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各类鱼鳞病皮肤活检中类固醇硫酸酯酶活性

Steroid sulphatase activity in the skin biopsies of various types of ichthyosis.

作者信息

Ruokonen A, Oikarinen A

出版信息

Br J Dermatol. 1981 Sep;105(3):291-5. doi: 10.1111/j.1365-2133.1981.tb01288.x.

Abstract

A simple method was developed for the determination of steroid sulphatase activity in a skin biopsy for routine use. In this method, 6 mg of minced tissue is incubated in 1 ml of Krebs-Ringer bicarbonate buffer with radioactive dehydroepiandrosterone sulphate (20,000 c.p.m., S.A. 1.1 Ci/mmol) for 4 h. After the incubation the liberated unconjugated dehydroepiandrosterone and its possible metabolites are separated from the conjugated compound by extraction with ethyl acetate-ethyl ether 10:90 (v/v). The organic phase is counted in a scintillation counter. The results are expressed as c.p.m. values per 6 mg tissue wet weight. Steroid sulphatase activity was measured in skin biopsies from nine control subjects and from thirteen patients with various types of ichthyosis. In the different groups studied, the ranges of the c.p.m. values were as follows: controls (n = 9) 377-1802; X-linked ichthyosis (n = 5) 140-214; ichthyosis vulgaris (n = 5) 607-1320; ichthyosiform erythroderma (n = 2) 2146-2214; lamellar ichthyosis (n = 1) 2185. The reagent blank varied from 180 to 259 c.p.m. In X-linked ichthyosis the c.p.m. values were always less than in the corresponding reagent blank, indicating that no enzyme activity was present in the tissue. In other types of ichthyosis, steroid sulphatase activity was normal. The method described is easy to accomplish in any clinical laboratory where scintillation counting is possible.

摘要

开发了一种用于常规皮肤活检中甾体硫酸酯酶活性测定的简单方法。在该方法中,将6mg切碎的组织在1ml含有放射性硫酸脱氢表雄酮(20,000 c.p.m.,比活度1.1 Ci/mmol)的 Krebs-Ringer 碳酸氢盐缓冲液中孵育4小时。孵育后,通过用10:90(v/v)的乙酸乙酯 - 乙醚萃取,将游离的未结合硫酸脱氢表雄酮及其可能的代谢产物与结合化合物分离。有机相在闪烁计数器中计数。结果以每6mg组织湿重的c.p.m.值表示。在9名对照受试者和13名患有各种鱼鳞病的患者的皮肤活检中测量了甾体硫酸酯酶活性。在所研究的不同组中,c.p.m.值范围如下:对照组(n = 9)377 - 1802;X连锁鱼鳞病(n = 5)140 - 214;寻常型鱼鳞病(n = 5)607 - 1320;鱼鳞病样红皮病(n = 2)2146 - 2214;板层状鱼鳞病(n = 1)2185。试剂空白在180至259 c.p.m.之间变化。在X连锁鱼鳞病中,c.p.m.值总是低于相应的试剂空白,表明组织中不存在酶活性。在其他类型的鱼鳞病中,甾体硫酸酯酶活性正常。所述方法在任何能够进行闪烁计数的临床实验室中都易于完成。

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