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一个水稻cab基因启动子包含调控双子叶植物和单子叶植物中表达的独立顺式作用元件。

A rice cab gene promoter contains separate cis-acting elements that regulate expression in dicot and monocot plants.

作者信息

Luan S, Bogorad L

机构信息

Department of Cellular and Developmental Biology, Harvard University, Cambridge, Massachusetts 02138.

出版信息

Plant Cell. 1992 Aug;4(8):971-81. doi: 10.1105/tpc.4.8.971.

Abstract

The major light-harvesting chlorophyll a/b binding proteins of the photosynthetic apparatus are encoded by families of nuclear cab genes. The expression of most cab genes is tissue specific and photoregulated in angiosperms. In transgenic tobacco plants, expression of the reporter gene beta-glucuronidase (GUS) is photoregulated and tissue specific from 5' upstream sequences of the rice cab1R gene; deletion of sequences upstream from position -170 with respect to the transcription start site eliminates the enhanced and photoregulated expression in the transgenic plants. Using an in situ transient expression assay, we have determined that the sequence OCT-R, an octamer repeat that lies within the -269 to -170 region of cab1R, is essential for photoregulated expression of the chimeric GUS gene in leaf cells of maize and rice but is not required for expression in illuminated tobacco leaves. Conversely, box III*- and G-box-like sequences found near OCT-R in cab1R are necessary for high-level transient expression of the reporter gene in tobacco leaf tissue but are not required for transient expression in maize or rice leaves.

摘要

光合机构的主要捕光叶绿素a/b结合蛋白由核cab基因家族编码。在被子植物中,大多数cab基因的表达具有组织特异性且受光调节。在转基因烟草植株中,报告基因β-葡萄糖醛酸酶(GUS)的表达受光调节且具有组织特异性,其来源于水稻cab1R基因的5'上游序列;相对于转录起始位点,缺失-170位上游的序列会消除转基因植株中增强的和受光调节的表达。通过原位瞬时表达分析,我们已经确定,位于cab1R基因-269至-170区域内的八聚体重复序列OCT-R,对于玉米和水稻叶细胞中嵌合GUS基因的光调节表达至关重要,但对于在光照下的烟草叶片中的表达并非必需。相反,在cab1R基因中靠近OCT-R发现的box III *和类G-box序列,对于报告基因在烟草叶组织中的高水平瞬时表达是必需的,但对于在玉米或水稻叶片中的瞬时表达并非必需。

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