Malucelli A, Sauerwein H, Pfaffl M W, Meyer H H
Institut für Physiologie, Forschungszentrum für Milch und LebensmittelWeihenstephan, Technische Universität München, Freising, Germany.
J Steroid Biochem Mol Biol. 1996 Aug;58(5-6):563-8. doi: 10.1016/0960-0760(96)00077-5.
We describe a polymerase chain reaction (PCR)-based method for the quantification of androgen receptor (AR) mRNA in tissues. The amount of PCR products depends on the exponential amplification of the initial cDNA copy number; therefore minor differences in the efficiency of amplification may dramatically influence the final product yield. To overcome these tube-to-tube differences in reaction efficiency, an internal control AR cRNA was reverse transcribed along with the target mRNA using the same primers. This standard was obtained by deleting a 38 bp fragment from an amplified bovine AR sequence, which was then subcloned and transcribed into cRNA. Known dilutions of the competitor cRNA were spiked into a series of RT-PCR reaction tubes containing equal amounts of the target mRNA. Following RT-PCR, the co-amplified specimens obtained were separated by gel electrophoresis and quantified by densitometric analysis of ethidium bromide stain. We applied this method to quantify the AR-mRNA in skeletal muscle of castrated as well as from intact male cattle. The applicability of the quantification system for AR-mRNA described herein was demonstrated for other species, e.g. man.
我们描述了一种基于聚合酶链反应(PCR)的方法,用于定量组织中的雄激素受体(AR)mRNA。PCR产物的量取决于初始cDNA拷贝数的指数扩增;因此,扩增效率的微小差异可能会显著影响最终产物的产量。为了克服反应效率在不同管之间的差异,使用相同的引物将内部对照AR cRNA与靶mRNA一起进行逆转录。该标准品是通过从扩增的牛AR序列中删除一个38 bp的片段获得的,然后将其亚克隆并转录为cRNA。将已知稀释度的竞争cRNA加入到一系列含有等量靶mRNA的RT-PCR反应管中。RT-PCR后,将获得的共扩增样本通过凝胶电泳分离,并通过溴化乙锭染色的光密度分析进行定量。我们应用该方法定量去势公牛以及完整雄性牛骨骼肌中的AR-mRNA。本文所述的AR-mRNA定量系统对其他物种(如人类)的适用性也得到了证实。
