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首页> 美国卫生研究院文献>Biochemical Journal >Low-spin ferric forms of cytochrome a3 in mixed-ligand and partially reduced cyanide-bound derivatives of cytochrome c oxidase.
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Low-spin ferric forms of cytochrome a3 in mixed-ligand and partially reduced cyanide-bound derivatives of cytochrome c oxidase.

机译:细胞色素c氧化酶的混合配体和部分还原的氰化物结合衍生物中的细胞色素a3的低旋铁形式。

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摘要

Optical-absorption-, e.p.r.- and m.c.d. (magnetic-circular-dichroism)-spectroscopic measurements were made on liganded derivatives of oxidized and partially reduced cytochrome c oxidase. When NO was added to oxidized cyanide-bound cytochrome c oxidase, no changes occurred in the optical-absorption difference spectrum. In contrast, NO induced reduction of cytochrome a3 and formation of the nitrosylferrohaem species when the oxidized resting enzyme was the starting material. E.p.r. spectroscopy of the NO-treated oxidized cyanide-bound enzyme revealed the presence of a low-spin haem signal at g = 3.40, whereas the g = 3.02 and g = 2.0 signals of the oxidized enzyme remained unchanged. Both haem groups in this species are e.p.r.-detectable simultaneously. Examination of an identical sample by m.c.d. spectroscopy in the near-i.r. region identified two distinct low-spin species at 1565 and 1785 nm. Irradiation with white light of the NO-treated cyanide-bound sample at 10K resulted in the disappearance of the g = 3.40 e.p.r. signal and the m.c.d. signal at 1785 nm, whereas a band at 1950nm increased in intensity. When the photolysed sample was warmed to 50K and held in the dark for 15 min, the original spectrum returned. Magnetization studies of the 1785nm m.c.d. band support the assignment of this signal to the same metal centre that gives rise to the g = 3.40 e.p.r. signal. The effect of NO on the oxidized cyanide-bound enzyme was compared with that obtained when the oxidized cyanide-bound species was taken to the partially reduced state. Cytochrome a3 is e.p.r.-detectable with a g-value of 3.58 [Johnson, Eglinton, Gooding, Greenwood & Thomson (1981) Biochem. J. 193, 699-708]. Its near-i.r. m.c.d. spectrum shifts from 1950nm in the oxidized cyanide-bound enzyme to 1545nm on addition of reductant. A scheme is advanced for the structure of the cytochrome a3-CuB site that allows for cyanide binding to Fea3 and NO binding to CuB. Cyanide is the bridging ligand in the ferromagnetically coupled cytochrome a3-CuB pair of oxidized cyanide-bound cytochrome c oxidase. The bridged structure and the magnetic interaction are broken when the enzyme is partially reduced. However, when NO binds to CuB the cyanide bridge remains intact, but now the odd spins of NO and CuB are magnetically coupled.
机译:光吸收-e.p.r.-和m.c.d. (磁性-圆二色性)光谱测量是对氧化的和部分还原的细胞色素c氧化酶的配体衍生物进行的。在氧化氰化物结合的细胞色素C氧化酶中添加NO时,吸光度差光谱未发生变化。相反,当氧化的静止酶为起始原料时,NO诱导细胞色素a3还原并形成亚硝酰基铁血红素。 E.p.r. NO处理的氧化氰化物结合的酶的光谱分析表明,在g = 3.40处存在低旋血红素信号,而氧化酶的g = 3.02和g = 2.0信号保持不变。该物种中的两个血红素族均可同时被e.p.r.检测到。通过m.c.d检查相同的样品近红外光谱该区域在1565和1785 nm处识别出两种不同的低自旋物种。在10K下用NO处理的氰化物结合的样品用白光照射导致g = 3.40 e.p.r的消失。信号和MCD信号在1785 nm处发射,而1950 nm处的波段强度增加。当将光解样品加热到50K并在黑暗中放置15分钟后,原始光谱恢复。 1785nm m.c.d.的磁化研究频段支持将此信号分配给同一金属中心,从而导致g = 3.40e.p.r。信号。将NO对氧化氰化物结合的酶的影响与当将氧化氰化物结合的物质变为部分还原状态时获得的效果进行比较。可以检测到细胞色素a3,其g值为3.58 [Johnson,Eglinton,Gooding,Greenwood&Thomson(1981)Biochem。 J. 193,699-708]。它的近红外立方米加入还原剂后,光谱从氧化氰化物结合的酶的1950nm转变为1545nm。对于细胞色素a3-CuB位点的结构,提出了一种方案,该方案允许氰化物与Fea3结合,而NO与CuB结合。氰化物是铁磁耦合的细胞色素a3-CuB对中氧化氰化物结合的细胞色素c氧化酶中的桥连配体。当酶部分还原时,桥连的结构和磁性相互作用被破坏。但是,当NO与CuB结合时,氰化物桥保持完整,但是现在NO和CuB的奇数自旋磁性耦合。

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