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用二醛 - ADP对兔肌肉丙酮酸激酶进行亲和标记。

Affinity labeling of rabbit muscle pyruvate kinase with dialdehyde-ADP.

作者信息

Hinrichs M V, Eyzaguirre J

出版信息

Biochim Biophys Acta. 1982 Jun 4;704(2):177-85. doi: 10.1016/0167-4838(82)90144-3.

DOI:10.1016/0167-4838(82)90144-3
PMID:7104366
Abstract

Periodate-oxidized ADP (dialdehyde-ADP) inactivates rabbit muscle pyruvate kinase (ATP:pyruvate 2-O-phosphotransferase, EC 2.7.1.40) and combines irreversibly to the enzyme. This inactivation is first-order with respect to dialdehyde-ADP and follows saturation kinetics, indicating that the enzyme first forms a reversible complex with the inactivator. Low Mg2+ concentrations stimulate the rate of inactivation, while higher concentrations have a protective effect. ADP and ATP, especially in the presence of Mg2+, protect very strongly against inactivation, while phosphoenolpyruvate and pyruvate are less effective. Dialdehyde-ADP is not a substrate, but acts as competitive inhibitor of ADP, with a KI of 4.5 mM. The analog has somewhat lower affinity to the enzyme than Mg-ADP, which has a Kd of 1.2 mM. Based on kinetic data, it is shown that one molecule of reagent must combine per enzyme active site in order to inactivate the enzyme. Incorporation of [14-C]dialdehyde-ADP to the enzyme and treatment of the data by the Tsou plot shows that 6-7 residues per subunit react with the modifier, two of them being essential for activity. From the evidence presented it is concluded: (1) dialdehyde-ADP behaves as an affinity label of rabbit muscle pyruvate kinase; (2) the inactivator binds probably to lysine residues at or near the active site, forming morpholine-like structures, and (3) the enzyme possesses two modifiable groups essential for activity, the reaction of one of them being sufficient to cause total loss in activity.

摘要

高碘酸盐氧化的ADP(二醛 - ADP)可使兔肌肉丙酮酸激酶(ATP:丙酮酸2 - O - 磷酸转移酶,EC 2.7.1.40)失活,并与该酶不可逆结合。这种失活对于二醛 - ADP而言是一级反应,并遵循饱和动力学,表明该酶首先与失活剂形成可逆复合物。低浓度的Mg2 +刺激失活速率,而较高浓度则具有保护作用。ADP和ATP,特别是在Mg2 +存在的情况下,对失活具有很强的保护作用,而磷酸烯醇丙酮酸和丙酮酸的保护作用较弱。二醛 - ADP不是底物,而是作为ADP的竞争性抑制剂,其抑制常数KI为4.5 mM。该类似物对酶的亲和力略低于Mg - ADP,Mg - ADP的解离常数Kd为1.2 mM。基于动力学数据表明,为了使酶失活,每个酶活性位点必须结合一个试剂分子。将[14 - C]二醛 - ADP掺入酶中并通过邹氏图处理数据表明,每个亚基有6 - 7个残基与修饰剂反应,其中两个残基对活性至关重要。根据所提供的证据得出以下结论:(1)二醛 - ADP表现为兔肌肉丙酮酸激酶的亲和标记物;(2)失活剂可能与活性位点或其附近的赖氨酸残基结合,形成吗啉样结构;(3)该酶具有两个对活性至关重要的可修饰基团,其中一个基团的反应足以导致活性完全丧失。

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