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离子对牛肾纯化的S-腺苷同型半胱氨酸水解酶的腺苷结合及酶活性的影响。

Effects of ions on adenosine binding and enzyme activity of purified S-adenosylhomocysteine hydrolase from bovine kidney.

作者信息

Kloor D, Fuchs S, Petroktistis F, Delabar U, Mühlbauer B, Quast U, Osswald H

机构信息

Department of Pharmacology, University of Tübingen, Germany.

出版信息

Biochem Pharmacol. 1998 Dec 1;56(11):1493-6. doi: 10.1016/s0006-2952(98)00250-0.

DOI:10.1016/s0006-2952(98)00250-0
PMID:9827583
Abstract

The present investigation was undertaken to determine the effect of various ions on the characteristics of S-adenosylhomocysteine (SAH) hydrolase from bovine kidney. The binding sites of [3H]-adenosine to purified SAH hydrolase were not influenced by phosphate, magnesium, potassium, sodium, chloride or calcium ions at physiological cytosolic concentrations. To test whether NAD+ in the SAH hydrolase is essential for adenosine binding, we prepared the apoenzyme by removing NAD+ with ammonium sulfate. The resulting apoenzyme did not exhibit any [3H]-adenosine binding. Since the apoenzyme was enzymatically inactive, it is suggested that adenosine binds to the active site and not to an allosteric site of the intact enzyme. The kinetics of the hydrolysis and the synthesis of SAH catalyzed by the enzyme SAH hydrolase were measured in the presence and absence of phosphate and magnesium. Phosphate increased the Vmax for both synthesis and hydrolysis. However, only the affinity of adenosine for SAH synthesis was significantly enhanced from 10.1+/-1.3 microM to 5.4+/-0.5 microM by phosphate. This effect was already maximal at a phosphate concentration of 1 mM. All other tested ions were without effect on the enzyme activity. Our results show that phosphate at physiological concentrations shifts the thermodynamic equilibrium of SAH hydrolase in the direction of SAH synthesis. These findings imply that SAH-sensitive transmethylation reactions are inhibited during renal hypoxia when intracellular levels of phosphate, adenosine, and SAH are elevated.

摘要

本研究旨在确定各种离子对牛肾S-腺苷同型半胱氨酸(SAH)水解酶特性的影响。在生理胞质浓度下,磷酸盐、镁、钾、钠、氯或钙离子对纯化的SAH水解酶与[3H]-腺苷的结合位点没有影响。为了测试SAH水解酶中的NAD+对腺苷结合是否至关重要,我们用硫酸铵去除NAD+制备了脱辅酶。所得脱辅酶未表现出任何[3H]-腺苷结合。由于脱辅酶无酶活性,表明腺苷结合到完整酶的活性位点而非变构位点。在有和没有磷酸盐及镁的情况下,测定了SAH水解酶催化SAH水解和合成的动力学。磷酸盐增加了合成和水解的Vmax。然而,只有腺苷对SAH合成的亲和力通过磷酸盐从10.1±1.3 microM显著提高到5.4±0.5 microM。在磷酸盐浓度为1 mM时,这种效应已达到最大值。所有其他测试离子对酶活性均无影响。我们的结果表明,生理浓度的磷酸盐使SAH水解酶的热力学平衡向SAH合成方向移动。这些发现意味着,当细胞内磷酸盐、腺苷和SAH水平升高时,在肾缺氧期间SAH敏感的转甲基反应受到抑制。

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