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使用甘胆酸盐和生物珠将NADPH-细胞色素P450还原酶和细胞色素P450物理掺入磷脂囊泡中。

Physical incorporation of NADPH-cytochrome P450 reductase and cytochrome P450 into phospholipid vesicles using glycocholate and Bio-Beads.

作者信息

Reed James R, Brignac-Huber Lauren M, Backes Wayne L

机构信息

Louisiana State University Health Science Center, Department of Pharmacology and the Stanley S. Scott Cancer Center, 533 Bolivar St., New Orleans, LA 70112, USA.

出版信息

Drug Metab Dispos. 2008 Mar;36(3):582-8. doi: 10.1124/dmd.107.018473. Epub 2007 Nov 29.

Abstract

In a previous study from our laboratory (Drug Metab Dispos 34: 660-666, 2006), we found several limitations with published methods (cholate gel filtration and cholate dialysis) for the incorporation of cytochromes P450 and P450 reductase into phospholipid vesicles. We found that a significant proportion of reductase was not incorporated in the vesicles when the amount of reductase was equal to or greater than that of CYP2B4 in the systems reconstituted with phosphatidylcholine. Furthermore, implementation of these methods compromised the ability of the CYP2B4 to form a ferrous carbon monoxy complex. In the current study, a comparison of results using the detergent-dialysis method with five similar detergents having the "bile salt" ring structure showed that glycocholate results in the greatest incorporation of reductase and the least loss in the ferrous carbon monoxy CYP2B4 complex. The method is further improved by using Bio-Beads SM-2 to remove detergent instead of the lengthy dialysis procedure or size exclusion chromatography that significantly dilutes the protein and lipid concentrations of the preparation. The method is shown to be applicable over a range of lipid/CYP2B4 ratios, and by using assay methods for total lipid, reductase, and CYP2B4, this improved reconstitution method resulted in increased incorporation efficiencies while minimizing the protein degradation inherent with these procedures.

摘要

在我们实验室之前的一项研究中(《药物代谢与处置》34: 660 - 666, 2006),我们发现已发表的将细胞色素P450和P450还原酶掺入磷脂囊泡的方法(胆酸盐凝胶过滤法和胆酸盐透析法)存在一些局限性。我们发现,在用磷脂酰胆碱重构的体系中,当还原酶的量等于或大于CYP2B4的量时,很大一部分还原酶未掺入囊泡中。此外,这些方法的实施损害了CYP2B4形成亚铁一氧化碳复合物的能力。在当前研究中,使用去污剂透析法并比较五种具有“胆盐”环结构的类似去污剂的结果表明,甘氨胆酸盐导致还原酶的掺入量最大,且亚铁一氧化碳CYP2B4复合物的损失最小。通过使用Bio - Beads SM - 2去除去污剂,而不是使用会显著稀释制剂中蛋白质和脂质浓度的冗长透析程序或尺寸排阻色谱法,该方法得到了进一步改进。结果表明该方法适用于一系列脂质/CYP2B4比例,并且通过使用针对总脂质、还原酶和CYP2B4的测定方法,这种改进的重构方法提高了掺入效率,同时将这些程序中固有的蛋白质降解降至最低。

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