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在缺乏功能性质体的情况下,细胞质激酶和磷酸酶活性可诱导PsaF基因表达:磷酸化/去磷酸化事件参与细胞器间串扰的证据

Cytoplasmic kinase and phosphatase activities can induce PsaF gene expression in the absence of functional plastids: evidence that phosphorylation/dephosphorylation events are involved in interorganellar crosstalk.

作者信息

Chandok M R, Sopory S K, Oelmüller R

机构信息

Institut für Allgemeine Botanik, Lehrstuhl für Pflanzenphysiologie der Friedrich-Schiller-Universität Jena, Germany.

出版信息

Mol Gen Genet. 2001 Feb;264(6):819-26. doi: 10.1007/s004380000371.

DOI:10.1007/s004380000371
PMID:11254129
Abstract

PsaF is a nuclear gene for subunit III of the reaction center of photosystem I, and its expression is stimulated by cytokinins and light, when monitored at the mRNA level or at the level of GUS activity directed by chimeric promoter::uidA gene fusions in transgenic tobacco. These inductive effects can be mimicked by pertussis toxin, serotonin, phorbol acetate myristate or Ca2+, suggesting the involvement of heterotrimeric G proteins, phospholipids and Ca2+-dependent processes. Both breakdown products of the phosphatidylinositol cycle, inositol triphosphate (IP3) and diacylglycerol (or its homolog phorbol myristate acetate, PMA) appear to be involved. The IP3-dependent pathway requires kinase activity, and the signal operates via a 42-bp Ca2+-responsive element located between positions -220 and -178, while the PMA-dependent pathway requires phosphatase activity and a binding element that lies further upstream in the promoter. The effects of G proteins, phospholipids and Ca2+ on GUS gene expression are restricted to tissues with functional plastids, while modulation of phosphatase and kinase activities activates the responsive PsaF promoter regions even in photobleached material. Thus, activation of kinases and phosphatases can bypass the plastid-mediated inhibition of PsaF gene expression in tobacco seedlings. One cytoplasmic target which reflects the functional state of the plastids is protein kinase C. The enzyme can be efficiently phosphorylated in protein extracts from seedlings in which plastid function is impaired, but not in extracts from green tissue.

摘要

PsaF是光系统I反应中心亚基III的一个核基因,当在转基因烟草中以mRNA水平或嵌合启动子::uidA基因融合所指导的GUS活性水平进行监测时,其表达受到细胞分裂素和光的刺激。百日咳毒素、血清素、佛波酯肉豆蔻酸酯或Ca2+可模拟这些诱导效应,表明异源三聚体G蛋白、磷脂和Ca2+依赖性过程参与其中。磷脂酰肌醇循环的两个分解产物,肌醇三磷酸(IP3)和二酰基甘油(或其同系物佛波肉豆蔻酸酯,PMA)似乎都参与其中。IP3依赖性途径需要激酶活性,信号通过位于-220至-178位之间的42bp Ca2+反应元件起作用,而PMA依赖性途径需要磷酸酶活性和位于启动子中更上游的一个结合元件。G蛋白、磷脂和Ca2+对GUS基因表达的影响仅限于具有功能质体的组织,而磷酸酶和激酶活性的调节即使在光漂白材料中也能激活反应性PsaF启动子区域。因此,激酶和磷酸酶的激活可以绕过烟草幼苗中质体介导的PsaF基因表达抑制。反映质体功能状态的一个细胞质靶点是蛋白激酶C。在质体功能受损的幼苗的蛋白提取物中,该酶可以被有效磷酸化,但在绿色组织的提取物中则不能。

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