首页> 外文OA文献 >Controlled expression of plastid transgenes in plants based on a nuclear DNA-encoded and plastid-targeted T7 RNA polymerase.
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Controlled expression of plastid transgenes in plants based on a nuclear DNA-encoded and plastid-targeted T7 RNA polymerase.

机译:基于核DNA编码和针对质体的T7 RNA聚合酶控制植物中质体转基因的表达。

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摘要

Phage T7 RNA polymerase has been used extensively in Escherichia coli for high-level expression of selected genes placed under the control of the phage T7 gene 10 promoter. We have constructed an analogous system for use in plastids of higher plants. A T7 RNA polymerase chimeric gene containing a cauliflower mosaic virus 35S promoter and a tobacco ribulose-bisphosphate carboxylase/oxygenase small-subunit chloroplast transit-peptide sequence was introduced into tobacco by nuclear transformation. Stable plastid transformation of tobacco expressing the T7 RNA polymerase activity with a T7 promoter/beta-glucuronidase (GUS) reporter gene construct resulted in expression of GUS mRNA and enzyme activity in all tissues examined. Expression of GUS activity was extremely high in mature leaves, moderate in young leaves and petals, and low in stems, roots, and developing seeds. Plastid transformation of wild-type tobacco with the same chimeric GUS gene resulted in undetectable levels of GUS mRNA and enzyme activity. Genetic crosses demonstrated that a silent T7/GUS reporter gene could be activated in the F1 generation by transmission of an active nuclear T7 RNA polymerase gene from the male parent.
机译:噬菌体T7 RNA聚合酶已在大肠杆菌中广泛使用,用于高表达在噬菌体T7基因10启动子控制下的选定基因。我们已经构建了用于高等植物质体的类似系统。通过核转化将包含花椰菜花叶病毒35S启动子和烟草核糖二磷酸羧化酶/加氧酶小亚基叶绿体转运肽序列的T7 RNA聚合酶嵌合基因引入烟草。用T7启动子/β-葡糖醛酸糖苷酶(GUS)报告基因构建表达T7 RNA聚合酶活性的烟草的稳定质体转化,导致在所有检查的组织中表达GUS mRNA和酶活性。 GUS活性的表达在成熟叶片中极高,在幼叶和花瓣中适中,而在茎,根和发育中的种子中极低。具有相同嵌合GUS基因的野生型烟草的质体转化导致无法检测到的GUS mRNA水平和酶活性。遗传杂交表明,沉默的T7 / GUS报告基因可以通过从雄性亲本传来的活性核T7 RNA聚合酶基因在F1代中被激活。

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