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作 者:王萍[1] 丛敏[1] 李忆梅[1] 唐淑珍[1] 刘晓明[1] 王宝恩[1] 贾继东[1] 尤红[1]
出 处:《首都医科大学学报》2006年第2期210-213,共4页Journal of Capital Medical University
摘 要:目的 比较Taqman荧光定量PCR法、SYBR GreenⅠ荧光定量PCR法和普通PCR法制作3-磷酸甘油醛(GAPDH)标准曲线的检出下限、线性范围的差异,确定一种较好的GAPDH绝对定量方法。方法 构建含GAPDH全长的质粒,经PCR和EcoRⅠ限制性酶切鉴定确认后,紫外定量并连续稀释10倍作为标准品。分别用Taqman法和SYBR GreenⅠ法于荧光定量PCR仪上制作标准曲线,同时用普通PCR结合琼脂糖凝胶电泳利用Quantity One软件定量并制作标准曲线。结果 Taqman法检出GAPDH的下限为2.0×10^4拷贝,线性范围:2.0×10^4~2.0×10^10拷贝;SYBR GreenⅠ法检出GAPDH的下限为2.0×10^7拷贝,线性范围:2.0×10^7~2.0×10^10拷贝;普通PCR检出GAPDH的下限为2.0×10^6拷贝,线性范围:2.0×10^7~2.0×10^9拷贝。结论 Taqman荧光定量PCR法比SYBR GreenⅠ荧光定量PCR法和普通PCR法的灵敏度高,线性范围宽,是核酸水平对GAPDH定量的好方法。Objective In order to find out the best method for GAPDH quantification, the levels of housekeeping gene GAPDH mRNA were detected by Taqman fluorescence quantitative polymerase chain reaction(FQ-PCR), SYBR Green Ⅰ FQ-PCR and conventional PCR, respectively. Methods GAPDH plasmids were constructed by Blue-White Clone method and checked by PCR and EcoR Ⅰ. One of the correct clones was selected for isolating a large amount of plasmids. The selected plasmids were then 10-fold diluted and served as standard. Standard curves were prepared using the data from Taqman FQ-PCR, SYBR Green Ⅰ FQ- PCR and conventional PCR, respectively. The sensitivity and linear range of the three methods were then analyzed. Results The detectable thresholds for Taqman FQ-PCR, SYBR Green I FQ-PCR and conventional PCR were 2.0 × 10^4 , 2.0 ×10^7 and 2.0 × 10^6 DNA copies, respectively. The linear range for these three methods were 2.0×10^4 -2.0×10^10 copies, 2.0×10^7 -2.0× 10^10 copies and 2.0 ×10^7 - 2. 0 ×10^9 DNA copies, respectively. Conclusion Taqman FQ-PCR is a better method for quantifying housekeeping gene GAPDH mRNA than SYBR Green Ⅰ FQ-PCR and conventional PCR.
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