Results of PCR amplification and restriction digestion showed that the fragment of antisense gene CYP86MF was introduced into pBI121 plasmid and the expression vector pBI35S-AMF was transferred into Agrobacterium successfully.

  • PCR扩增和酶切鉴定结果表明;所构建的反义CYP86MF基因植物表达载体pBI35S-AMF是正确的;并已成功导入了根癌农杆菌中.
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