10×Taq Buffer（Mg2+ Plus）

Taq酶PCR实验方法介绍

of a master mix containing water, buffer, dNTPs, primers and Taq DNA Polymerase in a single tube, which can then be aliquoted into individual tubes. MgCl2 and template DNA solutions are then added. This method of setting reactions minimizes the possibility

Taq Polymerase Purification

This is a protocol from Engelke et.al.(1990)which was modified by Dr.Baron.The enzyme has been used for RT-PCR,genotyping and cloning.Solutions1000X IPTG0.5M IPTG 1.19g IPTGup to 10 ml wih sterile Qfilter and store at -20℃Buffer A50 mM Tris 7.9 25

PCR反应体系的Mg2+的浓度

PCR 反应体系的Mg2+ 的浓度 Mg2+ 是Taq DNA聚合酶活性所必需的,Mg2+ 浓度除影响酶活性与忠实性外,也影响引物的退火, 模板与PCR产物的解链温度,产物的特异性引物二聚体的形成等。Mg2+ 浓度过低时,酶活力明显降低;过高时,酶可催化非特异性扩增。PCR中Mg2+ 浓度在0.5～2.5mmol/L之间。如果溶液中存在EDTA,或在引物贮备液中有其他螯合物或者DNA模板,会干扰Mg2+ 的浓度。因此,要适当调整Mg2+ 的用量。 Mg2+ 浓度