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西伯利亚仓鼠睾丸中促甲状腺激素释放激素(TRH)及TRH受体基因表达的检测

The detection of thyrotropin-releasing hormone (TRH) and TRH receptor gene expression in Siberian hamster testes.

作者信息

Rao J N, Debeljuk L, Bartke A, Gao Y P, Wilber J F, Feng P

机构信息

Department of Medicine, University of Maryland, School of Medicine, Baltimore 21201, USA.

出版信息

Peptides. 1997;18(8):1217-22. doi: 10.1016/s0196-9781(97)00183-6.

Abstract

Thyrotropin-releasing hormone (TRH) from the hypothalamus is the major regulator of TSH synthesis and secretion. Most recently, TRH and TRH receptors (TRH-R), as well as their mRNAs, have been identified in rat testis. To expand our knowledge on the testicular TRH and TRH receptor gene expression in different species, in the present study the mRNA levels of testicular TRH and TRH-R were investigated in Siberian hamsters. To further localize the cellular sites of the gene expression, the animal model was treated with a single injection of ethylene dimethane sulfonate (EDS) (i.p., 80 mg/kg body weight), a compound known as to specifically eliminate testicular Leydig cells. The elimination of Leydig cells induced by EDS treatment was confirmed by histological studies of the testis sections and by serum hormonal analyses, which showed a dramatic reduction of serum testosterone (T) levels and significantly elevated serum LH concentrations. Messenger RNA levels of TRH and TRH-R in the testes were determined by Northern blot analyses quantitated with densitometry scanning. The results showed that specific TRH-R mRNA, 3.8 kb in size, was identified in Siberian hamster testes and the mRNA levels were significantly elevated in the EDS-treated testes compared to the controls (p < 0.01). Testicular TRH mRNA was also detected; however, no significant differences in TRH mRNA levels were found between EDS-treated and control groups. The size of TRH mRNA was characterized as about 1.2 kb in hamster testes, which was smaller than that observed in the rat hypothalamus (1.6 kb) and in the rat testis (2.0 kb). Further studies by RNase H digestion revealed the presence of smaller TRH transcripts in the hamster testes than those in the rat testis. No hybridization signal for TRH mRNA was detected by RNase protection assay, when a rat TRH riboprobe was applied to hamster testis RNA, suggesting the limited homology of TRH gene sequences between these two species. Our results demonstrate that both TRH and TRH-R genes are expressed in Siberian hamster testes, and a significant increase of TRH-R mRNA levels occurs in the Leydig cell eliminated hamster testes. Unlike the rat testicular TRH mRNA mainly detected in Leydig cells, in hamster TRH mRNA could also be detected in other testicular compartment.

摘要

来自下丘脑的促甲状腺激素释放激素(TRH)是促甲状腺激素(TSH)合成和分泌的主要调节因子。最近,在大鼠睾丸中已鉴定出TRH及其受体(TRH-R)以及它们的mRNA。为了拓展我们对不同物种睾丸中TRH和TRH受体基因表达的认识,在本研究中,我们检测了西伯利亚仓鼠睾丸中TRH和TRH-R的mRNA水平。为了进一步定位基因表达的细胞位点,我们用单次腹腔注射乙烯二甲磺酸酯(EDS)(80 mg/kg体重)处理动物模型,EDS是一种已知能特异性消除睾丸间质细胞的化合物。通过对睾丸切片的组织学研究和血清激素分析证实了EDS处理诱导的间质细胞消除,结果显示血清睾酮(T)水平显著降低,血清促黄体生成素(LH)浓度显著升高。通过密度扫描定量的Northern印迹分析测定睾丸中TRH和TRH-R的mRNA水平。结果显示,在西伯利亚仓鼠睾丸中鉴定出大小为3.8 kb的特异性TRH-R mRNA,与对照组相比,EDS处理的睾丸中mRNA水平显著升高(p < 0.01)。也检测到了睾丸TRH mRNA;然而,EDS处理组和对照组之间的TRH mRNA水平没有显著差异。仓鼠睾丸中TRH mRNA的大小约为1.2 kb,小于在大鼠下丘脑(1.6 kb)和大鼠睾丸(2.0 kb)中观察到的大小。通过核糖核酸酶H消化的进一步研究表明,仓鼠睾丸中存在比大鼠睾丸中更小的TRH转录本。当用大鼠TRH核糖探针检测仓鼠睾丸RNA时,核糖核酸酶保护试验未检测到TRH mRNA的杂交信号,这表明这两个物种之间TRH基因序列的同源性有限。我们的结果表明,TRH和TRH-R基因在西伯利亚仓鼠睾丸中均有表达,并且在间质细胞消除的仓鼠睾丸中TRH-R mRNA水平显著增加。与主要在间质细胞中检测到的大鼠睾丸TRH mRNA不同,在仓鼠中,TRH mRNA也可在睾丸的其他区域检测到。

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