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借助荧光凝胶对欧洲亚硝化单胞菌的c型细胞色素进行表征。

Characterization of the c-type cytochromes of Nitrosomonas europaea with the aid of fluorescent gels.

作者信息

Miller D J, Wood P M

出版信息

Biochem J. 1982 Dec 1;207(3):511-7. doi: 10.1042/bj2070511.

Abstract

When a total soluble extract of Nitrosomonas europaea was denatured with dodecyl sulphate, subjected to dodecyl sulphate/polyacrylamide-gel electrophoresis and illuminated with near-u.v. light, eight bands of protein fluorescence were observed. All but one of these bands were red in colour, a property characteristic of c-type cytochromes. Standard techniques were used to purify soluble c-type cytochromes from this organism, and it was then possible to assign all but two very minor bands to specific c-type cytochromes, namely hydroxylamine oxidase, cytochrome c-554, cytochrome c-552 and a cytochrome c-550 not previously described. The eight band had fluorescence peaking in the green region of the spectrum, probably caused by covalently bound flavin, and co-purified with hydroxylamine oxidase. The following physical properties were determined for these components: isoelectric point, molecular weights according to gel filtration and mobility on dodecyl sulphate/polyacrylamide gels, and alpha-band spectra at room temperature and 77K. Redox potentials were measured as follows: cytochrome c-554, E(m,7) = +20mV; cytochrome c-552, E(m,7) = +230mV; cytochrome c-550, E(m,7) = +140mV. When washed membranes were applied to dodecyl sulphate/polyacrylamide gels in the same way, a number of fluorescent bands were observed that could be matched by soluble proteins. In addition, there was one band that could not be detected in supernatants, migrating with an apparent molecular weight of 24000. This species is probably coincident with a c-type cytochrome having E(m,7) = +170mV found in redox titration of these membranes. In future studies, gel fluorescence should form a useful complement to spectroscopy for analysis of cytochrome composition in active cell-free preparations or semi-purified material.

摘要

当欧洲亚硝化单胞菌的总可溶性提取物用十二烷基硫酸盐变性、进行十二烷基硫酸盐/聚丙烯酰胺凝胶电泳并用近紫外光照射时,观察到八条蛋白质荧光带。除了其中一条带外,其他所有带均为红色,这是c型细胞色素的特性。使用标准技术从该生物体中纯化可溶性c型细胞色素,然后除了两条非常小的带外,所有带都可以归属于特定的c型细胞色素,即羟胺氧化酶、细胞色素c-554、细胞色素c-552和一种以前未描述的细胞色素c-550。第八条带的荧光在光谱的绿色区域达到峰值,可能是由共价结合的黄素引起的,并与羟胺氧化酶共纯化。测定了这些组分的以下物理性质:等电点、根据凝胶过滤法测定的分子量以及在十二烷基硫酸盐/聚丙烯酰胺凝胶上的迁移率,以及在室温及77K下的α带光谱。氧化还原电位的测量结果如下:细胞色素c-554,E(m,7) = +20mV;细胞色素c-552,E(m,7) = +230mV;细胞色素c-550,E(m,7) = +140mV。当以相同方式将洗涤过的膜应用于十二烷基硫酸盐/聚丙烯酰胺凝胶时,观察到一些荧光带,这些带可以与可溶性蛋白质匹配。此外,有一条带在上清液中未检测到,其表观分子量为24000。该物种可能与在这些膜的氧化还原滴定中发现的E(m,7) = +170mV的c型细胞色素一致。在未来的研究中,凝胶荧光应该成为光谱学的有用补充,用于分析无细胞活性制剂或半纯化材料中的细胞色素组成。

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Detection of cytochromes on sodium dodecylsulphate-polyacrylamide gels by their intrinsic fluorescence.
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