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Glycerate kinase of the hyperthermophilic archaeon Thermoproteus tenax: new insights into the phylogenetic distribution and physiological role of members of the three different glycerate kinase classes

机译:嗜热古菌Thermoproteus tenax的甘油酸激酶:对三种不同甘油酸激酶类别成员的系统发育分布和生理作用的新见解

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Background The presence of the branched Entner-Doudoroff (ED) pathway in two hyperthermophilic Crenarchaea, the anaerobe Thermoproteus tenax and the aerobe Sulfolobus solfataricus, was suggested. However, so far no enzymatic information of the non-phosphorylative ED branch and especially its key enzyme – glycerate kinase – was available. In the T. tenax genome, a gene homolog with similarity to putative hydroxypyruvate reductase/glycerate dehydrogenase and glycerate kinase was identified. Results The encoding gene was expressed in E. coli in a recombinant form, the gene product purified and the glycerate kinase activity was confirmed by enzymatic studies. The enzyme was active as a monomer and catalyzed the ATP-dependent phosphorylation of D-glycerate forming exclusively 2-phosphoglycerate. The enzyme was specific for glycerate and highest activity was observed with ATP as phosphoryl donor and Mg2+ as divalent cation. ATP could be partially replaced by GTP, CTP, TTP and UTP. The enzyme showed high affinity for D-glycerate (Km 0.02 ± 0.01 mM, Vmax of 5.05 ± 0.52 U/mg protein) as well as ATP (Km of 0.03 ± 0.01 mM, Vmax of 4.41 ± 0.04 U/mg protein), although at higher glycerate concentrations, substrate inhibition was observed. Furthermore, the enzyme was inhibited by its product ADP via competitive inhibition. Data bank searches revealed that archaeal glycerate kinases are members of the MOFRL (multi-organism fragment with rich leucine) family, and homologs are found in all three domains of life. Conclusion A re-evaluation of available genome sequence information as well as biochemical and phylogenetic studies revealed the presence of the branched ED pathway as common route for sugar degradation in Archaea that utilize the ED pathway. Detailed analyses including phylogenetic studies demonstrate the presence of three distinct glycerate kinase classes in extant organisms that share no common origin. The affiliation of characterized glycerate kinases with the different enzyme classes as well as their physiological/cellular function reveals no association with particular pathways but a separate phylogenetic distribution. This work highlights the diversity and complexity of the central carbohydrate metabolism. The data also support a key function of the conversion of glycerate to 2- or 3-phosphoglycerate via glycerate kinase in funneling various substrates into the common EMP pathway for catabolic and anabolic purposes.
机译:背景建议在两个超嗜热克氏藻,即厌氧嗜热变形菌tenax和厌氧厌氧硫杆菌中存在分支的Entner-Doudoroff(ED)途径。但是,到目前为止,尚无有关非磷酸化ED分支的酶信息,尤其是其关键酶甘油酸激酶。在T. tenax基因组中,鉴定出与推定的羟基丙酮酸还原酶/甘油酸脱氢酶和甘油酸激酶相似的基因同源物。结果该编码基因在大肠杆菌中以重组形式表达,纯化了该基因产物,并通过酶学研究证实了甘油酸激酶活性。该酶作为单体具有活性,并催化D-甘油酸酯的ATP依赖性磷酸化,仅形成2-磷酸甘油酸酯。该酶对甘油酸酯具有特异性,在以ATP为磷酰基供体和以Mg 2+ 为二价阳离子的情况下观察到最高的活性。 ATP可以部分替换为GTP,CTP,TTP和UTP。该酶对D-甘油酸(K m 0.02±0.01 mM,V max 为5.05±0.52 U / mg蛋白)和ATP(K m 为0.03±0.01 mM,V max 为4.41±0.04 U / mg蛋白),尽管在较高甘油酸浓度下,仍观察到底物抑制作用。此外,通过竞争性抑制,酶被其产物ADP抑制。资料库搜索显示,古细菌甘油酸激酶是MOFRL(富含亮氨酸的多生物片段)家族的成员,并且在生活的所有三个域中都发现了同源物。结论对现有基因组序列信息的重新评估以及生化和系统发育研究表明,存在分支ED途径是利用ED途径在古细菌中糖降解的常见途径。包括系统发育研究在内的详细分析表明,在没有共同起源的现存生物中存在三种不同的甘油酸激酶类别。表征的甘油酸酯激酶与不同酶类别的结合以及它们的生理/细胞功能显示与特定途径没有关联,但揭示了独立​​的系统发生分布。这项工作突出了中央碳水化合物代谢的多样性和复杂性。数据还支持在通过分解代谢和合成代谢目的将各种底物集中到常见EMP途径中时,通过甘油酸激酶将甘油酸酯转化为2-或3-磷酸甘油酸酯的关键功能。

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