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Alu元件来源的侧翼序列通过与序列特异性转录因子相互作用,在体外刺激转录。

Flanking sequences of an Alu source stimulate transcription in vitro by interacting with sequence-specific transcription factors.

作者信息

Chesnokov I, Schmid C W

机构信息

Section of Molecular and Cellular Biology, University of California, Davis 95616, USA.

出版信息

J Mol Evol. 1996 Jan;42(1):30-6. doi: 10.1007/BF00163208.

Abstract

An Alu source gene, called the EPL Alu, was previously isolated by a phylogenetic strategy. Sequences flanking the EPL Alu family member stimulate its RNA polymerase III (Pol III) template activity in vitro. One cis-acting element maps within a 40-nucleotide region immediately upstream to the EPL Alu. This same region contains an Ap1 site which, when mutated, abolishes the transcriptional stimulation provided by this region. The flanking sequence, as assayed by gel mobility shift, forms sequence-specific complexes with several nuclear factors including Ap1. These results demonstrate that an an ancestral Alu source sequence fortuitously acquired positive transcriptional control elements by insertion into the EPL locus, thereby providing biochemical evidence for a model which explains the selective amplification of Alu subfamilies.

摘要

一个名为EPL Alu的Alu源基因先前是通过系统发育策略分离出来的。EPL Alu家族成员侧翼的序列在体外刺激其RNA聚合酶III(Pol III)模板活性。一个顺式作用元件定位于EPL Alu上游紧邻的40个核苷酸区域内。同一区域包含一个Ap1位点,该位点发生突变时,会消除该区域提供的转录刺激。通过凝胶迁移率变动分析检测的侧翼序列与包括Ap1在内的几种核因子形成序列特异性复合物。这些结果表明,一个祖先Alu源序列通过插入EPL基因座偶然获得了正转录控制元件,从而为解释Alu亚家族选择性扩增的模型提供了生化证据。

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