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人良性前列腺增生中的硫酸类固醇硫酸酯酶:上皮和基质中该酶的特性与定量分析

Steroid sulfate sulfatase in human benign prostatic hyperplasia: characterization and quantification of the enzyme in epithelium and stroma.

作者信息

Klein H, Molwitz T, Bartsch W

机构信息

Dept of Clinical Chemistry, University of Hamburg, F.R.G.

出版信息

J Steroid Biochem. 1989 Aug;33(2):195-200. doi: 10.1016/0022-4731(89)90294-x.

Abstract

Characteristics and activities of estrone sulfate (E1S) and dehydroepiandrosterone sulfate (DHAS) sulfatases were studied in epithelium and stroma of benign hyperplastic tissues from human prostates. Tissues were obtained by suprapubic prostatectomy, and epithelium and stroma were separated mechanically by standard techniques. The assay procedure comprised homogenization in Tris-buffer, incubation of the homogenate with [3H]E1S or [3H]DHAS, separation of free steroids from nonhydrolyzed steroid sulfates by extraction with ether, and their final quantification by LSC. The main results were: (1) The pH-optimum of the sulfatase was found at pH 7.0. (2) The highest specific sulfatase activity was found in the epithelium and was associated with its nuclear fraction. (3) Michaelis-Menten constants Km (microM) were 8.7 +/- 1.4 (7) and 4.3 +/- 0.8 (5), maximum velocity rates Vmax (nmol/h x mgDNA) were 47.4 +/- 8.8 (7) and 8.4 +/- 1.5 (5) for E1S and DHAS, respectively (means +/- SEM (n]. (4) The enzymatic cleavage of E1-sulfate was competitively inhibited by DHA-sulfate and vice versa with inhibition constants Ki (microM) of 4.0 +/- 0.5 (2) for E1S and 2.7 +/- 0.4 (2) for DHAS. On the basis of these findings, possible roles of steroid sulfate-sulfatases in forming precursors of active androgens and estrogens from the high amounts of E1S and DHAS in blood are discussed.

摘要

对硫酸雌酮(E1S)和硫酸脱氢表雄酮(DHAS)硫酸酯酶的特性及活性,在人前列腺良性增生组织的上皮和基质中进行了研究。组织通过耻骨上前列腺切除术获取,上皮和基质采用标准技术机械分离。检测步骤包括在Tris缓冲液中匀浆,匀浆液与[3H]E1S或[3H]DHAS孵育,用乙醚萃取将游离类固醇与未水解的类固醇硫酸盐分离,最后通过液体闪烁计数法进行定量。主要结果如下:(1)发现硫酸酯酶的最适pH值为7.0。(2)上皮中硫酸酯酶的比活性最高,且与其核部分相关。(3)对于E1S和DHAS,米氏常数Km(μM)分别为8.7±1.4(7)和4.3±0.8(5),最大反应速度Vmax(nmol/h×mgDNA)分别为47.4±8.8(7)和8.4±1.5(5)(均值±标准误[n])。(4)硫酸脱氢表雄酮对E1 - 硫酸盐的酶促裂解有竞争性抑制作用,反之亦然,E1S的抑制常数Ki(μM)为4.0±0.5(2),DHAS为2.7±0.4(2)。基于这些发现,讨论了类固醇硫酸盐 - 硫酸酯酶在从血液中大量的E1S和DHAS形成活性雄激素和雌激素前体中的可能作用。

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