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人血浆中的抑制素形式。

Inhibin forms in human plasma.

作者信息

Robertson D M, Sullivan J, Watson M, Cahir N

机构信息

Prince Henry's Institute of Medical Research, Monash Medical Centre, Clayton, Victoria, Australia.

出版信息

J Endocrinol. 1995 Feb;144(2):261-9. doi: 10.1677/joe.0.1440261.

Abstract

In order to identify the molecular weight forms of bioactive and immunoactive inhibin in human plasma, plasma/serum was sequentially fractionated by immunoaffinity chromatography (using immobilised inhibin alpha subunit antiserum), reversed phase HPLC and preparative SDS-PAGE. The electroeluted gel fractions were assayed for inhibin in vitro bioactivity and immunoactivity, the latter by RIA. Initial experiments examined human follicular fluid as an inhibin-rich source. Bioactive and immunoactive fractions of 30, 35, 53, 65 and approximately 120 kDa were identified in addition to bio-inactive, immunoactive fractions of 26 kDa and 32 kDa. These molecular weights correspond to those of known inhibin forms and are attributed to differing degrees of glycosylation of the inhibin alpha subunit and variable processing of the alpha and beta inhibin subunits. Fractionation of male plasma pools revealed the presence of higher molecular weight immunoactive forms (55-120 kDa) as well as 28-31 kDa forms although the molecular weight distribution of activity between pools varied. To assess if the molecular weight pattern was modified by storage and/or subsequent fractionation, protease inhibitors were added initially to plasma and fractionated as above. The molecular weight distribution of immunoactivity was largely unaffected by the treatment, indicating that minimal processing had occurred. Postmenopausal serum itself showed low to undetectable activity. The addition of recombinant human 31 kDa inhibin to postmenopausal serum resulted in a molecular weight profile of inhibin immunoactivity consistent with the presence of 31 kDa inhibin. Fractionation of a serum pool from women undergoing gonadotrophin stimulation, in which inhibin levels were elevated, showed a range of bioactive and immunoactive inhibin forms over the 30-120 kDa range.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

为了鉴定人血浆中生物活性和免疫活性抑制素的分子量形式,采用免疫亲和色谱法(使用固定化抑制素α亚基抗血清)、反相高效液相色谱法和制备性十二烷基硫酸钠-聚丙烯酰胺凝胶电泳对血浆/血清进行了连续分级分离。对电洗脱的凝胶级分进行体外生物活性和免疫活性检测,后者采用放射免疫分析。最初的实验以人卵泡液作为富含抑制素的来源。除了26 kDa和32 kDa的生物无活性、免疫活性级分之外,还鉴定出了30、35、53、65和大约120 kDa的生物活性和免疫活性级分。这些分子量与已知抑制素形式的分子量相对应,归因于抑制素α亚基糖基化程度的不同以及α和β抑制素亚基的可变加工。对男性血浆池的分级分离显示存在较高分子量的免疫活性形式(55 - 120 kDa)以及28 - 31 kDa的形式,尽管各血浆池之间活性的分子量分布有所不同。为了评估分子量模式是否因储存和/或后续分级分离而改变,最初向血浆中添加蛋白酶抑制剂并按上述方法进行分级分离。免疫活性的分子量分布在很大程度上不受该处理的影响,表明发生的加工极少。绝经后血清本身显示出低活性或无法检测到的活性。向绝经后血清中添加重组人31 kDa抑制素后,抑制素免疫活性的分子量谱与存在31 kDa抑制素一致。对接受促性腺激素刺激、抑制素水平升高的女性的血清池进行分级分离,结果显示在30 - 120 kDa范围内存在一系列生物活性和免疫活性抑制素形式。(摘要截断于250字)

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