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绵羊睾丸促卵泡激素受体的分子克隆与表达

Molecular cloning and expression of the ovine testicular follicle stimulating hormone receptor.

作者信息

Yarney T A, Sairam M R, Khan H, Ravindranath N, Payne S, Seidah N G

机构信息

Reproduction Research Laboratory, Clinical Research Institute of Montreal, Quebec, Canada.

出版信息

Mol Cell Endocrinol. 1993 Jun;93(2):219-26. doi: 10.1016/0303-7207(93)90127-6.

DOI:10.1016/0303-7207(93)90127-6
PMID:8394255
Abstract

A sheep testicular cDNA library constructed in pcDNA1 vector was screened with a probe generated by polymerase chain reaction (PCR) and corresponding to a 1.6 kb fragment of the rat luteinizing hormone receptor cDNA. Several clones hybridizing to the rat probe at low stringency were sequenced to obtain 95% of the putative full-length ovine follicle-stimulating hormone receptor (oFSH-R) cDNA. The missing 5' region was obtained by PCR amplification of the cDNA library. Sequencing revealed a 2085 nucleotide open reading frame encoding a mature protein of 678 amino acids (74,580 daltons). The oFSH-R is remarkably similar (> 90%) to the human and rat FSH receptors, has a structural motif like the G protein-coupled family of receptors and contains 3 potential sites for N-linked glycosylation. RNA blot analysis revealed two major transcripts of 2.6 kb and 6.7 kb in size and a smaller transcript of about 1 kb in the sheep testis. A 53 residue segment in the extracellular domain unique to the receptor contains more than 50% of residues bearing functional side chains that could participate in ligand (FSH) interaction and/or signal transduction. Transfection of human fetal kidney cell line (293) with the cloned oFSH receptor cDNA based in pcDNA1/Neo vector revealed functional expression. Labeled oFSH bound to receptor expressed on the membrane with high affinity and specificity. In stably transfected 293 cells, purified oFSH and hFSH but not oLH stimulated cyclic AMP accumulation. Chemically deglycosylated oFSH (DG-oFSH) was inactive in these cells but it effectively blocked the action of native hormone.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

用聚合酶链反应(PCR)产生的、对应于大鼠促黄体生成素受体cDNA 1.6 kb片段的探针,对构建于pcDNA1载体中的绵羊睾丸cDNA文库进行筛选。对几个在低严谨度下与大鼠探针杂交的克隆进行测序,获得了推测的全长绵羊促卵泡激素受体(oFSH-R)cDNA的95%。通过对cDNA文库进行PCR扩增获得缺失的5'区域。测序揭示了一个2085个核苷酸的开放阅读框,编码一个由678个氨基酸组成的成熟蛋白(74,580道尔顿)。oFSH-R与人及大鼠的FSH受体显著相似(>90%),具有类似于G蛋白偶联受体家族的结构基序,并含有三个潜在的N-糖基化位点。RNA印迹分析显示,绵羊睾丸中有两种大小分别为2.6 kb和6.7 kb的主要转录本以及一个约1 kb的较小转录本。受体胞外结构域中一个独特的53个残基片段,含有超过50%带有可参与配体(FSH)相互作用和/或信号转导的功能性侧链的残基。用基于pcDNA1/Neo载体的克隆oFSH受体cDNA转染人胚肾细胞系(293),显示有功能性表达。标记的oFSH以高亲和力和特异性与膜上表达的受体结合。在稳定转染的293细胞中,纯化的oFSH和hFSH可刺激环磷酸腺苷(cAMP)积累,而oLH则无此作用。化学去糖基化的oFSH(DG-oFSH)在这些细胞中无活性,但能有效阻断天然激素的作用。(摘要截短于250字)

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