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荚膜红假单胞菌泛醇 - 细胞色素c2氧化还原酶中醌的离散催化位点。来自泛醇氧化缺陷突变体的证据。

Discrete catalytic sites for quinone in the ubiquinol-cytochrome c2 oxidoreductase of Rhodopseudomonas capsulata. Evidence from a mutant defective in ubiquinol oxidation.

作者信息

Robertson D E, Davidson E, Prince R C, van den Berg W H, Marrs B L, Dutton P L

出版信息

J Biol Chem. 1986 Jan 15;261(2):584-91.

PMID:3001072
Abstract

A non-photosynthetic mutant (Ps-) of Rhodopseudomonas capsulata, designated R126, was analyzed for a defect in the cyclic electron transfer system. Compared to a Ps+ strain MR126, the mutant was shown to have a full complement of electron transfer components (reaction centers, ubiquinone-10, cytochromes b, c1, and c2, the Rieske 2-iron, 2-sulfur (Rieske FeS) center, and the antimycin-sensitive semiquinone). Functionally, mutant R126 failed to catalyze complete cytochrome c1 + c2 re-reduction or cytochrome b reduction following a short (10 microseconds) flash of actinic light. Evidence (from flash-induced carotenoid band shift) was characteristic of inhibition of electron transfer proximal to cytochrome c1 of the ubiquinol-cytochrome c2 oxidoreductase. Three lines of evidence indicate that the lesion of R126 disrupts electron transfer from quinol to Rieske FeS: 1) the degree of cytochrome c1 + c2 re-reduction following a flash is indicative of electron transfer from Rieske FeS to cytochrome c1 + c2 without redox equilibration with an additional electron from a quinol; 2) inhibitors that act at the Qz site and raise the Rieske FeS midpoint redox potential (Em), namely 5-undecyl-6-hydroxy-4,7-dioxobenzothiazole or 3-alkyl-2-hydroxy-1,4-napthoquinone, have no effect on cytochrome c1 + c2 oxidation in R126; 3) the Rieske FeS center, although it exhibits normal redox behavior, is unable to report the redox state of the quinone pool, as metered by its EPR line shape properties. Flash-induced proton binding in R126 is indicative of normal functional primary (QA) and secondary (QB) electron acceptor activity of the photosynthetic reaction center. The Qc functional site of cytochrome bc1 is intact in R126 as measured by the existence of antimycin-sensitive, flash-induced cytochrome b reduction.

摘要

对荚膜红假单胞菌的一个非光合突变体(Ps-)R126进行了循环电子传递系统缺陷分析。与光合阳性菌株MR126相比,该突变体显示具有完整的电子传递组分(反应中心、泛醌-10、细胞色素b、c1和c2、 Rieske 2-铁-2-硫(Rieske FeS)中心以及抗霉素敏感的半醌)。在功能上,突变体R126在短(10微秒)的光化光闪光后无法催化细胞色素c1 + c2的完全再还原或细胞色素b的还原。(来自闪光诱导的类胡萝卜素带位移的)证据表明泛醇-细胞色素c2氧化还原酶的细胞色素c1附近的电子传递受到抑制。三条证据表明R126的损伤破坏了从醌醇到Rieske FeS的电子传递:1)闪光后细胞色素c1 + c2的再还原程度表明电子从Rieske FeS传递到细胞色素c1 + c2,而没有与来自醌醇的额外电子进行氧化还原平衡;2)作用于Qz位点并提高Rieske FeS中点氧化还原电位(Em)的抑制剂,即5-十一烷基-6-羟基-4,7-二氧代苯并噻唑或3-烷基-2-羟基-1,4-萘醌,对R126中的细胞色素c1 + c2氧化没有影响;3)Rieske FeS中心虽然表现出正常的氧化还原行为,但无法通过其EPR线形特性来反映醌池的氧化还原状态。R126中闪光诱导的质子结合表明光合反应中心的初级(QA)和次级(QB)电子受体活性正常。通过抗霉素敏感的闪光诱导细胞色素b还原的存在来测量,细胞色素bc1的Qc功能位点在R126中是完整的。

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