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反硝化副球菌中节约能量的一氧化氮还原酶系统。与催化一氧化氮合成的亚硝酸还原酶的区别以及反硝化过程中一氧化氮作为游离中间体的捕获实验证据。

The energy-conserving nitric-oxide-reductase system in Paracoccus denitrificans. Distinction from the nitrite reductase that catalyses synthesis of nitric oxide and evidence from trapping experiments for nitric oxide as a free intermediate during denitrification.

作者信息

Carr G J, Page M D, Ferguson S J

机构信息

Department of Biochemistry, University of Oxford, England.

出版信息

Eur J Biochem. 1989 Feb 15;179(3):683-92. doi: 10.1111/j.1432-1033.1989.tb14601.x.

DOI:10.1111/j.1432-1033.1989.tb14601.x
PMID:2920732
Abstract
  1. A Clark-type electrode that responds to nitric oxide has been used to show that cytoplasmic membrane vesicles of Paracoccus denitrificans have a nitric-oxide reductase activity. Nitrous oxide is the reaction product. NADH, succinate or isoascorbate plus 2,3,5,6-tetramethyl-1,4-phenylene diamine can act as reductants. The NADH-dependent activity is resistant to freezing of the vesicles and thus the NADH:nitric-oxide oxidoreductase activity of stored frozen vesicles provides a method for calibrating the electrode by titration of dissolved nitric oxide with NADH. The periplasmic nitrite reductase and nitrous-oxide reductase enzymes are absent from the vesicles which indicates that nitric-oxide reductase is a discrete enzyme associated with the denitrification process. This conclusion was supported by the finding that nitric-oxide reductase activity was absent from both membranes prepared from aerobically grown P. denitrificans and bovine heart submitochondrial particles. 2. The NADH: nitric-oxide oxidoreductase activity was inhibited by concentrations of antimycin or myxothiazol that were just sufficient to inhibit the cytochrome bc1 complex of the ubiquinol--cytochrome-c oxidoreductase. The activity was deduced to be proton translocating by the observations of: (a) up to 3.5-fold stimulation upon addition of an uncoupler; and (b) ATP synthesis with a P:2e ratio of 0.75. 3. Nitrite reductase of cytochrome cd1 type was highly purified from P. denitrificans in a new, high-yield, rapid two- or three-step procedure. This enzyme catalysed stoichiometric synthesis of nitric oxide. This observation, taken together with the finding that the maximum rate of NADH:nitric-oxide oxidoreductase activity catalysed by the vesicles was comparable with that of NADH:nitrate-oxidoreductase, is consistent with a role for nitric-oxide reductase in the physiological conversion of nitrate or nitrite to dinitrogen gas. 4. Intact cells of P. denitrificans also reduced nitric oxide in an antimycin- or myxothiazol-sensitive manner. However, nitric oxide was not detected by the electrode during the reduction of nitrate. Nitric-oxide synthesis from nitrate could be detected with cells in the presence of very low concentrations of Triton X-100 which selectively inhibits nitric-oxide reductase activity. 5. Nitric oxide was detected as an intermediate in denitrification by including haemoglobin with an anaerobic suspension of cells that was reducing nitrate. The characteristic spectrum of the nitric oxide derivative of haemoglobin was observed.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 一种对一氧化氮有反应的克拉克型电极已被用于表明反硝化副球菌的细胞质膜囊泡具有一氧化氮还原酶活性。一氧化二氮是反应产物。烟酰胺腺嘌呤二核苷酸(NADH)、琥珀酸或异抗坏血酸加2,3,5,6 - 四甲基 - 1,4 - 苯二胺可作为还原剂。依赖NADH的活性对囊泡冷冻有抗性,因此储存的冷冻囊泡的NADH:一氧化氮氧化还原酶活性提供了一种通过用NADH滴定溶解的一氧化氮来校准电极的方法。囊泡中不存在周质亚硝酸还原酶和一氧化二氮还原酶,这表明一氧化氮还原酶是一种与反硝化过程相关的离散酶。这一结论得到以下发现的支持:从需氧生长的反硝化副球菌制备的膜和牛心亚线粒体颗粒中均不存在一氧化氮还原酶活性。2. NADH:一氧化氮氧化还原酶活性受到抗霉素或粘噻唑浓度的抑制,这些浓度刚好足以抑制泛醌 - 细胞色素c氧化还原酶的细胞色素bc1复合物。通过以下观察结果推断该活性是质子转运的:(a)加入解偶联剂后刺激高达3.5倍;(b)ATP合成的P:2e比值为0.75。3. 细胞色素cd1型亚硝酸还原酶通过一种新的、高产率、快速的两步或三步程序从反硝化副球菌中高度纯化。这种酶催化一氧化氮的化学计量合成。这一观察结果,连同囊泡催化的NADH:一氧化氮氧化还原酶活性的最大速率与NADH:硝酸盐氧化还原酶的最大速率相当这一发现,与一氧化氮还原酶在硝酸盐或亚硝酸盐向氮气的生理转化中的作用一致。4. 反硝化副球菌的完整细胞也以抗霉素或粘噻唑敏感的方式还原一氧化氮。然而,在硝酸盐还原过程中电极未检测到一氧化氮。在存在极低浓度的 Triton X - 100(其选择性抑制一氧化氮还原酶活性)的情况下,用细胞可以检测到从硝酸盐合成一氧化氮。5. 通过在还原硝酸盐的细胞厌氧悬浮液中加入血红蛋白,检测到一氧化氮是反硝化过程中的中间产物。观察到了血红蛋白一氧化氮衍生物的特征光谱。(摘要截断于400字)

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