体内对雀麦花叶病毒亚基因组RNA合成的要求及体外复制酶核心启动子相互作用
Requirements for brome mosaic virus subgenomic RNA synthesis in vivo and replicase-core promoter interactions in vitro.
作者信息
Sivakumaran K, Choi Seung-Kook, Hema Masarapu, Kao C Cheng
机构信息
Texas A&M University, Department of Biochemistry and Biophysics, College Station, TX 77843, USA.
出版信息
J Virol. 2004 Jun;78(12):6091-101. doi: 10.1128/JVI.78.12.6091-6101.2004.
Based solely on in vitro results, two contrasting models have been proposed for the recognition of the brome mosaic virus (BMV) subgenomic core promoter by the replicase. The first posits that the replicase recognizes at least four key nucleotides in the core promoter, followed by an induced fit, wherein some of the nucleotides base pair prior to the initiation of RNA synthesis (S. Adkins and C. C. Kao, Virology 252:1-8, 1998). The second model posits that a short RNA hairpin in the core promoter serves as a landing pad for the replicase and that at least some of the key nucleotides help form a stable hairpin (P. C. J. Haasnoot, F. Brederode, R. C. L. Olsthoorn, and J. Bol, RNA 6:708-716, 2000; P. C. J. Haasnoot, R. C. L. Olsthoorn, and J. Bol, RNA 8:110-122, 2002). We used transfected barley protoplasts to examine the recognition of the subgenomic core promoter by the BMV replicase. Key nucleotides required for subgenomic initiation in vitro were found to be important for RNA4 levels in protoplasts. In addition, additional residues not required in vitro and the formation of an RNA hairpin within the core promoter were correlated with wild-type RNA4 levels in cells. Using a template competition assay, the core promoter of ca. 20 nucleotides was found to be sufficient for replicase binding. Mutations of the key residues in the core promoter reduced replicase binding, but deletions that disrupt the predicted base pairing in the proposed stem retained binding at wild-type levels. Together, these results indicate that key nucleotides in the BMV subgenomic core promoter direct replicase recognition but that the formation of a stem-loop is required at a step after binding. Additional functional characterization of the subgenomic core promoter was performed. A portion of the promoter for BMV minus-strand RNA synthesis could substitute for the subgenomic core promoter in transfected cells. The comparable sequence from Cowpea Chlorotic Mottle Virus (CCMV) could also substitute for the BMV subgenomic core promoter. However, nucleotides in the CCMV core required for RNA synthesis are not identical to those in BMV, suggesting that the subgenomic core promoter can induce the BMV replicase in interactions needed for subgenomic RNA transcription in vivo.
仅基于体外实验结果,针对复制酶识别雀麦花叶病毒(BMV)亚基因组核心启动子,提出了两种截然不同的模型。第一种模型认为,复制酶识别核心启动子中至少四个关键核苷酸,随后发生诱导契合,即在RNA合成起始之前,部分核苷酸形成碱基对(S. 阿德金斯和C. C. 高,《病毒学》252:1 - 8,1998年)。第二种模型认为,核心启动子中的一个短RNA发夹结构作为复制酶的着陆平台,且至少部分关键核苷酸有助于形成稳定的发夹结构(P. C. J. 哈斯诺特、F. 布雷德罗德、R. C. L. 奥尔斯托恩和J. 博尔,《RNA》6:708 - 716,2000年;P. C. J. 哈斯诺特、R. C. L. 奥尔斯托恩和J. 博尔,《RNA》8:110 - 122,2002年)。我们利用转染的大麦原生质体来研究BMV复制酶对亚基因组核心启动子的识别。发现体外亚基因组起始所需的关键核苷酸对原生质体中RNA4的水平很重要。此外,体外不需要的其他残基以及核心启动子内RNA发夹结构的形成与细胞中野生型RNA4水平相关。通过模板竞争试验,发现约20个核苷酸的核心启动子足以与复制酶结合。核心启动子中关键残基的突变会降低复制酶的结合,但破坏所提议茎中预测碱基对的缺失仍能保持野生型水平的结合。这些结果共同表明,BMV亚基因组核心启动子中的关键核苷酸指导复制酶识别,但茎环结构的形成是在结合后的一个步骤中需要的。对亚基因组核心启动子进行了额外的功能表征。BMV负链RNA合成启动子的一部分可以在转染细胞中替代亚基因组核心启动子。来自豇豆花叶病毒(CCMV)的可比序列也可以替代BMV亚基因组核心启动子。然而,CCMV核心中RNA合成所需的核苷酸与BMV中的并不相同,这表明亚基因组核心启动子可以在体内亚基因组RNA转录所需的相互作用中诱导BMV复制酶。
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