首页> 外文学位 >Characterization of anti-Mullerian Hormone in the Stallion and Mare: Changes During Testis Development and Determination of Serum Concentrations in Normal Mares, Pregnant Mares and Mares with Granulosa-cell Tumors.
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Characterization of anti-Mullerian Hormone in the Stallion and Mare: Changes During Testis Development and Determination of Serum Concentrations in Normal Mares, Pregnant Mares and Mares with Granulosa-cell Tumors.

机译:种马和母马中抗穆勒激素的特性:睾丸发育过程中的变化以及正常母马,孕妇母马和具有颗粒细胞瘤的母马的血清浓度测定。

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摘要

Anti-Mullerian hormone (AMH) is a dimeric glycoprotein, member of the transforming growth factor beta superfamily of growth and differentiation factors. During sexual differentiation, testosterone is responsible for Wolffian (mesonephric) duct development in males while AMH is required for Mullerian (paramesonephric) duct regression. AMH is produced from the time of differentiation of seminiferous tubules in the fetal testis until pubertal maturation and appears to regulate Leydig cell differentiation and testosterone secretion. In females, AMH is not expressed before the time of birth, guaranteeing normal differentiation of the female genital tract. After birth, AMH is expressed in granulosa cells of preantral and small antral follicles in the ovary and has been related to inhibition of recruitment of primordial follicles into the pool of growing follicles. In addition, circulating AMH concentrations have been used for monitoring granulosa-cell tumor (GCT) in women.;In chapter 1 and 2, changes in expression of anti-Mullerian hormone (AMH) and its receptor (AMHR2), androgen receptor (AR), cyclin-dependent kinase inhibitor (CDKN1B), connexin 43 (Cx43), 3beta hydroxysteroid dehydrogenase/Delta 5-Delta4- isomerase (3betaHSD), 17alpha-hydroxylase/17,20-lyase (P450c17) and aromatase cytochrome P450 (P450arom) in testes of normal stallions throughout puberty were characterized based upon immunohistochemistry (IHC) and real-time quantitative PCR (RT-qPCR). In chapter 3, the same markers were characterized in undescended testes of cryptorchid stallions and compared with testes of normal stallions. In chapter 4, a specific enzyme immunoassay from Immunotech-Beckman Coulter was validated for determination of serum AMH in the horse and for determination of concentrations of AMH in the blood of mares during the estrous cycle and pregnancy as well in mares with granulosa cell tumors.;During testis development in the stallion, AMH expression decreased with age and was accompanied by increased AR and CDKN1B expression in Sertoli cells coinciding with the final stages of Sertoli cell maturation and AMH regulation by testosterone. In addition, expression and distribution of Cx43 changed throughout development, suggesting a role of Cx43 in the Sertoli cell signaling and maturation, hormone secretion and blood-testis barrier formation. As expected, P450c17 and 3betaHSD immunolabeling and mRNA expression increased with age. 3betaHSD was also observed within the seminiferous tubules (presumptive Sertoli cells) of prepubertal