用加端PCR技术改造h-IGF-1cDNA  被引量:1

Amplification of hIGF-1 Coding Sequence by PCR Technique

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作  者:罗进贤[1] 吉坤美[1] 张添元[1] 王红革[1] 

机构地区:[1]中山大学生命科学学院

出  处:《中山大学学报(自然科学版)》1996年第2期79-83,共5页Acta Scientiarum Naturalium Universitatis Sunyatseni

摘  要:用DNA合成仪合成了分别带有PstI位点和SalI位点及终止密码子的2个用于扩增hIGF-1cDNA的PCR引物.利用合成的引物,700bp长的hIGF-1cDNA模板和Taq聚合酶进行PCR扩增.扩增产物经电泳鉴定后克隆进M13mp18载体,进行核苷酸序列分析.结果显示:PCR产物含已发表的hIGF-1成熟蛋白的编码序列和5'端的PStI位点及3'端的SaiI位点及终止密码TAG.用加端PCR技术成功地扩增和改造了hIGF-1的编码序列.Two primers containing the Pst I site and Sal I site and stop codon respectively were synthesized and used to amplify a 232 hp DNA sequence coding for mature hIGF-1 protein with the 700 bp hIGF-1 cDNA fragment as template by Taq polymerase.The amplified DNA fragment was cloned into M13mp18 vector and sequenced by Sanger-s dideoxy chain termination method. The sequencing data show that the nucleotide sequence of the cloned fragment is the same as hIGF-1 coding sequence published and that we have successfully remoulded the hIGF-1 protein coding region with Pst I site at 5' end and Sal I site and stop codon at 3' end using the add-on PCR technique.

关 键 词:聚合酶链反应 胰岛素 生长因子 hIGF DNA 

分 类 号:R392-33[医药卫生—免疫学] R394.8[医药卫生—基础医学]

 

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