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Characterization of truncated testis-specific prolactin receptors in the chicken (Gallus domestics).

机译:鸡(家蝇)截短的睾丸特异性催乳素受体的特征。

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摘要

We have characterized two unique isoforms of truncated testis-specific (TTS) chicken prolactin receptor (cPRLR) transcripts in the domestic chicken. These two TTS cPRLR isoforms, which correspond to only the intracellular domain of the full-length cPRLR cDNA, are expressed at high levels in the sexually mature chicken. The most predominant TTS cPRLR mRNA contains the Box 1 motif [(+) Box 1 TTS], while the other transcript [(−) Box 1 TTS] contains a unique sequence that replaces the Box 1 motif. Two testes specific exons (TSE 1 and 2) are embedded in introns 8 and 9 of the cPRLR gene. These TSE are alternatively spliced to give rise to four different 5-untranslated regions (5-UTR) that are found in (+) Box 1 cPRLR transcripts and to the unique 5-end of the (−) Box 1 cPRLR mRNA. An alternative promoter was identified in the 5-flanking region of TSE 1. The levels of (+) Box 1 TTS cPRLR transcripts increase dramatically at the onset of sexual maturity, whereas the full-length cPRLR transcript is depressed. When transiently expressed in 293 cells, the (+) Box 1 cPRLR cDNA constitutively actives a STAT5 responsive reporter gene. The (−) Box 1 cPRLR does not stimulate PRL signaling. Photo-stimulation of pubescent cockerels increases their plasma levels of prolactin, leutinizing hormone, follicle-stimulating hormone and testosterone when compared to that of the photo-inhibited chickens. Photo-stimulation results in higher expression of the TTS cPRLR, while the abundance of full-length cPRLR mRNA is reduced. In contrast, the underdeveloped testes of the photo-inhibited cockerels show predominant expression of the full-length cPRLR mRNA. The expression of these unique truncated [(+) or (−) Box 1] cPRLR transcripts in the testes of sexually-mature chicken suggests a complex mechanism of PRL action on gonadal development and reproductive activity.
机译:我们已经表征了家禽中截短的睾丸特异性(TTS)鸡催乳素受体(cPRLR)转录本的两个独特同工型。这两种TTS cPRLR亚型仅对应于全长cPRLR cDNA的胞内结构域,在性成熟鸡中高水平表达。最主要的TTS cPRLR mRNA包含Box 1基序[(+)Box 1 TTS],而另一个转录物[(-)Box 1 TTS]包含一个独特的序列,该序列取代Box 1基序。两个睾丸特异性外显子(TSE 1和2)嵌入cPRLR基因的内含子8和9中。这些TSE可以选择性剪接,以产生在(+)Box 1 cPRLR转录本中发现的四个不同的5 '-非翻译区(5 ' -UTR),以及(-)Box 1 cPRLR mRNA的唯一5 '-末端。在TSE 1的5 '侧翼区域发现了一个替代启动子。在性成熟开始时,(+)Box 1 TTS cPRLR转录本的水平急剧增加,而全长cPRLR转录本沮丧。当在293细胞中瞬时表达时,(+)Box 1 cPRLR cDNA组成性地激活STAT5反应性报告基因。 (-)Box 1 cPRLR不刺激PRL信号。与受光抑制的鸡相比,对光阴的公鸡进行光刺激可增加其血浆催乳素,亮氨酸激素,促卵泡激素和睾丸激素的水平。光刺激导致TTS cPRLR的更高表达,而全长cPRLR mRNA的丰度降低。相反,未发育发育的受光抑制的公鸡的睾丸显示了全长cPRLR mRNA的主要表达。这些独特的截短的[(+)或(-)方框1] cPRLR转录本在性成熟鸡的睾丸中的表达表明PRL对性腺发育和生殖活动的作用机制复杂。

著录项

  • 作者

    Tang, Jianshan.;

  • 作者单位

    University of Delaware.;

  • 授予单位 University of Delaware.;
  • 学科 Biology Molecular.
  • 学位 Ph.D.
  • 年度 2002
  • 页码 185 p.
  • 总页数 185
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 分子遗传学;
  • 关键词

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