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Modulation, via Protein-Protein Interactions, of Glyceraldehyde-3-phosphate Dehydrogenase Activity through Redox Phosphoribulokinase Regulation

机译:通过蛋白质-蛋白质相互作用,通过氧化还原磷酸核糖激酶调节来调节3-磷酸甘油醛脱氢酶活性。

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摘要

The activity of glyceraldehyde-3-phosphate dehydrogenase (GAPDH) embedded in the phosphoribulokinase (PRK).GAPDH.CP12 complex was increased 2-3-fold by reducing agents. This occurred by interaction with PRK as the cysteinyl sulfhydryls (4 SH/subunit) of GAPDH within the complex were unchanged whatever the redox state of the complex. But isolated GAPDH was not activated. Alkylation plus mass spectrometry also showed that PRK had one disulfide bridge and three SH groups per monomer in the active oxidized complex. Reduction disrupted this disulfide bridge to give 2 more SH groups and a much more active enzyme. We assessed the kinetics and dynamics of the interactions between PRK and GAPDH/CP12 using biosensors to measure complex formation in real time. The apparent equilibrium binding constant for GAPDH/CP12 and PRK was 14 +/- 1.6 nm for oxidized PRK and 62 +/- 10 nm for reduced PRK. These interactions were neither pH- nor temperature-dependent. Thus, the dynamics of PRK.GAPDH.CP12 complex formation and GAPDH activity are modulated by the redox state of PRK.
机译:磷酸二氢激酶(PRK).GAPDH.CP12复合物中嵌入的甘油三磷酸三磷酸脱氢酶(GAPDH)的活性通过还原剂增加了2-3倍。这是通过与PRK相互作用而发生的,因为无论复合物的氧化还原状态如何,复合物中GAPDH的半胱氨酰巯基(4 SH /亚基)都没有改变。但是隔离的GAPDH未激活。烷基化加质谱分析还表明,PRK在活性氧化配合物中每个单体具有一个二硫键和三个SH基团。还原破坏了该二硫键,产生了另外两个SH基团和一个活性更高的酶。我们使用生物传感器实时测量复杂的形成,评估了PRK和GAPDH / CP12之间相互作用的动力学和动力学。 GAPDH / CP12和PRK的表观平衡结合常数对于氧化的PRK为14 +/- 1.6 nm,对于还原的PRK为62 +/- 10 nm。这些相互作用既不依赖pH,也不依赖温度。因此,PRK.GAPDH.CP12复合物形成的动力学和GAPDH活性受PRK的氧化还原状态调节。

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