首页> 美国卫生研究院文献>Journal of Virology >Multiple widely spaced elements determine the efficiency with which a distal cistron is expressed from the polycistronic pregenomic RNA of figwort mosaic caulimovirus.
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Multiple widely spaced elements determine the efficiency with which a distal cistron is expressed from the polycistronic pregenomic RNA of figwort mosaic caulimovirus.

机译:多个宽间隔的元件决定了从玄参花椰菜花椰菜花叶病毒的多顺反子前基因组RNA表达远端顺反子的效率。

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摘要

The polycistronic expression mechanism of the plant pararetrovirus figwort mosaic caulimovirus (FMV) depends upon cis-acting elements present in its pregenomic RNA and a trans-acting protein (P6) which is expressed from a monocistronic subgenomic RNA. Using transient expression of FMV-derived polycistronic reporter constructs in Nicotiana edwardsonii cell suspension protoplasts, we further analyzed the cis-acting elements involved in polycistronic expression. A cis-acting element located within the first 74 nucleotides of the 7,954-nucleotide pregenomic RNA appears to be essential for P6 to transactivate expression of an internal cistron. Expression of this internal cistron, in the presence of P6, is greatly enhanced by the combined presence of two cis-acting elements located at the 3' end of the polycistronic RNA. Surprisingly, deletion of the most upstream of these two 3' cis-acting elements exposed a negative-acting element located internally on the polycistronic RNA, at the 3' end of open reading frame I. The action of both this negative-acting internal element and the positive-acting 3' elements is more pronounced when the large 5' untranslated leader region is present. This indicates that the 5' untranslated leader region is central to regulation of the FMV gene expression mechanism. Although a limited set of elements suffices to direct polycistronic expression in this eukaryotic system, a complex interplay between elements is involved in the spatial regulation of the genes present on the pregenomic RNA of FMV.
机译:植物副逆转录病毒小花叶花椰菜花椰菜病毒(FMV)的多顺反子表达机制取决于其前基因组RNA中存在的顺式作用元件和由单顺反子亚基因组RNA表达的反式作用蛋白(P6)。使用瞬时表达的FMV来源的多顺反子记者构建体在爱德华烟草细胞悬浮原生质体中,我们进一步分析了参与多顺反子表达的顺式作用元件。位于7954个核苷酸的前基因组RNA的前74个核苷酸内的顺式作用元件对于P6激活内部顺反子的表达似乎是必不可少的。在P6存在下,该内部顺反子的表达通过位于多顺反子RNA 3'端的两个顺式作用元件的结合存在而大大增强。令人惊讶的是,这两个3'顺式作用元件最上游的缺失暴露了位于开放阅读框I 3'端的多顺反子RNA内部的一个负作用元件。这两个负作用内部元件的作用当存在较大的5'非翻译前导区时,正作用的3'元件更为明显。这表明5'非翻译的前导区对于FMV基因表达机制的调节至关重要。尽管在这种真核系统中,有限的一组元素就足以指导多顺反子表达,但是,在FMV前基因组RNA上存在的基因的空间调节中涉及到元素之间的复杂相互作用。

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