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绿眼虫(Euglena gracilis)中具有双功能乙醛酸循环酶特性的苹果酸合酶/异柠檬酸裂解酶的鉴定。

Characterization of a bifunctional glyoxylate cycle enzyme, malate synthase/isocitrate lyase, of Euglena gracilis.

机构信息

Department of Applied Biological Chemistry, School of Life and Environmental Sciences, Osaka Prefecture University, Naka-ku, Sakai, Osaka, Japan.

出版信息

J Eukaryot Microbiol. 2011 Mar-Apr;58(2):128-33. doi: 10.1111/j.1550-7408.2011.00534.x. Epub 2011 Feb 18.

DOI:10.1111/j.1550-7408.2011.00534.x
PMID:21332878
Abstract

The glyoxylate cycle is a modified form of the tricarboxylic acid cycle, which enables organisms to synthesize carbohydrates from C2 compounds. In the protozoan Euglena gracilis, the key enzyme activities of the glyoxylate cycle, isocitrate lyase (ICL) and malate synthase (MS), are conferred by a single bifunctional protein named glyoxylate cycle enzyme (Euglena gracilis glyoxylate cycle enzyme [EgGCE]). We analyzed the enzymatic properties of recombinant EgGCE to determine the functions of its different domains. The 62-kDa N-terminal domain of EgGCE was sufficient to provide the MS activity as expected from an analysis of the deduced amino acid sequence. In contrast, expression of the 67-kDa C-terminal domain of EgGCE failed to yield ICL activity even though this domain was structurally similar to ICL family enzymes. Analyses of truncation mutants suggested that the N-terminal residues of EgGCE are critical for both the ICL and MS activities. The ICL activity of EgGCE increased in the presence of micro-molar concentrations of acetyl-coenzyme A (CoA). Acetyl-CoA also increased the activity in a mutant type EgGCE with a mutation at the acetyl-CoA binding site in the MS domain of EgGCE. This suggests that acetyl-CoA regulates the ICL reaction by binding to a site other than the catalytic center of the MS reaction.

摘要

乙醛酸循环是三羧酸循环的一种修饰形式,它使生物能够从 C2 化合物合成碳水化合物。在原生动物眼虫中,乙醛酸循环的关键酶活性,异柠檬酸裂解酶(ICL)和苹果酸合酶(MS),由一种称为乙醛酸循环酶的单一双功能蛋白赋予(眼虫属乙醛酸循环酶[Euglena gracilis glyoxylate cycle enzyme [EgGCE])。我们分析了重组 EgGCE 的酶学特性,以确定其不同结构域的功能。EgGCE 的 62kDa N 端结构域足以提供 MS 活性,这与从推导的氨基酸序列分析一致。相比之下,即使该结构域在结构上与 ICL 家族酶相似,表达 67kDa C 端结构域的 EgGCE 未能产生 ICL 活性。截断突变体的分析表明,EgGCE 的 N 端残基对于 ICL 和 MS 活性都是至关重要的。在微摩尔浓度的乙酰辅酶 A(CoA)存在下,EgGCE 的 ICL 活性增加。乙酰 CoA 还增加了在 EgGCE 的 MS 结构域中乙酰 CoA 结合位点突变的突变型 EgGCE 中的活性。这表明乙酰 CoA 通过与 MS 反应的催化中心以外的位点结合来调节 ICL 反应。

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