pGEM-T Easy(不是T载体)

【原创】入门级T载体构建过程

在丁香园见过很多大佬分享载体构建经验，所以我这里写的T载体构建只能算是入门级，给新手提供一点思路，有什么不足之处还希望大家多多指正。 我克隆的这个片段大小是1.8kb，用的是TaKaRa的LA-Taq酶做的PCR。 反应体系：5*buffer 5 ul MgCl2 5 ul dNTPs 8 ul Primer 1 1 ul Primer 2 1 ul LA-Taq 0.5 ul cDNA 1 ul (1ug左右基因组DNA） ddH2O up to 50 ul

T载体自制法！

Making the T-vector: 1.Digest 5 ug of vector DNA ( pBluescript ＆ pUC18) with a restriction enzyme that generates a unique blunt end site, for example EcoRV or Sma I ( we prefere EcorV for it's stable activity at 37 C) for 2 hours at 37 C. 2.Run

T载体的制作和应用

  Also see DNA Cloning §         Making TA Vector (Crawford Lab) T-vectors are linear-blunt-ended plasmids with a few dT's added on by Taq polymerase. §         Making  TA Vector (Mounir Izallalen) §         Direct PCR