| 摘要: |
| 为进一步研究菘蓝APX基因的功能,构建了菘蓝APX基因真核表达载体。从菘蓝植株中提取总RNA,逆转录为cDNA,根据APX基因在该类植物中的同源性设计简并引物,利用PCR方法钓取目的基因,将目的基因与T载体连接,PCR检测阳性克隆,同时菌液送往测序公司进行测序。结果表明:测序片段的生物信息学分析证实了该序列与GenBank登录的APX基因一致。说明成功构建了菘蓝APX重组质粒和克隆鉴定了菘蓝APX基因,可进一步用于基因表达和表达产物的功能研究。 |
| 关键词: 菘蓝 APX基因 真核表达载体 基因克隆 |
| DOI: |
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| Fund project: |
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| Cloning and identification of APX gene from Isatis indigotica |
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SUN XiaoDong*, LI AiLing, HAN LiMin
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Department of Biological Science and Technology, Shaanxi Institute of Education, Xi′an 710061, China
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| Abstract: |
| To construct the recombinant eukaryotic expression plasmid of pTZ57R/T/APX. APX gene was amplified from the genomic DNA of Isatis indigotica by polymerase chain reaction(PCR). APX gene was then inserted into pTZ57R/T eukaryote expression vector. The positive colonies were screened and identified by PCR 〖JP3〗and sequencing. The specific gene APX which was about 1 257 bp,was successfully amplified and pTZ57R/T APX were constructed. The DNA sequence of APX gene was as the same as the APX gene nucleotide sequences published in Genebank. pTZ57R/T APX recombinant was successfully constructed. And the construction provides the basis for the further study. |
| Key words: Isatis indigotica APX gene eukaryote expression vector gene cloning |
