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Electron transfer reactions in the alkene mono-oxygenase complex from Nocardia corallina B-276

机译:诺卡氏菌B-276烯烃单加氧酶复合物的电子转移反应

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piNocardia corallina/i B-276 possesses a multi-component enzyme, alkene mono-oxygenase (AMO), that catalyses the stereoselective epoxygenation of alkenes. The reductase component of this system has been shown by EPR and fluorescence spectroscopy to contain two prosthetic groups, an FAD centre and a [2Fe–2S] cluster. The role of these centres in the epoxygenation reaction was determined by midpoint potential measurements and electron transfer kinetics. The order of potentials of the prosthetic groups of the reductase were FAD/FADsup?/sup = -216 mV, [2Fe–2S]/[2Fe–2S]sup?/sup = -160 mV and FADsup?/sup/FADsup?/supsup?/sup = -134 mV. Combined, these data implied that the reductase component supplied the energy required for the epoxygenation reaction and allowed a prediction of the mechanism of electron transfer within the AMO complex. The FAD moiety was reduced by bound NADH in a two-electron reaction. The electrons were then transported to the [2Fe–2S] centre one at a time, which in turn reduced the di-iron centre of the epoxygenase. Reduction of the di-iron centre is required for oxygen binding and substrate oxidation./p
机译:> 珊瑚诺卡氏菌 B-276具有多组分酶烯烃单加氧酶(AMO),可催化烯烃的立体选择性环氧化反应。 EPR和荧光光谱显示该系统的还原酶成分包含两个修复基团,一个FAD中心和一个[2Fe–2S]簇。这些中心在环氧反应中的作用由中点电势测量和电子转移动力学确定。还原酶假体组的电位顺序为:FAD / FAD ? = -216mV,[2Fe–2S] / [2Fe–2S] ? =- 160mV和FAD ? / FAD ? = -134mV。综合来看,这些数据表明还原酶组分提供了环氧化反应所需的能量,并可以预测AMO络合物内电子转移的机理。 FAD部分在两电子反应中被结合的NADH还原。然后,电子一次被传输到[2Fe-2S]中心,这反过来又降低了环氧合酶的二铁中心。氧结合和底物氧化需要还原二铁中心。

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