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来自花椰菜花叶病毒19S启动子的转录及花椰菜花叶病毒RNA的翻译自催化作用。

Transcription from the CaMV 19 S promoter and autocatalysis of translation from CaMV RNA.

作者信息

Driesen M, Benito-Moreno R M, Hohn T, Fütterer J

机构信息

Friedrich Miescher Institute, Basel, Switzerland.

出版信息

Virology. 1993 Jul;195(1):203-10. doi: 10.1006/viro.1993.1361.

Abstract

The 19 S promoter of cauliflower mosaic virus was analyzed in host protoplasts. In spite of its weakness, it contains a fully functional core promoter. It can be strongly activated by 35 S enhancer elements, even when these elements are located downstream of it, comparable to the situation in the viral genome. The 19 S promoter also contains an element that can strongly enhance expression from a heterologous core promoter. A plasmid expressing the same CAT ORF from two overlapping transcription units, a dicistronic one under control of the 35 S promoter and a monocistronic one under control of the 19 S promoter, was constructed. While in the absence of the virus ORF VI product (pVI, "transactivator") only low levels of CAT activity deriving from the 19 S promoter were observed, in the presence of this protein high levels of CAT activity derived from the 35 S unit were observed in addition. This suggests autocatalytic activation of pVI expression during virus infection.

摘要

对花椰菜花叶病毒的19S启动子在宿主原生质体中进行了分析。尽管它较弱,但它含有一个功能完全正常的核心启动子。它可以被35S增强子元件强烈激活,即使这些元件位于其下游,这与病毒基因组中的情况类似。19S启动子还含有一个元件,该元件可以强烈增强来自异源核心启动子的表达。构建了一个质粒,该质粒从两个重叠的转录单元表达相同的CAT开放阅读框,一个是在35S启动子控制下的双顺反子转录单元,另一个是在19S启动子控制下的单顺反子转录单元。在没有病毒开放阅读框VI产物(pVI,“反式激活因子”)的情况下,仅观察到来自19S启动子的低水平CAT活性,而在有这种蛋白质存在的情况下,除了观察到来自35S单元的高水平CAT活性外,还观察到了来自19S启动子的高水平CAT活性。这表明在病毒感染期间pVI表达的自催化激活。

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