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植物核糖激酶的鉴定及拟南芥核糖激酶在核苷代谢中的作用发现。

Identification of the Plant Ribokinase and Discovery of a Role for Arabidopsis Ribokinase in Nucleoside Metabolism.

作者信息

Riggs John W, Rockwell Nathan C, Cavales Philip C, Callis Judy

机构信息

From the Department of Molecular and Cellular Biology, University of California, Davis, California 95616.

From the Department of Molecular and Cellular Biology, University of California, Davis, California 95616

出版信息

J Biol Chem. 2016 Oct 21;291(43):22572-22582. doi: 10.1074/jbc.M116.754689. Epub 2016 Sep 6.

Abstract

Ribose can be used for energy or as a component of several important biomolecules, but for it to be used in either capacity it must first be phosphorylated by ribokinase (RBSK). RBSK proteins are part of the phosphofructokinase-B (pfkB) family of carbohydrate kinases. Sequence comparisons of pfkB proteins from the model plant Arabidopsis thaliana with the human and Escherichia coli RBSK identified a single candidate RBSK, At1g17160 (AtRBSK). AtRBSK is more similar to predicted RBSKs from other plant species and known mammalian and prokaryotic RBSK than to all other PfkB proteins in Arabidopsis AtRBSK contains a predicted chloroplast transit peptide, and we confirmed plastid localization using AtRBSK fused to YFP. Structure prediction software verified that the AtRBSK sequence mapped onto a known RBSK structure. Kinetic parameters of purified recombinant AtRBSK were determined to be K = 150 μm ± 17 μm, K = 45 μm ± 5.6 μm, and k = 2.0 s Substrate inhibition was observed for AtRBSK (K = 2.44 mm ± 0.36 mm), as has been demonstrated for other RBSK proteins. Ribose accumulated in Arabidopsis plants lacking AtRBSK. Such plants grew normally unless media was supplemented with ribose, which led to chlorosis and growth inhibition. Both chlorosis and ribose accumulation were abolished upon the introduction of a transgene expressing AtRBSK-MYC, demonstrating that the loss of protein is responsible for ribose hypersensitivity. Ribose accumulation in plants lacking AtRBSK was reduced in plants also deficient in the nucleoside ribohydrolase NSH1, linking AtRBSK activity to nucleoside metabolism.

摘要

核糖可用于提供能量或作为几种重要生物分子的组成部分,但要以任何一种方式被利用,它都必须首先被核糖激酶(RBSK)磷酸化。RBSK蛋白是碳水化合物激酶磷酸果糖激酶-B(pfkB)家族的一部分。对模式植物拟南芥的pfkB蛋白与人类和大肠杆菌的RBSK进行序列比较,确定了一个候选RBSK,即At1g17160(AtRBSK)。与拟南芥中的所有其他PfkB蛋白相比,AtRBSK与其他植物物种以及已知的哺乳动物和原核RBSK的预测RBSK更为相似。AtRBSK包含一个预测的叶绿体转运肽,我们通过将AtRBSK与黄色荧光蛋白(YFP)融合证实了其质体定位。结构预测软件验证了AtRBSK序列与已知的RBSK结构相匹配。纯化的重组AtRBSK的动力学参数确定为:Km = 150 μM ± 17 μM,Kd = 45 μM ± 5.6 μM,kcat = 2.0 s-1。观察到AtRBSK存在底物抑制现象(Ki = 2.44 mM ± 0.36 mM),其他RBSK蛋白也有此现象。在缺乏AtRBSK的拟南芥植株中核糖积累。除非培养基中添加核糖,否则这些植株正常生长,添加核糖会导致黄化和生长抑制。引入表达AtRBSK-MYC的转基因后,黄化和核糖积累现象均消失,表明该蛋白的缺失导致了核糖超敏反应。在同时缺乏核苷核糖水解酶NSH1的植株中,缺乏AtRBSK的植株中的核糖积累减少,这将AtRBSK的活性与核苷代谢联系起来。

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