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甘氨酸脱羧酶复合体H蛋白的光依赖性和组织特异性表达。

Light-dependent and tissue-specific expression of the H-protein of the glycine decarboxylase complex.

作者信息

Srinivasan R, Oliver D J

机构信息

Department of Molecular Biology and Biochemistry, University of Idaho, Moscow 83843, USA.

出版信息

Plant Physiol. 1995 Sep;109(1):161-8. doi: 10.1104/pp.109.1.161.

Abstract

Glycine decarboxylase is a mitochondrial enzyme complex, which is the site of photorespiratory CO2 and NH3 release. Although the proteins that constitute the complex are located within the mitochondria, because of their intimate association with photosynthesis their expression is controlled by light. Comparisons of the kinetics of mRNA accumulation between the small subunit of ribulose-1,5-bisphosphate carboxylase/oxygenase and the H-protein of glycine decarboxylase during the greening of etiolated Arabidopsis thaliana suggest that their expression is controlled in parallel. A genomic clone for the H-protein (gdcH) was isolated from Arabidopsis and sequenced. The upstream region from -856 to +62 was fused to the beta-glucuronidase (GUS) reporter gene, and this construct was transformed into tobacco. This 5' upstream regulatory region appears to control GUS expression in a manner very similar to that of the endogenous H-protein gene. Constructs with deletions in the 5' upstream region were transformed into tobacco. These deletions revealed that light-dependent and tissue-specific expression was largely controlled by a 259-bp region between -376 and -117 bp. This region contains several putative GT boxes with the GGTTAA consensus core sequence. Once these strong light-dependent elements were removed, a second level of control was revealed. In constructs in which the gdcH 5' regulatory region was shortened to -117 bp or less, there was more GUS activity in the roots than in the leaves, and in dark-grown plants than in light-grown plants. This suggests that more proximal control elements may be responsible for the constitutive low levels of gene expression noted in all nonphotosynthetic tissues.

摘要

甘氨酸脱羧酶是一种线粒体酶复合体,是光呼吸过程中二氧化碳和氨释放的场所。尽管构成该复合体的蛋白质位于线粒体内,但由于它们与光合作用密切相关,其表达受光的控制。在黄化拟南芥变绿过程中,对1,5 - 二磷酸核酮糖羧化酶/加氧酶小亚基和甘氨酸脱羧酶H蛋白的mRNA积累动力学进行比较,结果表明它们的表达是平行控制的。从拟南芥中分离并测序了H蛋白(gdcH)的基因组克隆。将 - 856至 + 62的上游区域与β - 葡萄糖醛酸酶(GUS)报告基因融合,并将该构建体转化到烟草中。这个5'上游调控区域似乎以与内源性H蛋白基因非常相似的方式控制GUS表达。将5'上游区域有缺失的构建体转化到烟草中。这些缺失表明,光依赖性和组织特异性表达在很大程度上受 - 376至 - 117 bp之间的259 bp区域控制。该区域包含几个具有GGTTAA共有核心序列的推定GT框。一旦去除这些强光依赖性元件,就揭示了第二级控制。在gdcH 5'调控区域缩短至 - 117 bp或更短的构建体中,根部的GUS活性比叶片中高,在黑暗生长的植物中比在光照生长的植物中高。这表明更近端的控制元件可能负责所有非光合组织中观察到的基因组成型低水平表达。

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