Rozhin J, Corombos J D, Horwitz J P, Brooks S C
J Steroid Biochem. 1986 Dec;25(6):973-9. doi: 10.1016/0022-4731(86)90331-6.
Steroid alcohol sulfotransferase (SAS) has been isolated from the cytosol of a human breast carcinoma cell line, MCF-7. This enzyme from Sephadex G-200 chromatography displayed a mol. wt of 118 KDa. The conditions for optimal enzymic activity of SAS were determined to be 20 min incubations at 45 degrees C in 0.2 M Tris buffer (pH 7.5) containing 0.06 M Mg2+. Chromatofocusing chromatography also yielded a single peak of SAS with a pI of 5.8. Results from the incubations of a series of androstane analogues revealed that SAS required a 3 beta-hydroxyl on a steroid with the trans bridge between the A and B rings. Neither the 3 beta-allylic hydroxyl group nor the A-ring phenolic 3-hydroxyl accepted the sulfate group from 3'-phosphoadenosine-5'-phosphosulfate. D-ring beta-hydroxyl groups were tolerated by the enzyme, however, alpha-hydroxyl groups on the D-ring appeared to interfere with the reaction. Sulfurylation of steroids by SAS was related inversely to the sum of the displacements of the 3-hydroxyl plus that of the 17-hydroxyl groups relative to the plane of symmetry of the dehydroepiandrosterone nucleus. This enzyme was also capable of sulfurylating short chain aliphatic alcohols, although at greatly reduced rates. 3 beta-Chloro-5-androstene-17-one and 2-nitroestradiol. 17 beta proved to be the best inhibitors of SAS.
类固醇醇磺基转移酶(SAS)已从人乳腺癌细胞系MCF-7的胞质溶胶中分离出来。经Sephadex G-200色谱分析,该酶的分子量为118 kDa。已确定SAS最佳酶活性的条件为:在含有0.06 M Mg2+的0.2 M Tris缓冲液(pH 7.5)中于45℃孵育20分钟。色谱聚焦层析也得到了一个单一的SAS峰,其pI为5.8。一系列雄甾烷类似物的孵育结果表明,SAS需要甾体上的3β-羟基以及A环和B环之间的反式桥。3β-烯丙基羟基和A环酚性3-羟基均不能从3'-磷酸腺苷-5'-磷酸硫酸酯接受硫酸基团。该酶可耐受D环β-羟基,然而,D环上的α-羟基似乎会干扰反应。SAS对类固醇的硫酸化作用与3-羟基和17-羟基相对于脱氢表雄酮核对称平面的位移总和呈负相关。该酶也能够硫酸化短链脂肪醇,尽管速率大大降低。3β-氯-5-雄烯-17-酮和17β-2-硝基雌二醇被证明是SAS的最佳抑制剂。
