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植物硫代谢工程中丝氨酸乙酰转移酶和半胱氨酸合酶的分子与生化分析

Molecular and biochemical analysis of serine acetyltransferase and cysteine synthase towards sulfur metabolic engineering in plants.

作者信息

Noji M, Saito K

机构信息

Department of Molecular Biology and Biotechnology, Graduate School of Pharmaceutical Sciences, Chiba University, Japan.

出版信息

Amino Acids. 2002;22(3):231-43. doi: 10.1007/s007260200011.

Abstract

Serine acetyltransferase (SATase) and cysteine synthase (O-acetylserine (thiol)-lyase) (CSase) are committed in the final step of cysteine biosynthesis. Six cDNA clones encoding SATase have been isolated from several plants, e.g. watermelon, spinach, Chinese chive and Arabidopsis thaliana. Feedback-inhibition pattern and subcellular localization of plant SATases were evaluated. Two types of SATase that differ in their sensitivity to the feedback inhibition by L-cysteine were found in plants. In Arabidopsis, cytosolic SATase was inhibited by L-cysteine at a physiological concentration in an allosteric manner, but the plastidic and mitochondrial forms were not subjected to this feedback regulation. These results suggest that the regulation of cysteine biosynthesis through feedback inhibition may differ depending on the subcellular compartment. The allosteric domain responsible for L-cysteine inhibition was characterized, using several SATase mutants. The single change of amino acid residue, glycine-277 to cysteine, in the C-terminal region of watermelon SATase caused a significant decrease of the feedback-inhibition sensitivity of watermelon SATase. We made the transgenic Arabidopsis overexpressing point-mutated watermelon SATase gene whose product was not inhibited by L-cysteine. The contents of OAS, cysteine, and glutathione in transgenic Arabidopsis were significantly increased as compared to the wild-type Arabidopsis. Transgenic tobacco (Nicotiana tabacum) (F1) plants with enhanced CSase activities both in the cytosol and in the chloroplasts were generated by cross-fertilization of two transgenic tobacco expressing either cytosolic CSase or chloroplastic CSase. Upon fumigation with 0.1 microLL(-1) sulfur dioxide, both the cysteine and glutathione contents in leaves of F1 plants were increased significantly, but not in leaves of non-transformed control plants. These results indicated that both SATase and CSase play important roles in cysteine biosynthesis and its regulation in plants.

摘要

丝氨酸乙酰转移酶(SATase)和半胱氨酸合酶(O-乙酰丝氨酸(硫醇)裂解酶)(CSase)参与半胱氨酸生物合成的最后一步。已经从几种植物中分离出六个编码SATase的cDNA克隆,例如西瓜、菠菜、韭菜和拟南芥。对植物SATase的反馈抑制模式和亚细胞定位进行了评估。在植物中发现了两种对L-半胱氨酸反馈抑制敏感性不同的SATase。在拟南芥中,胞质SATase在生理浓度下被L-半胱氨酸以变构方式抑制,但质体和线粒体形式不受这种反馈调节。这些结果表明,通过反馈抑制对半胱氨酸生物合成的调节可能因亚细胞区室而异。使用几种SATase突变体对负责L-半胱氨酸抑制的变构结构域进行了表征。西瓜SATase C末端区域的氨基酸残基甘氨酸-277单突变为半胱氨酸,导致西瓜SATase的反馈抑制敏感性显著降低。我们构建了过表达点突变西瓜SATase基因的转基因拟南芥,其产物不受L-半胱氨酸抑制。与野生型拟南芥相比,转基因拟南芥中OAS、半胱氨酸和谷胱甘肽的含量显著增加。通过将两种分别表达胞质CSase或叶绿体CSase的转基因烟草杂交,培育出了胞质和叶绿体中CSase活性均增强的转基因烟草(烟草)(F1)植株。用0.1 μL L⁻¹二氧化硫熏蒸后,F1植株叶片中的半胱氨酸和谷胱甘肽含量均显著增加,但未转化的对照植株叶片中未增加。这些结果表明,SATase和CSase在植物半胱氨酸生物合成及其调节中均起重要作用。

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