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马铃薯双功能果糖-6-磷酸,2-激酶/果糖-2,6-二磷酸酶的克隆、特性分析及表达

Cloning, characterization and expression of a bifunctional fructose-6-phosphate, 2-kinase/fructose-2,6-bisphosphatase from potato.

作者信息

Draborg H, Villadsen D, Nielsen T H

机构信息

Dept. of Plant Biology, Royal Veterinary and Agricultural University, Frederiksberg, Denmark.

出版信息

Plant Mol Biol. 1999 Mar;39(4):709-20. doi: 10.1023/a:1006102412693.

DOI:10.1023/a:1006102412693
PMID:10350085
Abstract

We have isolated cDNA clones encoding the regulatory enzyme fructose-6-phosphate,2-kinase/fructose-2,6-bisphosphatase from a potato (Solanum tuberosum) leaf cDNA library. All clones represented transcripts of the same gene (F2KP1). Functionality of the encoded protein was verified by expression of the active enzyme in Escherichia coli. The expressed enzyme had both kinase activity which forms fructose-2,6-bisphosphate from fructose-6-phosphate and ATP, and phosphatase activity which degrade fructose-2,6-bisphosphate. The recombinant potato enzyme was radiolabelled by [2-32P]fructose-2,6-bisphosphate verifying conservation of the phosphatase catalytic mechanism which involves a phospho-protein intermediate. The deduced amino acid sequence corresponding to the catalytic core for F2KPI is homologous to the fructose-6-phosphate, 2-kinase/fructose-2,6-bisphosphatase isolated from animals and yeast, with conservation of amino acids involved in substrate binding and catalytic mechanisms. The sequence for F2KP1 also includes a 102 amino acids long NH2-terminal with no homology to any previously identified enzymes. This NH2 terminal may be even longer since an upstream stop codon has not yet been identified. Northern blot analysis of potato showed that the F2KP1 transcript is present in several tissues including source leaves, sink leaves and flowers, whereas the transcripts were not detectable in developing tubers. Southern blot analysis of Solanum phureja suggest there to be only one copy of the gene.

摘要

我们从马铃薯(Solanum tuberosum)叶片cDNA文库中分离出了编码调节酶果糖-6-磷酸,2-激酶/果糖-2,6-二磷酸酶的cDNA克隆。所有克隆均代表同一基因(F2KP1)的转录本。通过在大肠杆菌中表达活性酶来验证所编码蛋白质的功能。所表达的酶既具有从果糖-6-磷酸和ATP形成果糖-2,6-二磷酸的激酶活性,又具有降解果糖-2,6-二磷酸的磷酸酶活性。重组马铃薯酶被[2-32P]果糖-2,6-二磷酸放射性标记,证实了涉及磷蛋白中间体的磷酸酶催化机制的保守性。与F2KPI催化核心相对应的推导氨基酸序列与从动物和酵母中分离出的果糖-6-磷酸,2-激酶/果糖-2,6-二磷酸酶同源,底物结合和催化机制中涉及的氨基酸具有保守性。F2KP1的序列还包括一个102个氨基酸长的NH2末端,与任何先前鉴定的酶均无同源性。由于尚未鉴定到上游终止密码子,这个NH2末端可能更长。马铃薯的Northern印迹分析表明,F2KP1转录本存在于包括源叶、库叶和花在内的多个组织中,而在发育中的块茎中未检测到转录本。Solanum phureja的Southern印迹分析表明该基因只有一个拷贝。

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通过双功能酶6-磷酸果糖-2-激酶/果糖-2,6-二磷酸2-磷酸酶活性的差异变化,白骨壤叶片中的果糖-2,6-二磷酸含量在盐胁迫、水分胁迫和渗透胁迫下增加。
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