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大鼠雄激素受体:一级结构、其信使核糖核酸的自调节以及受体蛋白的免疫细胞化学定位

The rat androgen receptor: primary structure, autoregulation of its messenger ribonucleic acid, and immunocytochemical localization of the receptor protein.

作者信息

Tan J A, Joseph D R, Quarmby V E, Lubahn D B, Sar M, French F S, Wilson E M

机构信息

Laboratories for Reproductive Biology, University of North Carolina, Chapel Hill 27599.

出版信息

Mol Endocrinol. 1988 Dec;2(12):1276-85. doi: 10.1210/mend-2-12-1276.

Abstract

A composite androgen receptor DNA sequence 4,181 base pairs in length was determined from three cDNA clones isolated from a rat epididymal bacteriophage lambda gt11 library. An open reading frame of 902 amino acids encodes a protein of 98,227 mol wt. Structural domains characteristic of the steroid receptor family include an amino-terminal region with five repeated amino acid motifs, a central DNA-binding domain homologous with other steroid receptors, and a carboxyl-terminal steroid-binding region. A receptor cDNA probe used in Northern blot analysis hybridized with a predominant 10-kilobase androgen receptor mRNA in male reproductive tissues of the rat. Autoregulation of androgen receptor mRNA was indicated in rat ventral prostate by an increase in the level of 10-kilobase mRNA after castration and suppression of receptor mRNA upon androgen restimulation. A 15 amino acid peptide with sequence derived from the deduced androgen receptor sequence was synthesized and used as immunogen in raising receptor antibodies in rabbits. Antisera reacted with high titer against the synthetic peptide by enzyme-linked immunosorbent assay and against the native [3H]dihydrotestosterone-labeled androgen receptor as evidenced by an increase in receptor sedimentation rate determined by sucrose gradient centrifugation. Immunocytochemical staining localized the androgen receptor to epithelial cell nuclei in rat ventral prostate.

摘要

从大鼠附睾噬菌体λgt11文库中分离出的三个cDNA克隆中确定了一个长度为4181个碱基对的复合雄激素受体DNA序列。一个由902个氨基酸组成的开放阅读框编码一个分子量为98227的蛋白质。类固醇受体家族特有的结构域包括一个具有五个重复氨基酸基序的氨基末端区域、一个与其他类固醇受体同源的中央DNA结合结构域以及一个羧基末端类固醇结合区域。用于Northern印迹分析的受体cDNA探针与大鼠雄性生殖组织中占主导地位的10千碱基雄激素受体mRNA杂交。大鼠腹侧前列腺中雄激素受体mRNA的自调节表现为去势后10千碱基mRNA水平升高,雄激素再刺激后受体mRNA受到抑制。合成了一个由15个氨基酸组成的肽段,其序列源自推导的雄激素受体序列,并用作免疫原在兔中产生受体抗体。通过酶联免疫吸附测定法,抗血清与合成肽反应产生高滴度,并且通过蔗糖梯度离心法测定的受体沉降率增加证明抗血清与天然[3H]双氢睾酮标记的雄激素受体反应。免疫细胞化学染色将雄激素受体定位在大鼠腹侧前列腺的上皮细胞核中。

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