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酵母RNA聚合酶II在体外腺病毒主要晚期启动子处的起始作用。

Initiation by yeast RNA polymerase II at the adenoviral major late promoter in vitro.

作者信息

Lue N F, Flanagan P M, Sugimoto K, Kornberg R D

机构信息

Department of Cell Biology, Beckman Laboratories, Fairchild Center, Stanford School of Medicine, CA 94305.

出版信息

Science. 1989 Nov 3;246(4930):661-4. doi: 10.1126/science.2510298.

Abstract

Transcription of the yeast CYC1 promoter fused to a sequence lacking guanosine residues provided a rapid, sensitive assay of initiation by RNA polymerase II in yeast extracts. Initiation was enhanced by yeast and mammalian activator proteins. The adenoviral major late promoter fused to the G-minus sequence was transcribed in yeast extracts with an efficiency comparable to that observed in HeLa extracts, showing that promoters as well as transcription factors are functionally interchangeable across species. Initiation occurred at different sites, approximately 30 and 63 to 69 base pairs downstream of the TATA element of the adenoviral promoter in HeLa and yeast extracts, respectively, distances characteristic of initiation in the two systems in vivo. A component of the transcription system and not the promoter sequence determines the distance to the initiation site.

摘要

与缺乏鸟苷残基的序列融合的酵母CYC1启动子的转录为酵母提取物中RNA聚合酶II的起始提供了一种快速、灵敏的检测方法。酵母和哺乳动物激活蛋白增强了起始作用。与G-减序列融合的腺病毒主要晚期启动子在酵母提取物中被转录,其效率与在HeLa提取物中观察到的相当,表明启动子以及转录因子在不同物种间功能上是可互换的。起始发生在不同位点,在HeLa和酵母提取物中分别位于腺病毒启动子TATA元件下游约30和63至69个碱基对处,这是两个系统在体内起始的特征距离。转录系统的一个组成部分而非启动子序列决定了到起始位点的距离。

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