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人中性粒细胞细胞色素b558小亚基的纯化及某些性质

Purification and some properties of the small subunit of cytochrome b558 from human neutrophils.

作者信息

Yamaguchi T, Hayakawa T, Kaneda M, Kakinuma K, Yoshikawa A

机构信息

National Institute of Hygienic Sciences, Tokyo, Japan.

出版信息

J Biol Chem. 1989 Jan 5;264(1):112-8.

PMID:2909509
Abstract

We have attempted to purify the heme moiety of cytochrome b558 from human neutrophils. Cytochrome b558 was solubilized from the crude membrane fraction which was pretreated with both 1 M potassium phosphate buffer and 1% octyl glucoside at low ionic strength. The solubilization of cytochrome b558 was carried out efficiently with 1.6% octyl glucoside in the presence of 100 mM phosphate buffer. Solubilized cytochrome b558 was purified by hydroxylapatite, DEAE-Sephacel, and Mono Q fast protein liquid chromatography. The specific content of purified cytochrome b558 was 37 nmol/mg of protein. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis analysis of purified cytochrome b558 revealed a single band of 20,000 Da. The large subunit of cytochrome b558, which has been reported by others, could not be found in purified cytochrome b558 even with silver staining. The amino acid composition of the heme-containing moiety of cytochrome b558 was abundant in hydrophobic amino acids. The circular dichroism spectra of both oxidized and reduced b558-type cytochromes exhibited bilobed bands with wavelengths of crossover points closely corresponding to those of the maxima in the optical absorbance spectra at the Soret region. Furthermore, there were some differences in the shoulders and peak widths of CD spectra between oxidized and reduced b558-type cytochromes. These results indicate that this method provides the purification of the small subunit of human cytochrome b558 which is the heme-carrying subunit of cytochrome b558, and suggest that cytochrome b558 has heme-heme interaction and some conformational changes in the alternation of the redox state.

摘要

我们已尝试从人中性粒细胞中纯化细胞色素b558的血红素部分。细胞色素b558是从粗膜组分中溶解出来的,该粗膜组分在低离子强度下用1 M磷酸钾缓冲液和1%辛基葡糖苷进行了预处理。在100 mM磷酸缓冲液存在下,用1.6%辛基葡糖苷可有效地溶解细胞色素b558。溶解的细胞色素b558通过羟基磷灰石、DEAE-琼脂糖凝胶和Mono Q快速蛋白质液相色谱进行纯化。纯化的细胞色素b558的比含量为37 nmol/mg蛋白质。纯化的细胞色素b558的十二烷基硫酸钠-聚丙烯酰胺凝胶电泳分析显示有一条20,000 Da的单带。即使进行银染,在纯化的细胞色素b558中也未发现其他人报道的细胞色素b558的大亚基。细胞色素b558含血红素部分的氨基酸组成富含疏水氨基酸。氧化型和还原型b558型细胞色素的圆二色光谱均呈现双叶带,其交叉点波长与索雷特区域光吸收光谱中的最大值波长密切对应。此外,氧化型和还原型b558型细胞色素的圆二色光谱在肩部和峰宽上存在一些差异。这些结果表明该方法提供了人细胞色素b558小亚基的纯化,该小亚基是细胞色素b558的血红素携带亚基,并表明细胞色素b558在氧化还原状态转变中存在血红素-血红素相互作用和一些构象变化。

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