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A specific immunoassay for proAMH, the uncleaved proprotein precursor of anti-Mallerian hormone

机译:促胰腺的特定免疫测定,抗Mallerian激素的未切割的ProProtein前体

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The utility of serum anti-Mtillerian hormone (AMH) assays in assessment of female fertility have been investigated extensively but little is known about the biological activity of the hormone being studied. ProAMH is the proprotein precursor and is incapable of binding to the AMH-specific type II receptor. Proteolytic cleavage generates receptor-competent AMHN,c which is a non-covalent complex of the N- and C-terminal cleavage fragments. Commercially available AMH assays do not differentiate the two forms of AMH. Techniques were developed to dissociate the AMH(N,C) complex and abolish its two-site immunoassay immunoreactivity. This allowed specific quantification of proAMH. The surfactant sodium deoxycholate (DOC) dissociated AMHN,c without disrupting binding of proAMH to the capture antibody with an optimal concentration of 0.1-0.2%wiv. The incorporation of a DOC incubation step into the AMH Gen II ELISA detected proAMH, with AMHN,c cross-detection conservatively estimated at 6.0% +/- 2.5% (mean +/- S.D.). The intra-assay and inter-assay variability were estimated at 8.0%CV and 13.0% CV respectively. The levels of proAMH and total AMH were assessed in 5 boys and 5 men and the proportion of proAMH was found to be significantly higher in boys (p = 0.005). This study will facilitate further investigation of the role of proteolytic cleavage in AMH signalling. (C) 2015 Elsevier Ireland Ltd. All rights reserved.
机译:血清抗mtillerian激素(AMH)测定评估的血清抗mtillerian激素(AMH)测定的效用已经广泛研究,但关于所研究的激素的生物活性很少。 ProAMH是ProProtein前体,并且不能与AMH特异性II型受体结合。蛋白水解裂解产生受体 - 竞争力的AMHN,C是N-和C-末端切割片段的非共价络合物。市售的AMH测定不会区分两种形式的AMH。开发了技术以解离AMH(N,C)复合物并取消其双位免疫测定免疫反应性。这允许ProAMH的特定量化。表面活性剂脱氧胆酸钠(DOC)解离AMHN,C不破坏PROMH与捕获抗体的结合,最佳浓度为0.1-0.2%WIV。将DOC孵育步骤掺入AMH Gen II ELISA检测到的ProAMH,C型交叉检测保守估计为6.0%+/- 2.5%(平均+/- S.D.)。测定内和测定间变异性分别估计为8.0%CV和13.0%CV。在5个男孩和5名男性中评估了ProAMH和总AMH的水平,男孩的比例明显高(P = 0.005)。该研究将促进进一步调查蛋白水解裂解在AMH信号传导中的作用。 (c)2015 Elsevier Ireland Ltd.保留所有权利。

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