首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Analysis of clustered point mutations in the human ribosomal RNA gene promoter by transient expression in vivo.
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Analysis of clustered point mutations in the human ribosomal RNA gene promoter by transient expression in vivo.

机译:通过体内瞬时表达分析人核糖体RNA基因启动子中的聚集点突变。

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摘要

We have mapped the cis regulatory elements required in vivo for initiation at the human rRNA promoter by RNA polymerase I. Transient expression in COS-7 cells was used to evaluate the transcription phenotype of clustered base substitution mutations in the human rRNA promoter. The promoter consists of two major elements: a large upstream region, composed of several domains, that lies between nucleotides -234 and -107 relative to the transcription initiation site and affects transcription up to 100-fold and a core element that lies between nucleotides -45 and +20 and affects transcription up to 1000-fold. The upstream region is able to retain partial function when positioned within 100-160 nucleotides of the transcription initiation site, but it cannot stimulate transcription from distances of greater than or equal to 600 nucleotides. In addition, we demonstrate, using mouse-human hybrid rRNA promoters, that the sequences responsible for human species-specific transcription in vivo appear to reside in both the core and upstream elements, and sequences from the mouse rRNA promoter cannot be substituted for them.
机译:我们已经绘制了通过RNA聚合酶I在人rRNA启动子上体内启动所需的体内顺式调控元件。在COS-7细胞中的瞬时表达用于评估人rRNA启动子中簇状碱基取代突变的转录表型。启动子由两个主要元件组成:一个较大的上游区域,由多个结构域组成,相对于转录起始位点位于核苷酸-234和-107之间,并影响转录达100倍;而核心元件位于核苷酸之间- 45和+20,影响转录达1000倍。当位于转录起始位点的100-160个核苷酸内时,上游区域能够保留部分功能,但是它不能从大于或等于600个核苷酸的距离刺激转录。此外,我们证明,使用小鼠-人类杂种rRNA启动子,负责人类物种特异性体内转录的序列似乎驻留在核心和上游元件中,并且不能用小鼠rRNA启动子的序列替代它们。

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