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植物辅酶A生物合成:拟南芥中两种泛酸激酶的特性分析

Plant coenzyme A biosynthesis: characterization of two pantothenate kinases from Arabidopsis.

作者信息

Tilton G B, Wedemeyer W J, Browse J, Ohlrogge J

机构信息

Plant Biology Department, Michigan State University, East Lansing, MI 48824-6340, USA.

出版信息

Plant Mol Biol. 2006 Jul;61(4-5):629-42. doi: 10.1007/s11103-006-0037-4.

DOI:10.1007/s11103-006-0037-4
PMID:16897480
Abstract

In bacterial and animal coenzyme A (CoA) biosynthesis, pantothenate kinase (PANK) activity is critical in regulating intracellular CoA levels. Less is known about the role of PANK in plants, although a single plant isozyme from Arabidopsis, AtPANK1, was previously cloned and analyzed in vitro. We report here the characterization of a second pantothenate kinase of Arabidopsis, AtPANK2, as well as characterization of the physiological roles of both plant enzymes. The activity of the second pantothenate kinase, AtPANK2, was confirmed by its ability to complement the temperature-sensitive mutation of the bacterial pantothenate kinase in E. coli strain ts9. Knock-out mutation of either AtPANK1 or AtPANK2 did not inhibit plant growth, whereas pank1-1/pank2-1 double knockout mutations were embryo lethal. The phenotypes of the mutant plants demonstrated that only one of the AtPANK enzymes is necessary and sufficient for producing adequate CoA levels, and that no other enzyme can compensate for the loss of both isoforms. Real-time PCR measurements of AtPANK1 and AtPANK2 transcripts indicated that both enzymes are expressed with similar patterns in all tissues examined, further suggesting that AtPANK1 and AtPANK2 have complementary roles. The two enzymes have homologous pantothenate kinase domains, but AtPANK2 also carries a large C-terminal protein domain. Sequence comparisons indicate that this type of "bifunctional" pantothenate kinase is conserved in other higher eukaryotes as well. Although the function of the C-terminal domain is not known, homology structure modeling suggests it contains a highly conserved cluster of charged residues that likely constitute a metal-binding site.

摘要

在细菌和动物的辅酶A(CoA)生物合成过程中,泛酸激酶(PANK)活性对于调节细胞内CoA水平至关重要。尽管之前已克隆并在体外分析了来自拟南芥的单一植物同工酶AtPANK1,但关于PANK在植物中的作用了解较少。我们在此报告拟南芥的第二种泛酸激酶AtPANK2的特性,以及这两种植物酶的生理作用特性。通过其互补大肠杆菌菌株ts9中细菌泛酸激酶温度敏感突变的能力,证实了第二种泛酸激酶AtPANK2的活性。AtPANK1或AtPANK2的敲除突变均未抑制植物生长,而pank1-1/pank2-1双敲除突变则导致胚胎致死。突变植物的表型表明,仅一种AtPANK酶对于产生足够的CoA水平是必要且充分的,并且没有其他酶能够补偿两种同工型的缺失。对AtPANK1和AtPANK2转录本的实时PCR测量表明,这两种酶在所有检测的组织中表达模式相似,进一步表明AtPANK1和AtPANK2具有互补作用。这两种酶具有同源的泛酸激酶结构域,但AtPANK2还带有一个大的C末端蛋白结构域。序列比较表明,这种类型的“双功能”泛酸激酶在其他高等真核生物中也保守。尽管C末端结构域的功能尚不清楚,但同源结构建模表明它包含一个高度保守的带电残基簇,可能构成一个金属结合位点。

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