| 2003 年12 月 第1 卷 第4 期 生命科学趋势Trends in Life Sciences
摘要:
少量的DNA 序列的准确定量曾经是一件很难很累的事情,不过real timePCR 的出现把它变为和普通PCR 差不多一样容易。原理是利用能特异标记PCR产物的荧光物质,显示PCR 产物的动态累积,得到S 型的扩增曲线;假设该曲线的前期PCR 符合指数性扩增,于是在单纯指数方程的基础上,通过比较产物积累的速度(时间)来间接比较(进而确定)初始模板的分子数。我们试验了标准曲线的制作,以及对免疫相关的目的基因IL-4 转录水平的定量,而且用HPRT持家基因对IL-4 进行归一化。结果与RT-PCR 相近。灵敏度,误差降低,可重复性有望更上一层楼。
关键词:
real time PCR 定量 荧光SYBR 扩增曲线 标准曲线 cDNA
Abstract:
It had been difficult and tiring to quantitate a small amount of DNA until the invention of real time PCR technique, which is as easy as regular PCR.It produces and displays the kinetic accumulation of PCR product (oramplicon)----called amplification curve. Assuming that amplicons are amplified exponentially during the earlier cycles, we make use of the simple equation y=axto compare the start copy number of a gene in different samples, by measuring the threshold cycle (Ct). And with some standard, copy number of a gene can be
quantified. In this experiment we tried making some standard curves. Then we quantified IL-4 cDNA in 3 subsets of T helper cell, normalized by HPRT housekeeping gene. The result correlates with RT-PCR. However, sensitivity,deviation and precision still need to be improved.
Key word:
real time PCR quantitation fluorescence SYBR Green I amplification curve standard curve cDNA
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