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[来自牛肾上腺皮质线粒体的11-β-类固醇羟化细胞色素P-450:分离、物理化学及功能特性]

[11-beta-Steroid hydroxylating cytochrome P-450 from bovine adrenal cortex mitochondria: isolation, physico-chemical and functional properties].

作者信息

Martsev S P, Chashchin V L, Akhrem A A

出版信息

Biokhimiia. 1982 Jul;47(7):1070-83.

PMID:6981432
Abstract

It was shown that of the two cytochromes P-450, i.e. cholesterol-hydroxylating (SCC) and 11 beta-steroid-hydroxylating (11 beta) ones, involved in mitochondrial steroidogenesis in adrenal cortex cells cytochrome P-450 (11 beta) is more tightly bound to the membrane. The quantitative ratio of P-450 (SCC)/P-450 (11 beta) in the mitochondrial membrane is 2 to 1. The isolation procedure for cytochrome P-450 (11 beta) included separation of cytochromes P-450 (11 beta) and P-450 (SCC) by ammonium sulfate fractionation in the presence of sodium cholate, Tween 80 and affinity chromatography on adrenodoxin-Sepharose allowing to achieve a high degree of cytochrome P-450 (11 beta) purification. The obtained protein has a high specific heme content (19 nmole per mg of protein), minimal molecular weight (47000), is homogeneous as can be evidenced by Na-DS polyacrylamide gel electrophoresis and N-terminal analysis, possesses spectral properties typical for a high spin hemoprotein and is highly active in the reaction of steroid substrate hydroxylation. The Km values for hydroxylation of deoxycorticosterone (DOC), 11-deoxycorticol and testosterone are 0.69, 0.54 and 0.21 s-1, respectively. The use of adrenodoxin possessing a high stabilizing action allows to obtain cytochrome P-450 (11 beta) free from substrate (a low spin form) by washing of adrenodoxin-Sepharose adsorbed hemoprotein with large volumes of steroid-free phosphate buffer. The eluted cytochrome P-450 (11 beta) reveals spectral properties typical for the low spin hemoprotein; an addition of DOC induces type I spectral changes. The Kd values for the cytochrome P-450 (11 beta)-steroid complex determined by spectrophotometric titration at 10 degrees for DOC and testosterone are 0.32 and 0.67 muM, respectively.

摘要

结果表明,在肾上腺皮质细胞线粒体类固醇生成过程中涉及的两种细胞色素P - 450,即胆固醇羟化酶(SCC)和11β - 类固醇羟化酶(11β)中,细胞色素P - 450(11β)与膜的结合更为紧密。线粒体膜中P - 450(SCC)/P - 450(11β)的定量比例为2比1。细胞色素P - 450(11β)的分离程序包括在胆酸钠、吐温80存在下通过硫酸铵分级分离细胞色素P - 450(11β)和P - 450(SCC),以及在肾上腺铁氧还蛋白 - 琼脂糖上进行亲和色谱,从而实现细胞色素P - 450(11β)的高度纯化。所获得的蛋白质具有高特异性血红素含量(每毫克蛋白质19纳摩尔)、最小分子量(47000),通过Na - DS聚丙烯酰胺凝胶电泳和N端分析可证明其具有均一性,具有高自旋血红素蛋白典型的光谱特性,并且在类固醇底物羟化反应中具有高活性。脱氧皮质酮(DOC)、11 - 脱氧皮质醇和睾酮羟化反应的Km值分别为0.69、0.54和0.21 s-1。使用具有高稳定作用的肾上腺铁氧还蛋白,通过用大量无类固醇的磷酸盐缓冲液洗涤吸附在肾上腺铁氧还蛋白 - 琼脂糖上的血红素蛋白,可获得无底物的细胞色素P - 450(11β)(低自旋形式)。洗脱的细胞色素P - 450(11β)显示出低自旋血红素蛋白典型的光谱特性;加入DOC会诱导I型光谱变化。通过在10℃下分光光度滴定法测定的细胞色素P - 450(11β) - 类固醇复合物对于DOC和睾酮的Kd值分别为0.32和0.67μM。

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