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二氢神经酰胺:鞘氨醇C-4羟基化需要Des2羟化酶和细胞色素b5的膜形式。

Dihydroceramide:sphinganine C-4-hydroxylation requires Des2 hydroxylase and the membrane form of cytochrome b5.

作者信息

Enomoto Ayako, Omae Fumio, Miyazaki Masao, Kozutsumi Yasunori, Yubisui Toshitsugu, Suzuki Akemi

机构信息

Sphingolipid Expression Laboratory, Frontier Research System, RIKEN, Wako 351-0198, Japan.

出版信息

Biochem J. 2006 Jul 15;397(2):289-95. doi: 10.1042/BJ20051938.

Abstract

Des2 (degenerative spermatocyte 2) is a bifunctional enzyme that produces phytoceramide and ceramide from dihydroceramide. The molecular mechanism involved in C-4-hydroxylation has not been studied in detail. In the present paper, we report that C-4-hydroxylation requires an electron-transfer system that includes cytochrome b5 and that the hydroxylase activity is reconstituted in an in vitro assay with purified recombinant Des2. FLAG-tagged mouse Des2 was expressed in insect Sf9 cells and was purified by solubilization with digitonin and anti-FLAG antibody affinity column chromatography. The activity of dihydroceramide:sphinganine C-4-hydroxylase was reconstituted with the purified FLAG-Des2, mb5 (the membrane form of cytochrome b5) and bovine erythrocyte membrane. The apparent K(m) and V(max) of Des2 for the substrate N-octanoylsphinganine were 35 microM and 40 nmol x h(-1) x mg of protein(-1) respectively. The K(m) of the hydroxylase for mb5 was 0.8 microM. Interestingly, mb5 was not replaced with the soluble form of cytochrome b5, which lacks the C-terminal membrane-spanning domain. The erythrocyte membrane was separated into Triton X-100-soluble and -insoluble fractions, and the detergent-soluble fraction was replaced by the soluble or membrane form of b5R (NADH-cytochrome b5 reductase). The Triton-X-100-insoluble fraction contained trypsin-resistant factors. The Des2 protein is found in the endoplasmic reticulum and is assumed to have three membrane-spanning domains. The findings of the present study indicate that the hydroxylation requires complex formation between Des2 and mb5 via their membrane-spanning domains and electron transfer from NADH to the substrate via the reduction of mb5 by b5R.

摘要

Des2(退行性精母细胞2)是一种双功能酶,可从二氢神经酰胺生成植物神经酰胺和神经酰胺。尚未对参与C-4羟基化的分子机制进行详细研究。在本文中,我们报告C-4羟基化需要一个包括细胞色素b5的电子传递系统,并且在使用纯化的重组Des2进行的体外试验中可重建羟化酶活性。带有FLAG标签的小鼠Des2在昆虫Sf9细胞中表达,并通过用洋地黄皂苷溶解和抗FLAG抗体亲和柱色谱法进行纯化。用纯化的FLAG-Des2、mb5(细胞色素b5的膜形式)和牛红细胞膜重建二氢神经酰胺:鞘氨醇C-4羟化酶的活性。Des2对底物N-辛酰鞘氨醇的表观K(m)和V(max)分别为35 microM和40 nmol x h(-1) x mg蛋白质(-1)。羟化酶对mb5的K(m)为0.8 microM。有趣的是,mb5不能被缺乏C末端跨膜结构域的细胞色素b5的可溶性形式所替代。红细胞膜被分离为Triton X-100可溶性和不可溶性部分,去污剂可溶性部分被b5R(NADH-细胞色素b5还原酶)的可溶性或膜形式所替代。Triton-X-100不可溶性部分含有抗胰蛋白酶因子。Des2蛋白在内质网中发现,推测具有三个跨膜结构域。本研究结果表明,羟基化需要Des2和mb5通过其跨膜结构域形成复合物,并通过b5R将mb5还原,从而将电子从NADH转移到底物。

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