部分绵羊催产素受体cDNA的分离、结构及其作为探针用于子宫内膜RNA的Northern分析
Isolation and structure of a partial sheep oxytocin receptor cDNA and its use as a probe for northern analysis of endometrial RNA.
作者信息
Stewart H J, Stevenson K R, Flint A P
机构信息
AFRC Research Group on Hormones and Farm Animal Reproduction, Babraham, Cambridge, UK.
出版信息
J Mol Endocrinol. 1993 Jun;10(3):359-61. doi: 10.1677/jme.0.0100359.
The polymerase chain reaction (PCR) was used to generate a 131 bp cDNA encoding part of the sheep endometrial oxytocin receptor. The nucleotide sequence of this cDNA was 93.8% identical to the human oxytocin receptor sequence in this region. When used to probe Northern blots of sheep endometrial RNA the PCR product identified a 6.7 kb mRNA which appeared and disappeared during the oestrous cycle in parallel with the oxytocin receptor molecule as measured by ligand binding. The sheep endometrial receptor mRNA was significantly larger than the human myometrial mRNA (4.7 kb). It is suggested that the cloned cDNA described here is an appropriate probe for use where it is required to measure sheep oxytocin receptor mRNA.
采用聚合酶链反应(PCR)生成了一段131 bp的cDNA,其编码绵羊子宫内膜催产素受体的部分序列。该cDNA的核苷酸序列与该区域的人催产素受体序列有93.8%的同源性。当用该PCR产物探测绵羊子宫内膜RNA的Northern印迹时,鉴定出一条6.7 kb的mRNA,其在发情周期中出现和消失的情况与通过配体结合测定的催产素受体分子一致。绵羊子宫内膜受体mRNA明显大于人子宫肌层mRNA(4.7 kb)。提示此处描述的克隆cDNA是用于检测绵羊催产素受体mRNA的合适探针。
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