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腺病毒主要晚期衰减位点处的转录暂停、停滞和通读。

Transcriptional pausing, arrest, and readthrough at the adenovirus major late attenuation site.

作者信息

Hawley D K, Wiest D K, Holtz M S, Wang D

机构信息

Institute of Molecular Biology, University of Oregon, Eugene 97403.

出版信息

Cell Mol Biol Res. 1993;39(4):339-48.

PMID:8312969
Abstract

RNA polymerase II (pol II) transcription complexes initiated from the adenovirus major late promoter can become blocked both in vitro and in vivo at a specific site within the first intron of the transcription unit. In vitro, polymerases that fail to read through the major late attenuation site remain stably bound to the template in a ternary complex that is indefinitely blocked from continuing elongation, a phenomenon referred to as "arrest." Elongation factor SII has been shown both to promote readthrough of this and other arrest sites and to stimulate a previously unknown 3' to 5' exonuclease activity of pol II. We have proposed that the two activities are related and that SII promotes readthrough by means of the enhancement of the exonuclease activity. In the experiments reported here, we have tested several features of that model. In particular, we have examined the hypothesis that SII stimulates readthrough by allowing the polymerase to undergo multiple cycles of removal and resynthesis of RNA bases preceding the attenuation site. In addition, we present experimental support for the proposal that the length of time polymerase pauses at the attenuation site is important to the efficiency of arrest. The results of these experiments are discussed in the context of the model.

摘要

从腺病毒主要晚期启动子起始的RNA聚合酶II(pol II)转录复合物,在体外和体内均可在转录单元第一个内含子内的特定位点受阻。在体外,未能通读主要晚期衰减位点的聚合酶会以三元复合物的形式稳定地结合在模板上,该复合物被无限期地阻止继续延伸,这种现象被称为“停滞”。已表明延伸因子SII既能促进此衰减位点及其他停滞位点的通读,又能刺激pol II一种先前未知的3'到5'核酸外切酶活性。我们提出这两种活性是相关的,并且SII通过增强核酸外切酶活性来促进通读。在本文报道的实验中,我们测试了该模型的几个特征。特别是,我们检验了这样一个假说,即SII通过允许聚合酶在衰减位点之前对RNA碱基进行多次去除和重新合成的循环来刺激通读。此外,我们为以下提议提供了实验支持,即聚合酶在衰减位点暂停的时间长度对停滞效率很重要。这些实验的结果将在该模型的背景下进行讨论。

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