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赋予人类RNA聚合酶I启动子特异性的转录因子的纯化与特性分析

Purification and characterization of a transcription factor that confers promoter specificity to human RNA polymerase I.

作者信息

Learned R M, Cordes S, Tjian R

出版信息

Mol Cell Biol. 1985 Jun;5(6):1358-69. doi: 10.1128/mcb.5.6.1358-1369.1985.

Abstract

A whole-cell HeLa extract was fractionated into two components required for accurate in vitro transcription of human rRNA. One fraction contained endogenous RNA polymerase I, and the second component contained a factor (SL1) that confers promoter selectivity to RNA polymerase I. Analysis of mutant templates suggests that the core control element of the rRNA promoter is required for activation of transcription by SL1. We purified SL1 approximately 100,000-fold by column chromatography and have shown that the addition of SL1 can reprogram the otherwise nonpermissive mouse transcription system to recognize and initiate accurate RNA synthesis from human rDNA. Antibodies raised against SL1 bind preferentially to a protein localized in the nucleolus of primate cells and specifically inhibit in vitro transcription initiating from the human rRNA promoter. By contrast, anti-SL1 does not react with the nucleolus of rodent cells and has no effect on the in vitro synthesis of mouse rRNA by a transcription system derived from mouse cells. These findings suggest that SL1 is a selectivity factor present in the nucleolus that imparts promoter recognition to RNA polymerase I and that can discriminate between rRNA promoters from different species.

摘要

将全细胞HeLa提取物分级分离成两个组分,这两个组分是体外准确转录人rRNA所必需的。一个组分含有内源性RNA聚合酶I,另一个组分含有赋予RNA聚合酶I启动子选择性的因子(SL1)。对突变模板的分析表明,rRNA启动子的核心控制元件是SL1激活转录所必需的。我们通过柱色谱法将SL1纯化了约100,000倍,并表明添加SL1可以重新编程原本不允许的小鼠转录系统,使其能够识别并从人rDNA起始准确的RNA合成。针对SL1产生的抗体优先结合定位于灵长类细胞核仁中的一种蛋白质,并特异性抑制从人rRNA启动子起始的体外转录。相比之下,抗SL1抗体不与啮齿动物细胞的核仁发生反应,并且对源自小鼠细胞的转录系统体外合成小鼠rRNA没有影响。这些发现表明,SL1是存在于核仁中的一种选择性因子,它赋予RNA聚合酶I启动子识别能力,并且能够区分来自不同物种的rRNA启动子。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0bff/366865/bf094fdff947/molcellb00102-0172-a.jpg

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