jun 9;232(2):269-80. doi: 10.1006/viro.1997.8549.

Abstract

Tomato golden mosaic virus (TGMV) is a bipartite member of the subgroup III Geminiviridae. Like all geminiviruses, TGMV replicates in the nucleus of susceptible cells by rolling circle replication (RCR). Double-stranded replicative form DNA generated during RCR serves as template for the transcription of viral genes by RNA polymerase II and the associated cellular transcription machinery. Previous studies in tobacco protoplasts and Nicotiana benthamiana leaf discs have shown that the viral AL2 gene product transactivates expression of the coat protein (CP) and BR1 movement protein genes, and that activation occurs at the level of transcription. Because of its function and properties, we propose the name TrAP, transcriptional activator protein, for the AL2 gene product. Using transgenes consisting of complete and truncated versions of the CP promoter fused to the GUS reporter gene, we show in the studies presented here that TrAP is required for CP gene expression in both mesophyll and phloem tissues. Surprisingly, TrAP appears to induce CP expression by different mechanisms in different cell types: it may activate the CP promoter in mesophyll cells, and acts to derepress the promoter in phloem tissue. In addition, TrAP is clearly capable of inducing the expression of responsive chromosomal promoters and could, in principle, activate host genes. Distinct viral sequence elements mediate expression and derepression in phloem and activation in mesophyll, suggesting that TrAP interacts with different components of the cellular transcription machinery to accomplish CP gene expression in different cell types, and underscoring the intricacy and complexity of virus-host interactions.

摘要

番茄金色花叶病毒(TGMV)是双生病毒科III亚组的一种双分体病毒。与所有双生病毒一样,TGMV通过滚环复制(RCR)在敏感细胞的细胞核中进行复制。RCR过程中产生的双链复制型DNA作为RNA聚合酶II和相关细胞转录机制转录病毒基因的模板。先前在烟草原生质体和本氏烟草叶片圆盘上的研究表明,病毒AL2基因产物可反式激活外壳蛋白(CP)和BR1运动蛋白基因的表达,且这种激活发生在转录水平。基于其功能和特性,我们提议将AL2基因产物命名为TrAP,即转录激活蛋白。在此呈现的研究中,我们使用由与GUS报告基因融合的CP启动子的完整和截短版本组成的转基因,表明TrAP是叶肉组织和韧皮部组织中CP基因表达所必需的。令人惊讶的是,TrAP似乎在不同细胞类型中通过不同机制诱导CP表达:它可能在叶肉细胞中激活CP启动子,并在韧皮部组织中发挥作用使启动子去抑制。此外,TrAP显然能够诱导反应性染色体启动子的表达,并且原则上可以激活宿主基因。不同的病毒序列元件介导韧皮部中的表达和去抑制以及叶肉中的激活,这表明TrAP与细胞转录机制的不同组分相互作用,以在不同细胞类型中完成CP基因表达,并强调了病毒 - 宿主相互作用的复杂性和 intricacy。

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