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细胞色素c2对于红假单胞菌中电子从生理底物转移至一氧化二氮还原酶至关重要,并且在体外可作为该还原酶的电子供体。与光抑制研究的相关性。

Cytochrome c2 is essential for electron transfer to nitrous oxide reductase from physiological substrates in Rhodobacter capsulatus and can act as an electron donor to the reductase in vitro. Correlation with photoinhibition studies.

作者信息

Richardson D J, Bell L C, McEwan A G, Jackson J B, Ferguson S J

机构信息

School of Biochemistry, University of Birmingham, England.

出版信息

Eur J Biochem. 1991 Aug 1;199(3):677-83. doi: 10.1111/j.1432-1033.1991.tb16170.x.

DOI:10.1111/j.1432-1033.1991.tb16170.x
PMID:1651241
Abstract
  1. Addition of nitrous oxide to a periplasmic fraction released from Rhodobacter capsulatus strains MT1131, N22DNAR+ or AD2 caused oxidation of c-type cytochrome, as judged by the decrease in absorbance at 550 nm. The periplasmic fraction catalysed reduction of nitrous oxide in the presence of either isoascorbate plus phenazine ethosulphate or reduced methyl viologen. The rates with these two electron donors were similar and were comparable to the activity observed with a quantity of cells equivalent to those from which the periplasm sample had been derived. Activity in the periplasm could not be observed with ascorbate plus 2,3,5,6-tetramethyl-p-phenylenediamine although this reductant was effective with intact cells treated with myxothiazol to block the activity of the cytochrome-bc1 complex. 2. Cells of R. capsulatus MTG4/S4, a mutant from which the gene for cytochrome c2 has been specifically deleted, did not catalyse detectable rates of nitrous-oxide reduction. A nitrous-oxide reductase activity was present, as shown by activity of both cells and a periplasmic fraction with isoascorbate plus phenazine ethosulphate as reductant. The rates in cells and the periplasmic fraction were similar to those observed in the corresponding wild-type strain (MT1131). In contrast to wild-type cells, 2,3,5,6-tetramethyl-p-phenylenediamine and N,N,N',N'-tetramethyl-p-phenylenediamine [Ph(NMe2)2] were ineffective as mediators of electrons from isoascorbate. Visible absorption spectra showed that no detectable cytochromes in either the periplasm or intact cells of the MTG4/S4 mutant were oxidised by nitrous oxide. 3. Purified ferroycytochrome c2 from R. capsulatus was oxidised by nitrous oxide in the presence of periplasm from R. capsulatus MTG4/S4. The rate of oxidation was proportional to the amount of periplasm added, but was considerably lower than the rate of nitrous-oxide reduction observed with the same periplasmic fraction when either ascorbate plus phenazine ethosulphate or reduced methyl viologen were used as substrates. The oxidation of cytochrome c2 was inhibited by acetylene and by low concentrations of NaCl. 4. Oxidation of ferrocytochrome c2 by nitrous oxide was observed when the purified cytochrome was mixed with a preparation of nitrous-oxide reductase. However, oxidation of ferrocytochrome c' by nitrous oxide was not observed in the presence of the reductase. The observations with the mutant MTG4/S4 suggest that cytochrome c2 is the only periplasmic cytochrome involved in nitrous-oxide reduction. 5. Nitrous-oxide-dependent oxidation of a c-type cytochrome was observed in a periplasmic fraction from Paracoccus denitrificans, provided the fraction was first reduced.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 向来自荚膜红细菌菌株MT1131、N22DNAR+或AD2释放的周质组分中添加一氧化二氮,导致c型细胞色素氧化,这可通过550nm处吸光度的降低来判断。周质组分在异抗坏血酸加吩嗪硫酸乙酯或还原型甲基紫精存在的情况下催化一氧化二氮的还原。这两种电子供体的反应速率相似,且与用相当于衍生出周质样品的细胞数量所观察到的活性相当。抗坏血酸加2,3,5,6 - 四甲基 - 对苯二胺时,周质中未观察到活性,尽管这种还原剂对用粘噻唑处理以阻断细胞色素bc1复合物活性的完整细胞有效。2. 荚膜红细菌MTG4/S4是一个特异性缺失细胞色素c2基因的突变体,其细胞不能催化可检测到的一氧化二氮还原速率。存在一氧化二氮还原酶活性,这可通过细胞和周质组分以异抗坏血酸加吩嗪硫酸乙酯作为还原剂的活性来表明。细胞和周质组分中的反应速率与在相应野生型菌株(MT1131)中观察到的相似。与野生型细胞相反,2,3,5,6 - 四甲基 - 对苯二胺和N,N,N',N' - 四甲基 - 对苯二胺[Ph(NMe2)2]作为来自异抗坏血酸的电子传递介质无效。可见吸收光谱表明,MTG4/S4突变体的周质或完整细胞中没有可检测到的细胞色素被一氧化二氮氧化。3. 在存在荚膜红细菌MTG4/S4周质的情况下,来自荚膜红细菌的纯化亚铁细胞色素c2被一氧化二氮氧化。氧化速率与添加的周质量成正比,但远低于当抗坏血酸加吩嗪硫酸乙酯或还原型甲基紫精用作底物时用相同周质组分观察到的一氧化二氮还原速率。细胞色素c2的氧化受到乙炔和低浓度氯化钠的抑制。4. 当纯化的细胞色素与一氧化二氮还原酶制剂混合时,观察到一氧化二氮对亚铁细胞色素c2的氧化。然而,在还原酶存在的情况下未观察到一氧化二氮对亚铁细胞色素c'的氧化。对突变体MTG4/S4的观察表明,细胞色素c2是参与一氧化二氮还原的唯一周质细胞色素。5. 在反硝化副球菌的周质组分中观察到一氧化二氮依赖的c型细胞色素氧化,前提是该组分首先被还原。(摘要截短至400字)

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