Hardy D O, Ge R S, Catterall J F, Hou Y T, Penning T M, Hardy M P
Population Council and The Rockefeller University, New York, New York 10021, USA.
Endocrinology. 2000 May;141(5):1608-17. doi: 10.1210/endo.141.5.7445.
Dihydrotestosterone (DHT) is the most potent naturally occurring androgen, and its production in the testis may have important consequences in developmental and reproductive processes. In the rat testis, three factors can contribute to intracellular DHT levels: 1) synthesis of DHT from T by 5alpha-reductase, 2) conversion of DHT to 5alpha-androstane-3alpha, 17beta-diol (3alpha-DIOL) by the reductive activity of 3alpha-hydroxysteroid dehydrogenase (3alpha-HSD), and 3) conversion of 3alpha-DIOL by an oxidative 3alpha-HSD activity. While the type I 3alpha-HSD enzyme (3alpha-HSD1 or AKR1C9) is an oxidoreductase in vitro and could theoretically be responsible for factors 2 and 3, we have shown previously that rat Leydig cells have two 3alpha-HSD activities: a cytosolic NADP(H)- dependent activity, characteristic of 3alpha-HSD1, and a microsomal NAD(H)-dependent activity. The two activities were separable by both developmental and biochemical criteria, but the identity of the second enzyme was unknown. To identify the microsomal NAD(H)-dependent 3alpha-HSD in rat Leydig cells, degenerate primers were used to amplify a number of short-chain alcohol dehydrogenases. Sequence analysis of cloned PCR products identified retinol dehydrogenase type II (RoDH2) as the prevalent species in purified Leydig cells. RoDH2 cDNA was subcloned into expression vectors and transiently transfected into CHOP and COS-1 cells. Its properties were compared with transiently transfected 3alpha-HSD1. When measured in intact CHOP and COS-1 cells, RoDH2 cDNA produced a protein that catalyzed the conversions of 3alpha-DIOL to DHT and androsterone to androstanedione, but not the reverse reactions. Therefore, the 3alpha-HSD activity of RoDH2 was exclusively oxidative. In contrast, type I 3alpha-HSD cDNA produced a protein that was exclusively a 3alpha-HSD reductase. In cell homogenates and subcellular fractions, RoDH2 catalyzed both 3alpha-HSD oxidation and reduction reactions that were NAD(H) dependent, and the enzyme activities were located in the microsomes. Type I 3alpha-HSD also catalyzed both oxidation and reduction, but was located in the cytosol and was NADP(H) dependent. We conclude that type I 3alpha-HSD and RoDH2 have distinct 3alpha-HSD activities with opposing catalytic directions, thereby controlling the rates of DHT production by Leydig cells.
双氢睾酮(DHT)是最具活性的天然雄激素,其在睾丸中的产生可能对发育和生殖过程产生重要影响。在大鼠睾丸中,有三个因素可影响细胞内DHT水平:1)5α-还原酶将睾酮转化为DHT;2)3α-羟基类固醇脱氢酶(3α-HSD)的还原活性将DHT转化为5α-雄烷-3α,17β-二醇(3α-DIOL);3)氧化型3α-HSD活性将3α-DIOL进行转化。虽然I型3α-HSD酶(3α-HSD1或AKR1C9)在体外是一种氧化还原酶,理论上可能与因素2和3有关,但我们之前已经表明,大鼠睾丸间质细胞有两种3α-HSD活性:一种是胞质NADP(H)依赖性活性,是3α-HSD1的特征,另一种是微粒体NAD(H)依赖性活性。这两种活性在发育和生化标准上都是可分离的,但第二种酶的身份尚不清楚。为了鉴定大鼠睾丸间质细胞中微粒体NAD(H)依赖性3α-HSD,使用简并引物扩增了一些短链醇脱氢酶。对克隆的PCR产物进行序列分析,确定II型视黄醇脱氢酶(RoDH2)是纯化的睾丸间质细胞中的主要类型。将RoDH2 cDNA亚克隆到表达载体中,并瞬时转染到CHOP和COS-1细胞中。将其特性与瞬时转染的3α-HSD1进行比较。在完整的CHOP和COS-1细胞中检测时,RoDH2 cDNA产生一种蛋白质,该蛋白质催化3α-DIOL向DHT以及雄酮向雄烷二酮的转化,但不催化反向反应。因此,RoDH2的3α-HSD活性完全是氧化性的。相比之下,I型3α-HSD cDNA产生的蛋白质完全是一种3α-HSD还原酶。在细胞匀浆和亚细胞组分中,RoDH2催化NAD(H)依赖性的3α-HSD氧化和还原反应,且酶活性位于微粒体中。I型3α-HSD也催化氧化和还原反应,但位于胞质中,且是NADP(H)依赖性的。我们得出结论,I型3α-HSD和RoDH具有不同的3α-HSD活性,催化方向相反,从而控制睾丸间质细胞产生DHT的速率。
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