与萝卜rDNA启动子上游的富含dA/ dt序列结合的核蛋白片段[更正]。

M. Echeverria, D. Delcasso-Tremousaygue, M. Delseny
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引用次数: 25

摘要

rRNA核基因(rDNA)的外间隔段(ES)包含控制rDNA转录起始和增强的序列。ES在大多数物种中也以存在多个重复元素为特征。在高等植物中,关于控制rDNA转录的顺式和反式元件的资料很少。电泳迁移率转移试验(EMSA)表明,幼萝卜叶的核提取物(NER)含有与萝卜ES中特定序列结合的蛋白质片段。dna酶I足迹分析可以将NER蛋白与dA/dT均聚物延伸和13-bp的富含dA/dT的短重复序列结合,在7个大约100 bp的重复区域(位于转录起始位点-1077至-740)和包含rDNA转录起始启动子的区域(-120至-55)中发现。目前尚不清楚这种ES结合是由于一种还是几种不同的蛋白质。到目前为止,与植物rDNA ES富含dA/ dt区域结合的蛋白质尚未被描述。它是一种特异的RNA聚合酶I转录因子,还是在基因组表达中发挥更普遍的作用仍有待阐明。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
A nuclear protein fraction binding to dA/dT-rich sequences upstream from the radish rDNA promoter [corrected].
The external spacer (ES) of rRNA nuclear genes (rDNA) contains the sequences that control rDNA transcription initiation and enhancement. The ES is also characterized in most species by the presence of multiple repeated elements. In higher plants very few data are available on the cis- and trans-acting elements which control rDNA transcription. Using electrophoretic mobility shift assays (EMSA) it is shown that nuclear extracts from young radish leaves (NER) contain a protein fraction which binds to specific sequences in the radish ES. DNase I footprinting analysis allows mapping of the NER protein binding to dA/dT homopolymer stretches and to a 13-bp dA/dT-rich short repeat, found both in the seven approximately 100 bp repeat regions (located -1077 to -740 from transcription initiation site) and the region (-120 to -55) containing the putative promoter for rDNA transcription initiation. Whether this ES binding is due to a single or several different proteins is not known. So far, protein(s) binding to dA/dT-rich regions of a plant rDNA ES has not yet been described. Whether it is a specific RNA polymerase I transcription factor(s) or plays a more general role in genome expression remains to be elucidated.
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