采用基于PAS(PCR-based Accurate Synthesis)的方法合成target-gene基因,双酶切连接至pAZ-V5载体的Afl II和Xba I之间;将获得的重组质粒转入TOP10克隆菌株,挑取阳性克隆子测序,测序结果拼接如下所示,单划线区为目的基因基因区域。紫色区域为酶切位点,黄色区域为v5信号肽,绿色区域为6XHis标签;
T A G C A G A G C T C T C T G G C T A C T A G A G A A C C C A C T G C T T A C T G G C T T A T C G A A A T T A A T A C G A C T C A C T A T A G G G A G A C C C A A G C T G G C T A G C G T T T A A A C T T A A G C * * X 3 * * * * N N N N N N---略-----N N N N N N * * T G A G T A G G C A C C A C C A C C A C C A C C A C T G A C T C T A G A G G