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差异的富马酸结合到拟南芥 NAD+-苹果酸酶 1 和 -2 上,产生相反的活性调节。

Differential fumarate binding to Arabidopsis NAD+-malic enzymes 1 and -2 produces an opposite activity modulation.

机构信息

Centro de Estudios Fotosintéticos y Bioquímicos, Universidad Nacional de Rosario, Suipacha 531, Rosario 2000, Argentina.

出版信息

Biochimie. 2012 Jun;94(6):1421-30. doi: 10.1016/j.biochi.2012.03.017. Epub 2012 Apr 2.

DOI:10.1016/j.biochi.2012.03.017
PMID:22487558
Abstract

Arabidopsis mitochondria contain two NAD(+)-malic enzymes, NAD-ME1 and NAD-ME2. These proteins have similar affinity for their substrates but display opposite regulation by fumarate, which strongly stimulates NAD-ME1 but inhibits NAD-ME2 activity. Here, the interaction of NAD-ME1 and -2 with fumarate was investigated by kinetic approaches, urea denaturation assays and intrinsic fluorescence quenching, in the absence and presence of NAD(+). Fumarate inhibited NAD-ME2 at saturating, but not at low, levels of NAD(+), and it behaved as competitive inhibitor with respect to L-malate. In contrast, NAD-ME1 fumarate activation was higher at suboptimal NAD(+) concentrations. In the absence of cofactor, the fluorescence of both NAD-ME1 and -2 is quenched by fumarate. However, for NAD-ME2 the quenching arises from a collisional phenomenon, while in NAD-ME1 the fluorescence decay can be explained by a static process that involves fumarate binding to the protein. Furthermore, the residue Arg84 of NAD-ME1 is essential for fumarate binding, as the mutant protein R84A exhibits a collisional quenching by this metabolite. Together, the results indicate that the differential fumarate regulation of Arabidopsis NAD-MEs, which is further modulated by NAD(+) availability, is related to the gaining of an allosteric site for fumarate in NAD-ME1 and an active site-associated inhibition by this C(4)-organic acid in NAD-ME2.

摘要

拟南芥线粒体含有两种 NAD(+)苹果酸酶,NAD-ME1 和 NAD-ME2。这两种蛋白对其底物具有相似的亲和力,但受到富马酸盐的相反调节,富马酸盐强烈刺激 NAD-ME1,但抑制 NAD-ME2 活性。在这里,通过动力学方法、尿素变性测定和内源荧光猝灭研究了 NAD-ME1 和 -2 与富马酸盐的相互作用,在不存在和存在 NAD(+)的情况下进行。富马酸盐在饱和但不在低 NAD(+)水平下抑制 NAD-ME2,并且对 L-苹果酸表现为竞争性抑制剂。相比之下,在亚最优 NAD(+)浓度下,NAD-ME1 的富马酸盐激活更高。在没有辅因子的情况下,NAD-ME1 和 -2 的荧光都被富马酸盐猝灭。然而,对于 NAD-ME2,猝灭源于碰撞现象,而对于 NAD-ME1,荧光衰减可以通过涉及富马酸盐与蛋白质结合的静态过程来解释。此外,NAD-ME1 的残基 Arg84 对于富马酸盐结合是必需的,因为突变蛋白 R84A 表现出这种代谢物的碰撞猝灭。总之,结果表明,拟南芥 NAD-MEs 的富马酸盐差异调节,进一步受到 NAD(+)可用性的调节,与 NAD-ME1 中获得富马酸盐的变构位点以及 NAD-ME2 中与活性位点相关的抑制有关。

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