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卵泡调节蛋白的生化及生理学特性:卵泡发生的旁分泌调节因子

Biochemical and physiologic characterization of follicle regulatory protein: a paracrine regulator of folliculogenesis.

作者信息

Ono T, Campeau J D, Holmberg E A, Nakamura R M, Ujita E L, Devereaux D L, Tonetta S A, DeVinna R, Ugalde M, diZerega G S

出版信息

Am J Obstet Gynecol. 1986 Apr;154(4):709-16. doi: 10.1016/0002-9378(86)90441-2.

Abstract

Further purification of a porcine follicular fluid fraction, referred to as follicle regulatory protein, that inhibits granulosa cell aromatase was performed and the results of in vitro bioassays with these highly purified reagents are reported. The 0% to 35% saturated ammonium sulfate extract of porcine follicular fluid was percolated through an orange A dye matrex gel column and the bound fraction was eluted. Further purification of 0% to 35% orange A-bound fraction of porcine follicular fluid was performed by anion exchange chromatography with the use of the Mono Q column. Mono Q eluents containing follicle regulatory protein activity were injected onto a Mono P hydrogen ion-exchange column. Samples obtained from Mono P chromatography were injected onto preparative and analytical scale gel exclusion columns. Eluent fractions in the apparent molecular weight of 16,000 daltons were tested for aromatase inhibition. Throughout each step, parallelism of an aromatase inhibitor was apparent in both a cell-free microsomal assay and a granulosa cell assay. Follicle regulatory protein, purified about 6666-fold from the orange A-bound fraction of porcine follicular fluid, had a 50% inhibitory concentration of 25 ng/ml for granulosa cell aromatase activity.

摘要

对一种被称为卵泡调节蛋白的猪卵泡液组分进行了进一步纯化,该蛋白可抑制颗粒细胞芳香化酶,并报告了使用这些高度纯化试剂进行的体外生物测定结果。将猪卵泡液0%至35%饱和度的硫酸铵提取物通过橙A染料基质凝胶柱进行渗滤,并洗脱结合部分。使用Mono Q柱通过阴离子交换色谱法对猪卵泡液0%至35%橙A结合部分进行进一步纯化。将含有卵泡调节蛋白活性的Mono Q洗脱液注入Mono P氢离子交换柱。从Mono P色谱法获得的样品注入制备型和分析型凝胶排阻柱。对表观分子量为16,000道尔顿的洗脱液组分进行芳香化酶抑制测试。在每个步骤中,在无细胞微粒体测定和颗粒细胞测定中,芳香化酶抑制剂的平行性都很明显。从猪卵泡液橙A结合部分纯化约6666倍的卵泡调节蛋白对颗粒细胞芳香化酶活性的50%抑制浓度为25 ng/ml。

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