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A conserved core element is functionally important for maize mitochondrial promoter activity in vitro.

机译:保守的核心元件对于玉米体外线粒体启动子活性在功能上很重要。

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摘要

We have previously used a homologous in vitro transcription system to define functional elements of the maize mitochondrial atpA promoter. These elements comprise a central domain extending from -7 to +5, relative to the transcription start site, and an upstream domain of 1-3 bp that is purine rich and centered around positions -11 to -12. Within the central domain lies an essential 5 bp core element. These elements are conserved in many mitochondrial promoters, but their functionality has only been tested for atpA. In this study we have introduced mutations into the corresponding elements of two cox3 promoters and show that while the core element is essential for cox3 promoter activity, upstream element mutations have little or no effect. To define the minimal sequence required for in vitro promoter activity a series of short cloned oligonucleotides corresponding to the atpA promoter was used. While some activity was seen with a 14 bp sequence, full activity required 26 bp, suggesting that elements other than the core and upstream region can influence promoter strength. Another series of clones showed that altered spacing between the upstream and core elements of atpA had a significant effect on promoter activity. These results further define important features of the plant mitochondrial transcriptional machinery.
机译:我们以前已经使用了同源的体外转录系统来定义玉米线粒体atpA启动子的功能元件。这些元件包括相对于转录起始位点从-7延伸至+5的中央结构域和富含嘌呤且以位置-11至-12为中心的1-3 bp的上游结构域。在中央结构域内有一个必不可少的5 bp核心元件。这些元件在许多线粒体启动子中均是保守的,但其功能仅针对atpA进行过测试。在这项研究中,我们已经将突变引入了两个cox3启动子的相应元件中,并表明虽然核心元件对于cox3启动子的活性至关重要,但上游元件突变几乎没有影响。为了确定体外启动子活性所需的最小序列,使用了一系列对应于atpA启动子的短克隆寡核苷酸。虽然看到了一些具有14 bp序列的活性,但完整的活性需要26 bp,这表明除核心和上游区域外的其他元件均可影响启动​​子的强度。另一系列的克隆表明,atpA上游和核心元件之间间隔的改变对启动子活性有重大影响。这些结果进一步定义了植物线粒体转录机制的重要特征。

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  • 作者

    Caoile, A G; Stern, D B;

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  • 年度 1997
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  • 原文格式 PDF
  • 正文语种 en
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