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与雌激素反应元件结合的人类雌激素受体会使DNA弯曲。

Human estrogen receptor bound to an estrogen response element bends DNA.

作者信息

Nardulli A M, Greene G L, Shapiro D J

机构信息

Department of Physiology and Biophysics, University of Illinois, Urbana 61801.

出版信息

Mol Endocrinol. 1993 Mar;7(3):331-40. doi: 10.1210/mend.7.3.8483477.

Abstract

We have used gel mobility shift assays to examine changes in DNA bending induced by binding of human estrogen receptor (hER) to a series of estrogen response element (ERE) containing DNA fragments. Competition experiments with ERE-containing DNA fragments and antibody supershift experiments demonstrated that ER in crude extracts from MCF-7 human breast cancer cells exhibited specific interaction with the ERE. Using DNA bending standards, we found that binding of ER to a single ERE induced a reproducible DNA bend of 56 degrees. This was 1.65-fold greater than the 34 degrees bending angle we recently reported for binding of bacterially expressed ER DNA binding domain. The DNA bending angle induced was the same whether the salt-extracted receptor was unoccupied, occupied by 17 beta-estradiol, or occupied by trans-hydroxytamoxifen. To determine if proteins associated with ER in MCF-7 cells affect the degree of bending, we examined the ability of partially purified hER expressed in yeast to bend DNA. The degree of bending induced by the partially purified yeast ER was the same as the bending induced by crude MCF-7 cell ER. More highly purified ER from yeast extracts did not bind to an ERE-containing DNA fragment, suggesting that additional proteins may play an important role in the interaction of the ER with the ERE. When two EREs were present in the DNA fragment, a small but reproducible increase in bending was observed. Our demonstration that binding of hER to the ERE induces DNA bending suggests a possible role for DNA bending in ER-induced transcription activation.

摘要

我们已使用凝胶迁移率变动分析来检测人雌激素受体(hER)与一系列含雌激素反应元件(ERE)的DNA片段结合所诱导的DNA弯曲变化。用含ERE的DNA片段进行的竞争实验和抗体超迁移实验表明,MCF-7人乳腺癌细胞粗提物中的ER与ERE表现出特异性相互作用。使用DNA弯曲标准,我们发现ER与单个ERE的结合诱导了56度的可重复DNA弯曲。这比我们最近报道的细菌表达的ER DNA结合结构域结合时的34度弯曲角度大1.65倍。无论盐提取的受体是未被占据、被17β-雌二醇占据还是被反式羟基他莫昔芬占据,所诱导的DNA弯曲角度都是相同的。为了确定MCF-7细胞中与ER相关的蛋白质是否影响弯曲程度,我们检测了酵母中表达的部分纯化的hER使DNA弯曲的能力。部分纯化的酵母ER诱导的弯曲程度与MCF-7细胞粗提物诱导的弯曲程度相同。酵母提取物中更高纯度的ER不与含ERE的DNA片段结合,这表明其他蛋白质可能在ER与ERE的相互作用中起重要作用。当DNA片段中存在两个ERE时,观察到弯曲有小但可重复的增加。我们证明hER与ERE的结合诱导DNA弯曲,这表明DNA弯曲在ER诱导的转录激活中可能起作用。

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