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人25-羟基维生素D3-24-羟化酶,一种多功能酶。

Human 25-hydroxyvitamin D3-24-hydroxylase, a multicatalytic enzyme.

作者信息

Beckman M J, Tadikonda P, Werner E, Prahl J, Yamada S, DeLuca H F

机构信息

Department of Biochemistry, University of Wisconsin-Madison, 53706, USA.

出版信息

Biochemistry. 1996 Jun 25;35(25):8465-72. doi: 10.1021/bi960658i.

DOI:10.1021/bi960658i
PMID:8679605
Abstract

Human 25-hydroxyvitamin D-24-hydroxylase has been expressed in Spodoptera frugiperda (Sf21) insect cells using the previously cloned cDNA in baculovirus (AcNPV-P450cc24). The activity of recombinant h-P450cc24 required adrenodoxin, adrenodoxin reductase, and NADPH. Incubation of this reconstituted system with 25-OH-[26,27-(3)H]D3 substrate produced several metabolites that were resolved on a normal-phase cyano HPLC system. These products exactly comigrated with authentic standards for 24-oxo-25-OH-D3, 23(S),25-(OH)2D3, 24(R),25-(OH)2D3, and 24-oxo-23(S),25-(OH)2D3. The soluble proteins from Sf21 cells infected with wild-type baculovirus produced neither 24,25-(OH)2D3 nor any of the other 25-OH-D3 metabolites. The products were isolated and subjected to a normal-phase amino HPLC for further separation, purification, and characterization. Comigration on two HPLC systems, periodate cleavage reactions, and NaBH4 reduction established clearly the identity of these metabolites. Incubation of recombinant h-P450cc24 with 25-OH-[3 alpha-3H]D3 led to the isolation of an additional product that comigrated with 24,25,26,27-tetranor-23-OH-D3. Treatment of putative 24,25,26,27-tetranor-23-OH-[3 alpha-3H]D3 with acetic anhydride changed its migration on amino HPLC to a less polar position, indicating acetylation of a hydroxyl group(s). These data demonstrate conclusively that h-P450cc24 is a multicatalytic enzyme catalyzing most, if not all, of the reactions in the C-24/C-23 pathway of 25-OH-D3 metabolism. It is likely that this enzyme by itself converts 25-OH-D3 and 1,25-(OH)2D3 to one of its final excretion products.

摘要

利用先前在杆状病毒(AcNPV-P450cc24)中克隆的cDNA,已在草地贪夜蛾(Sf21)昆虫细胞中表达了人25-羟基维生素D-24-羟化酶。重组h-P450cc24的活性需要肾上腺皮质铁氧化还原蛋白、肾上腺皮质铁氧化还原蛋白还原酶和NADPH。用25-OH-[26,27-(3)H]D3底物孵育该重组系统产生了几种代谢产物,这些代谢产物在正相氰基HPLC系统上得以分离。这些产物与24-氧代-25-OH-D3、23(S),25-(OH)2D3、24(R),25-(OH)2D3和24-氧代-23(S),25-(OH)2D3的标准品在HPLC上完全共迁移。感染野生型杆状病毒的Sf21细胞的可溶性蛋白既不产生24,25-(OH)2D3,也不产生任何其他25-OH-D3代谢产物。对这些产物进行分离,并通过正相氨基HPLC进行进一步分离、纯化和鉴定。在两个HPLC系统上的共迁移、高碘酸盐裂解反应和NaBH4还原明确确定了这些代谢产物的身份。用25-OH-[3α-3H]D3孵育重组h-P450cc24导致分离出一种与24,25,26,27-四降-23-OH-D3共迁移的额外产物。用乙酸酐处理假定的24,25,26,27-四降-23-OH-[3α-3H]D3会使其在氨基HPLC上的迁移位置变为极性较小的位置,表明有羟基发生了乙酰化。这些数据确凿地证明,h-P450cc24是一种多催化酶,催化25-OH-D3代谢的C-24/C-23途径中的大部分(如果不是全部)反应。很可能这种酶自身将25-OH-D3和1,25-(OH)2D3转化为其最终排泄产物之一。

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