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内分泌类固醇硫酸转移酶:来自人乳腺癌细胞系MCF-7的类固醇醇硫酸转移酶。

Endocrine steroid sulfotransferases: steroid alcohol sulfotransferase from human breast carcinoma cell line MCF-7.

作者信息

Rozhin J, Corombos J D, Horwitz J P, Brooks S C

出版信息

J Steroid Biochem. 1986 Dec;25(6):973-9. doi: 10.1016/0022-4731(86)90331-6.

DOI:10.1016/0022-4731(86)90331-6
PMID:2948075
Abstract

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.

摘要

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。

相似文献

1
Endocrine steroid sulfotransferases: steroid alcohol sulfotransferase from human breast carcinoma cell line MCF-7.内分泌类固醇硫酸转移酶:来自人乳腺癌细胞系MCF-7的类固醇醇硫酸转移酶。
J Steroid Biochem. 1986 Dec;25(6):973-9. doi: 10.1016/0022-4731(86)90331-6.
2
Enzymatic sulfation of steroids. XVIII. study of the specific estradiol-17 beta sulfotransferase of rat liver cytosol, that converts the estrogen to its 3-sulfate, and some elements of the endocrine control of its production.类固醇的酶促硫酸化。十八。大鼠肝细胞溶胶中特异性雌二醇-17β硫酸转移酶的研究,该酶将雌激素转化为其3-硫酸盐,以及其产生的内分泌控制的一些要素。
Can J Biochem Cell Biol. 1983 Jan;61(1):15-22. doi: 10.1139/o83-003.
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Testicular steroid sulfotransferases: comparison to liver and adrenal steroid sulfotransferases of the mature rat.睾丸类固醇硫酸转移酶:与成熟大鼠肝脏和肾上腺类固醇硫酸转移酶的比较。
Endocrinology. 1980 May;106(5):1365-70. doi: 10.1210/endo-106-5-1365.
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Endocrine steroid sulfotransferases: porcine endometrial estrogen sulfotransferase.内分泌类固醇硫酸转移酶:猪子宫内膜雌激素硫酸转移酶
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Steroid sulfotransferase in hamster epididymis.仓鼠附睾中的类固醇硫酸转移酶。
Steroids. 1981 Nov;38(5):523-35. doi: 10.1016/0039-128x(81)90052-0.
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Partial characterization of steroid sulfohydrolase and steroid sulfotransferase activities in purified porcine Leydig cells.纯化猪睾丸间质细胞中类固醇硫酸酯酶和类固醇磺基转移酶活性的部分特性分析。
J Steroid Biochem. 1989 Mar;32(3):387-92. doi: 10.1016/0022-4731(89)90211-2.
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Enzymic synthesis of steroid sulfates XVI. Specificity and regulation of human adrenal hydroxysteroid sulfotransferase.甾体硫酸盐的酶促合成XVI. 人肾上腺羟类固醇硫酸转移酶的特异性与调节
Steroids. 1983 May;41(5):575-86. doi: 10.1016/0039-128x(83)90023-5.
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Enzymic synthesis of steroid sulphates. XIV. Properties of human adrenal steroid alcohol sulphotransferase.
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The assay and partial characterization of 3 beta-hydroxysteroid sulfotransferase of the hamster epididymis.仓鼠附睾3β-羟基类固醇硫酸转移酶的测定及部分特性分析。
Can J Biochem Cell Biol. 1985 Jan;63(1):71-6. doi: 10.1139/o85-010.
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Dehydroepiandrosterone sulfotransferase as a possible shunt for the control of steroid metabolism in human mammary carcinoma.硫酸脱氢表雄酮磺基转移酶作为控制人乳腺癌中类固醇代谢的一种可能分流途径。
Cancer Res. 1977 Jan;37(1):278-84.

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