糖原磷酸化酶1在盘状盘齿龙发育和camp介导的调控。

J F Sucic, S Luo, B D Williamson, Y Yin, P V Rogers, C L Rutherford
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引用次数: 2

摘要

盘状盘齿盘骨糖原磷酸化酶-1 (gp-1)表现出复杂的发育表达模式,在这种模式中,酶活性、蛋白水平和mRNA水平受到不同时间的调节。这种表达模式表明gp-1调控发生在多个水平,可能涉及转录和转录后事件。翻译后对gp-1活性的控制,实际上从发育的角度调控了蛋白质。在本报告中,我们研究了这一规定的几个方面。我们发现,在悬浮培养的细胞中添加外源cAMP会引起gp-1酶活性和mRNA水平的变化,这些变化与正常发育过程中观察到的相同,这表明cAMP参与了gp-1的调节。外源cAMP可以在低至1.0 μ m的浓度下调节gp-1 mRNA的表达。cAMP对gp-1 mRNA的调控似乎是通过一种需要细胞内cAMP信号传导的机制发生的。我们通过使用gp-1启动子缺失来驱动荧光素酶报告基因的表达,确定了gp-1表达所必需的启动子区域。这些实验结果表明,发育和camp介导的gp-1 mRNA水平的变化是转录改变的结果。启动子分析还表明,植物特异性元件位于转录起始位点-785和-1894核苷酸之间。最大发育和camp介导表达所需的元件似乎位于帽位的-1153和-1894核苷酸之间。位于-180和-1153之间的序列元件似乎是发育后期基础水平表达所必需的。
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Developmental and cAMP-mediated regulation of glycogen phosphorylase 1 in Dictyostelium discoideum.

The Dictyostelium discoideum glycogen phosphorylase-1 (gp-1) exhibits a complex pattern of developmental expression in which differential temporal regulation of enzyme activity, protein levels and mRNA levels is observed. This pattern of expression implies that gp-1 regulation occurs at multiple levels, probably involving both transcriptional and post-transcriptional events. Post-translational control of gp-1 activity, in effect, actually regulates the protein from a developmental perspective. In this report we have examined several facets of this regulation. We show that addition of exogenous cAMP to cells in suspension culture caused changes in gp-1 enzyme activity and mRNA levels that are identical to those observed during normal development, suggesting that cAMP is involved in the regulation of gp-1. Exogenous cAMP could regulate gp-1 mRNA expression at concentrations as low as 1.0 microM. cAMP regulation of gp-1 mRNA appeared to occur through a mechanism that required intracellular cAMP signalling. We identified regions of the promoter necessary for gp-1 expression by using gp-1 promoter deletions to drive the expression of a luciferase reporter gene. Results of these experiments suggested that developmental and cAMP-mediated changes in gp-1 mRNA levels were the result of alterations in transcription. The promoter analysis also suggested that a vegetative specific element is located between -785 and -1894 nucleotides from the transcriptional start site. Elements necessary for maximal developmental and cAMP-mediated expression appear to be located between -1153 and -1894 nucleotides from the cap site. Sequence elements located between -180 and -1153 appear to be required for a basal level of late developmental expression.

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