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大肠杆菌有氧呼吸链含硫铁的NADH-泛醌氧化还原酶的电子顺磁共振表征

EPR characterization of the iron-sulfur-containing NADH-ubiquinone oxidoreductase of the Escherichia coli aerobic respiratory chain.

作者信息

Meinhardt S W, Matsushita K, Kaback H R, Ohnishi T

机构信息

Department of Biochemistry and Biophysics, University of Pennsylvania, Philadelphia 19104.

出版信息

Biochemistry. 1989 Mar 7;28(5):2153-60. doi: 10.1021/bi00431a029.

DOI:10.1021/bi00431a029
PMID:2541776
Abstract

The energy coupled NADH-ubiquinone (Q) oxidoreductase segment of the respiratory chain of Escherichia coli GR19N has been studied by EPR spectroscopy. Previously Matsushita et al. [(1987) Biochemistry 26, 7732-7737] have demonstrated the presence of two distinct NADH-Q oxidoreductases in E. coli membrane particles and designated them NADH dh I and NADH dh II. Although both enzymes oxidize NADH, only NADH dh I is coupled to the formation of the H+ electrochemical gradient. In addition to NADH, NADH dh I oxidizes nicotinamide hypoxanthine dinucleotide (deamino-NADH), while NADH dh II does not. In membrane particles we have detected EPR signals arising from four low-potential iron-sulfur clusters, one binuclear, one tetranuclear, and two fast spin relaxing g perpendicular = 1.94 type clusters (whose cluster structure has not yet been assigned). The binuclear cluster, temporarily designated [N-1]E, shows an EPR spectrum with gx,y,z = 1.92, 1.935, 2.03 and the Em7.4 value of -220 mV (n = 1). The tetranuclear cluster, [N-2]E, elicits a spectrum with gx,y,z = 1.90, 1.91, 2.05 and an Em7.4 of -240 mV (n = 1). These two clusters have been shown to be part of the NADH dh I complex by stability and inhibitor studies. When stored at 4 degrees C, both clusters are extremely labile as is the deamino-NADH-Q oxidoreductase activity. Addition of deamino-NADH in the presence of piericidin A results in nearly full reduction of [N-2]E within 17 s. In membrane particles pretreated with piericidin A, the cluster [N-1]E is only partly reducible by deamino-NADH and shows an altered line shape.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

通过电子顺磁共振波谱法对大肠杆菌GR19N呼吸链中能量偶联的NADH-泛醌(Q)氧化还原酶片段进行了研究。此前,松下等人[(1987年)《生物化学》26卷,7732 - 7737页]已证明大肠杆菌膜颗粒中存在两种不同的NADH-Q氧化还原酶,并将它们命名为NADH dh I和NADH dh II。虽然这两种酶都能氧化NADH,但只有NADH dh I与H⁺电化学梯度的形成偶联。除了NADH,NADH dh I还能氧化烟酰胺次黄嘌呤二核苷酸(脱氨基-NADH),而NADH dh II则不能。在膜颗粒中,我们检测到了来自四个低电位铁硫簇的电子顺磁共振信号,一个双核簇、一个四核簇以及两个快速自旋弛豫的g⊥ = 1.94型簇(其簇结构尚未确定)。双核簇暂时命名为[N - 1]E,其电子顺磁共振谱显示gx,y,z = 1.92、1.935、2.03,Em7.4值为 - 220 mV(n = 1)。四核簇[N - 2]E产生的谱线gx,y,z = 1.90、1.91、2.05,Em7.4为 - 240 mV(n = 1)。通过稳定性和抑制剂研究表明,这两个簇是NADH dh I复合物的一部分。当在4℃储存时,这两个簇以及脱氨基-NADH-Q氧化还原酶活性都极其不稳定。在存在粉蝶霉素A的情况下添加脱氨基-NADH会导致[N - 2]E在17秒内几乎完全还原。在用粉蝶霉素A预处理的膜颗粒中,簇[N - 1]E仅能被脱氨基-NADH部分还原,并且谱线形状发生改变。(摘要截断于250字)

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