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High intrinsic hydrolytic activity of cyanobacterial RNA polymerase compensates for the absence of transcription proofreading factors

机译:青霉菌RNA聚合酶的高固有水解活性补偿了没有转录校对因子的情况

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The vast majority of organisms possess transcription elongation factors, the functionally similar bacterial Gre and eukaryotic/archaeal TFIIS/TFS. Their main cellular functions are to proofread errors of transcription and to restart elongation via stimulation of RNA hydrolysis by the active centre of RNA polymerase (RNAP). However, a number of taxons lack these factors, including one of the largest and most ubiquitous groups of bacteria, cyanobacteria. Using cyanobacterial RNAP as a model, we investigated alternative mechanisms for maintaining a high fidelity of transcription and for RNAP arrest prevention. We found that this RNAP has very high intrinsic proofreading activity, resulting in nearly as low a level of in vivo mistakes in RNA as Escherichia coli. Features of the cyanobacterial RNAP hydrolysis are reminiscent of the Gre-assisted reaction—the energetic barrier is similarly low, and the reaction involves water activation by a general base. This RNAP is resistant to ubiquitous and most regulatory pausing signals, decreasing the probability to go off-pathway and thus fall into arrest. We suggest that cyanobacterial RNAP has a specific Trigger Loop domain conformation, and isomerises easier into a hydrolytically proficient state, possibly aided by the RNA 3′-end. Cyanobacteria likely passed these features of transcription to their evolutionary descendants, chloroplasts.
机译:绝大多数生物具有转录伸长因子,功能性相似的细菌GRE和真核/古氏菌/ TFS。它们的主要细胞功能是通过RNA聚合酶(RNAP)的活性中心刺激RNA水解的校对和重新启动伸长率。然而,许多稗级缺乏这些因素,包括最大,最无处不在的细菌,蓝藻之一。使用蓝藻RNAP作为模型,我们研究了维持转录高保真度和RNAP逮捕预防的替代机制。我们发现,该RNAP具有非常高的内在校样活动,导致RNA中的体内错误差异几乎低于RNA作为大肠杆菌。蓝细菌RNAP水解的特征是让抗体辅助反应的激发 - 能量屏障类似地低,反应涉及一般碱的水活化。该RNAP对普遍存在和最具监管暂停信号的耐受性,降低了途径的概率,因此陷入困境。我们建议蓝细菌RNAP具有特定的触发环形域构象,并且异构体更容易进入水解熟化状态,可能由RNA 3'-END辅助。 Cyanobacteria可能将这些特征通过了转录到其进化的后代,叶绿体。

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