testes and disappeared in the postpubertal testes. P450arom was absent or weakly expressed in immature Leydig cells of prepubertal testes and increased in the postpubertal and adult testis. In cryptorchid testes, AMH and AMHR2 immunoexpression was increased compared to normal testes. The persistence of high AMH expression accompanied by low AR expression in Sertoli cells of cryptorchid testes indicates failure of maturation of Sertoli cells and/or lack of testosterone suppression. The steroidogenic enzymes P450arom, P450c17 and 3betaHSD showed lower immunolabeling in the cryptorchid testes, which is also consistent with an underdeveloped testis. In addition, Cx43 expression is decreased in the cryptorchid testis, indicating disruption in intercellular communication.;In chapter 4, ovariectomized mares showed AMH concentrations at or below the limit of detection for the assay. AMH concentrations were higher in cycling and pregnant mares when compared to ovariectomized mares and did not change significantly throughout estrous cycle or pregnancy. Mares with granulosa-cell tumor showed an increase in AMH concentrations, when compared to normal cycling mares, pregnant mares and ovariectomized mares. A decrease of approximately 50% in AMH concentration was observed after 48 hours of tumor removal. These data indicate that AMH is expressed in equine GCTs and that serum levels are a useful biomarker for their diagnosis.
机译:抗穆勒氏激素(AMH)是一种二聚体糖蛋白,是生长和分化因子的转化生长因子β超家族的成员。在性别分化期间,睾丸激素负责男性的Wolffian(中肾)导管发育,而AMH是Mullerian(中肾上肾)导管退化所必需的。从胎睾丸中的生精小管分化到青春期成熟,就会产生AMH,并且它似乎在调节Leydig细胞分化和睾丸激素的分泌。在女性中,AMH在出生前不表达,从而保证了女性生殖道的正常分化。出生后,AMH在卵巢的前窦卵泡和小窦卵泡的颗粒细胞中表达,并且与抑制原始卵泡募集到生长的卵泡池中有关。此外,循环中的AMH浓度已用于监测女性的颗粒细胞瘤(GCT)。;在第1章和第2章中,抗穆勒激素(AMH)及其受体(AMHR2)和雄激素受体(AR)的表达变化),细胞周期蛋白依赖性激酶抑制剂(CDKN1B),连接蛋白43(Cx43),3beta羟基类固醇脱氢酶/ Delta 5-Delta4-异构酶(3betaHSD),17alpha-羟化酶/ 17,20-裂合酶(P450c17)和芳香酶细胞色素P450(P450arom)基于免疫组化(IHC)和实时定量PCR(RT-qPCR)对整个青春期睾丸中的雌性进行了表征。在第三章中,相同的标记物在隐睾种马的未降睾丸中进行了表征,并与正常种马的睾丸进行了比较。在第4章中,对Immunotech-Beckman Coulter的一种特异性酶免疫测定法进行了验证,该测定法可用于测定马中的血清AMH以及测定发情周期和妊娠期间母马血液中的AMH浓度,以及具有颗粒细胞瘤的母马。 ;在种马睾丸发育期间,AMH表达随年龄下降,并伴有Sertoli细胞AR和CDKN1B表达增加,这与Sertoli细胞成熟的最后阶段和睾丸激素对AMH的调节相吻合。此外,Cx43的表达和分布在整个发育过程中都发生了变化,表明Cx43在支持细胞的信号传导和成熟,激素分泌和血液睾丸屏障形成中发挥了作用。如预期的那样,P450c17和3betaHSD免疫标记和mRNA表达随年龄增长而增加。在青春期前睾丸的生精小管(推测的支持细胞)中也观察到了3betaHSD,在青春期后睾丸中消失了。 P450arom在青春期前睾丸的未成熟Leydig细胞中不存在或表达较弱,而在青春期后和成人睾丸中则有所增加。在隐睾睾丸中,与正常睾丸相比,AMH和AMHR2免疫表达增加。在隐睾睾丸支持细胞中,高AMH表达持续存在,而AR表达却较低,这表明支持细胞成熟失败和/或睾丸激素缺乏抑制。类固醇生成酶P450arom,P450c17和3betaHSD在隐睾睾丸中显示出较低的免疫标记,这也与睾丸发育不足相一致。此外,隐睾睾丸中的Cx43表达降低,表明细胞间通讯受到破坏。在第4章中,去卵巢母马的AMH浓度达到或低于检测限。与卵巢切除的母马相比,​​骑自行车和母马中的AMH浓度更高,并且在整个发情周期或妊娠中并未发生明显变化。与正常自行车母马,怀孕母马和去卵巢母马相比,​​患有颗粒细胞瘤的母马显示AMH浓度增加。去除肿瘤48小时后,观察到AMH浓度降低了约50%。这些数据表明AMH在马GCT中表达,并且血清水平是对其诊断有用的生物标志物。

著录项

  • 作者

    Almeida, Juliana Lopes.;

  • 作者单位

    University of California, Davis.;

  • 授予单位 University of California, Davis.;
  • 学科 Agriculture Animal Pathology.;Biology Physiology.;Biology Veterinary Science.
  • 学位 Ph.D.
  • 年度 2010
  • 页码 194 p.
  • 总页数 194
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

  • 入库时间 2022-08-17 11:45:36

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