绵羊膜孕激素受体α的结合特性及发情周期中该受体的表达

Binding characteristics of the ovine membrane progesterone receptor alpha and expression of the receptor during the estrous cycle.

作者信息

Ashley Ryan L, Arreguin-Arevalo J Alejandro, Nett Terry M

机构信息

Department of Biomedical Sciences, Animal Reproduction and Biotechnology Laboratory, Colorado State University, Colorado, USA.

出版信息

Reprod Biol Endocrinol. 2009 May 11;7:42. doi: 10.1186/1477-7827-7-42.

DOI:10.1186/1477-7827-7-42

PMID:19432978

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2685384/

Abstract

BACKGROUND

Classically, progesterone has been thought to act only through the well-known genomic pathway involving hormone binding to nuclear receptors and subsequent modulation of gene expression. However, there is increasing evidence for rapid, non-genomic effects of progesterone in a variety of mammalian tissues and it is possible that a membrane PR (mPR) is causing these events. We recently isolated and characterized an ovine mPR referred to as mPR-alpha, distinct from the nuclear PR. Based on predicted structural analysis, the ovine mPR-alpha possesses seven transmembrane domains typical of G protein-coupled receptors. Despite the homology to other reported mPRs, information pertaining to the steroid binding characteristics of the ovine mPR-alpha was lacking. Additionally, the ovine mPR-alpha transcript has been identified in the hypothalamus, pituitary, uterus, ovary and corpus luteum, yet changes in expression of the ovine mPR-alpha in these tissues were not known. Consequently, the purpose of this work was to determine the steroid binding characteristics of the ovine mPR-alpha and to investigate possible changes in expression of the ovine mPR-alpha in reproductive tissues throughout the estrous cycle.

METHODS

Binding studies were performed using crude membrane fractions from CHO cells expressing the mPR-alpha. Using quantitative Real-time PCR we determined the expression pattern of mRNA for the ovine mPR-alpha during the ovine estrous cycle in tissues known to express the mPR-alpha. Jugular blood samples were also collected and analyzed for serum concentrations of P4 to ensure ewes were at the appropriate stage of their cycle.

RESULTS

Only progesterone, 20alpha-hydroxyprogesterone and 17alpha-hydroxyprogesterone were able to displace binding of 3H-P4 (P < 0.001) to membrane fractions from CHO cells expressing ovine mPR-alpha. The average B-max and Kd values for three separate experiments were 624 +/- 119 fmol/micro gram protein and 122 +/- 50 nM, respectively. Significant changes in expression of mRNA for the mPR-alpha during the estrous cycle were noted in the corpus luteum and uterus.

CONCLUSION

The mPR-alpha specifically binds progestins and its expression was correlated to progesterone secretion during the ovine estrous cycle. Results from the present studies suggest that mPR-alpha may have an important physiological role during the ovine estrous cycle.

摘要

背景

传统上，人们认为孕酮仅通过众所周知的基因组途径发挥作用，即激素与核受体结合，随后调节基因表达。然而，越来越多的证据表明，孕酮在多种哺乳动物组织中具有快速的非基因组效应，并且可能是一种膜孕激素受体（mPR）引发了这些事件。我们最近分离并鉴定了一种绵羊mPR，称为mPR-α，它与核孕激素受体不同。基于预测的结构分析，绵羊mPR-α具有典型的G蛋白偶联受体的七个跨膜结构域。尽管与其他已报道的mPR具有同源性，但缺乏有关绵羊mPR-α类固醇结合特性的信息。此外，已在绵羊下丘脑、垂体、子宫、卵巢和黄体中鉴定出绵羊mPR-α转录本，但这些组织中绵羊mPR-α表达的变化尚不清楚。因此，本研究的目的是确定绵羊mPR-α的类固醇结合特性，并研究整个发情周期中生殖组织中绵羊mPR-α表达的可能变化。

方法

使用表达mPR-α的CHO细胞的粗膜部分进行结合研究。我们通过定量实时PCR确定了已知表达mPR-α的组织中绵羊发情周期内绵羊mPR-α mRNA的表达模式。还采集了颈静脉血样并分析了血清P4浓度，以确保母羊处于其周期的适当阶段。

结果

只有孕酮、20α-羟孕酮和17α-羟孕酮能够取代3H-P4（P < 0.001）与表达绵羊mPR-α的CHO细胞膜部分的结合。三个独立实验的平均B-max和Kd值分别为624 +/- 119 fmol/微克蛋白质和122 +/- 50 nM。在黄体和子宫中，发情周期中mPR-α mRNA的表达有显著变化。

结论

mPR-α特异性结合孕激素，其表达与绵羊发情周期中的孕酮分泌相关。本研究结果表明，mPR-α在绵羊发情周期中可能具有重要的生理作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/884b/2685384/7ef1ed57d39a/1477-7827-7-42-1.jpg

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绵羊膜孕激素受体α的结合特性及发情周期中该受体的表达

Binding characteristics of the ovine membrane progesterone receptor alpha and expression of the receptor during the estrous cycle.

作者信息

Ashley Ryan L, Arreguin-Arevalo J Alejandro, Nett Terry M

机构信息

Department of Biomedical Sciences, Animal Reproduction and Biotechnology Laboratory, Colorado State University, Colorado, USA.