猪和人的羰基还原酶参与了表雄酮、11-氧代类固醇、神经类固醇和皮质类固醇的代谢。

IF 4.6 Q2 MATERIALS SCIENCE, BIOMATERIALS

ACS Applied Bio Materials Pub Date : 2024-06-28 DOI:10.1016/j.jsbmb.2024.106574

Satoshi Endo , Yoshifumi Morikawa , Koichi Suenami , Yuji Sakai , Naohito Abe , Toshiyuki Matsunaga , Akira Hara , Masaki Takasu

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引用次数: 0

摘要

猪羰基还原酶（pCBR1 和 pCBR-N1）和醛酮还原酶（pAKR1C1 和 pAKR1C4）具有羟类固醇脱氢酶（HSD）活性。然而，它们在孔雀特异性雄激素（19-去甲睾酮和表雄酮）、11-氧代雄激素、神经类固醇和皮质类固醇的代谢中的作用仍不清楚。在这里，我们通过动力学和产物分析比较了四种重组酶的类固醇特异性。在C18/C19-类固醇中，11-酮和11β-羟基-5α-雄甾烷-3,17-二酮被所有酶还原，而5α-二氢诺龙（19-去甲睾酮代谢物）和11-酮二氢睾酮被pCBR1、pCBR-N1和pAKR1C1还原，其中pCBR1的Km值最低（亚微摩尔）。产物分析表明，pCBR1 和 pCBR-N1 作为 3α/β-HSD 起作用，而 pAKR1C1 和 pAKR1C4 则不同（分别作为 3β-HSD 和 3α-HSD）。此外，在 pCBR1 和 pCBR-N1（针对表雄酮及其 11 氧衍生物）以及 pAKR1C1（针对雄甾酮、4-雄烯-3,17-二酮及其 11 氧衍生物）中观察到了 17β-HSD 活性。这四种酶对 3-酮-5α/β-二氢-C21-类固醇（包括 GABA 能神经类固醇前体和皮质类固醇代谢物）也表现出不同的底物特异性。所有酶都能减少 5β-二氢黄体酮，而只有 pCBR1 能减少 5α-二氢黄体酮，pCBR1 和 pCBR-N1 能减少 5α/β-二氢脱氧皮质酮。pCBR1 对 3-酮-C21-类固醇的 Km 值（0.3-2.9μM）低于 pCBR-N1（Km=10-36μM）。pCBR1 和 pCBR-N1 对 3-酮-C21-类固醇的还原产物是它们的 3α-羟基代谢物。最后，我们发现人 CBR1 对 C18/C19/C21 类固醇的底物特异性与 pCBR-N1 相似。基于这些结果，我们得出结论：猪和人的 CBR 可作为 3α/β,17β-HSD，参与上述类固醇的代谢。

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Involvement of porcine and human carbonyl reductases in the metabolism of epiandrosterone, 11-oxygenated steroids, neurosteroids, and corticosteroids

Porcine carbonyl reductases (pCBR1 and pCBR-N1) and aldo-keto reductases (pAKR1C1 and pAKR1C4) exhibit hydroxysteroid dehydrogenase (HSD) activity. However, their roles in the metabolism of porcine-specific androgens (19-nortestosterone and epiandrosterone), 11-oxygenated androgens, neurosteroids, and corticosteroids remain unclear. Here, we compared the steroid specificity of the four recombinant enzymes by kinetic and product analyses. In C₁₈/C₁₉-steroids,11-keto- and 11β-hydroxy-5α-androstane-3,17-diones were reduced by all the enzymes, whereas 5α-dihydronandrolone (19-nortestosterone metabolite) and 11-ketodihydrotestosterone were reduced by pCBR1, pCBR-N1, and pAKR1C1, of which pCBR1 exhibited the lowest (submicromolar) K_m values. Product analysis showed that pCBR1 and pCBR-N1 function as 3α/β-HSDs, in contrast to pAKR1C1 and pAKR1C4 (acting as 3β-HSD and 3α-HSD, respectively). Additionally, 17β-HSD activity was observed in pCBR1 and pCBR-N1 (toward epiandrosterone and its 11-oxygenated derivatives) and in pAKR1C1 (toward androsterone, 4-androstene-3,17-dione and their 11-oxygenated derivatives). The four enzymes also showed different substrate specificity for 3-keto-5α/β-dihydro-C₂₁-steroids, including GABAergic neurosteroid precursors and corticosteroid metabolites. 5β-Dihydroprogesterone was reduced by all the enzymes, whereas 5α-dihydroprogesterone was reduced only by pCBR1, and 5α/β-dihydrodeoxycorticosterones by pCBR1 and pCBR-N1. The two pCBRs also reduced the 5α/β-dihydro-metabolites of cortisol, 11-deoxycortisol, cortisone, and corticosterone. pCBR1 exhibited lower K_m values (0.3–2.9 μM) for the 3-keto-C₂₁-steroids than pCBR-N1 (K_m=10–36 μM). The reduced products of the 3-keto-C₂₁-steroids by pCBR1 and pCBR-N1 were their 3α-hydroxy-metabolites. Finally, we found that human CBR1 has similar substrate specificity for the C₁₈/C₁₉/C₂₁-steroids to pCBR-N1. Based on these results, it was concluded that porcine and human CBRs can be involved in the metabolism of the aforementioned steroids as 3α/β,17β-HSDs.

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来源期刊

ACS Applied Bio Materials Chemistry-Chemistry (all)

CiteScore

9.40

自引率

2.10%

发文量

464