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Activation of Hydrogen Peroxide in Horseradish Peroxidase Occurs within ∼200 μs Observed by a New Freeze-Quench Device

机译:新型冷冻淬灭装置观察到辣根过氧化物酶中的过氧化氢活化在约200μs内发生。

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摘要

To observe the formation process of compound I in horseradish peroxidase (HRP), we developed a new freeze-quench device with ∼200 μs of the mixing-to-freezing time interval and observed the reaction between HRP and hydrogen peroxide (H2O2). The developed device consists of a submillisecond solution mixer and rotating copper or silver plates cooled at 77 K; it freezes the small droplets of mixed solution on the surface of the rotating plates. The ultraviolet-visible spectra of the sample quenched at ∼1 ms after the mixing of HRP and H2O2 suggest the formation of compound I. The electron paramagnetic resonance spectra of the same reaction quenched at ∼200 μs show a convex peak at g = 2.00, which is identified as compound I due to its microwave power and temperature dependencies. The absence of ferric signals in the electron paramagnetic resonance spectra of the quenched sample indicates that compound I is formed within ∼200 μs after mixing HRP and H2O2. We conclude that the activation of H2O2 in HRP at ambient temperature completes within ∼200 μs. The developed device can be generally applied to investigate the electronic structures of short-lived intermediates of metalloenzymes.
机译:为了观察辣根过氧化物酶(HRP)中化合物I的形成过程,我们开发了一种新的冷冻淬灭装置,其混合至冻结时间间隔约为200μs,并观察了HRP与过氧化氢(H2O2)之间的反应。开发的设备包括一个亚毫秒级的溶液混合器和冷却至77 K的旋转铜或银板;它冻结了旋转板表面上混合溶液的小滴。 HRP和H2O2混合后在约1 ms处淬灭的样品的紫外-可见光谱表明形成了化合物I。在〜200μs处淬灭的同一反应的电子顺磁共振谱在g = 2.00处显示凸峰,由于其微波功率和温度依赖性,其被鉴定为化合物I。淬火样品的电子顺磁共振光谱中没有铁信号,表明在混合HRP和H2O2后约200μs内形成了化合物I。我们得出结论,环境温度下HRP中H2O2的活化在约200μs内完成。所开发的装置通常可用于研究金属酶的短寿命中间体的电子结构。

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