CLONING AND EXPRESSION OF A cDNA SEQUENCE FOR HUMAN THIOREDOXIN

被引:1
作者
刘庆勇
阮喜云
刘效恭
纪宗正
南勋义
王全颖
杨广笑
机构
[1] Center Hospital of Jinan
[2] Department of Surgery
[3] Second Hospital of Xi'an Jiaotong University
[4] First Hospital of Xian Jiao tong University
[5] Xian Huaguang Biotechnology CoLtd
[6] China
[7] Xi 'an
[8] Xian
关键词
thioredoxin; gene clone; RT PCR; sequencing; expression;
D O I
暂无
中图分类号
R346 [];
学科分类号
1001 ;
摘要
Objective To clone and determine the sequence and expression of a cDNA segment for human thioredoxin. Methods The cDNA segment of thioredoxin was obtained through amplification by RT PCR cloning from 143 (TK -) human osteosarcoma cell. The amplified products were cloned into pGEM T Easy vector and sequenced. Then the expressed vector pBV220 hTRX was constructed and transformed into E.coli strain DH5α for hTRX expression. The hTRX was purified by DEAE Sephadex A 50 column and the activity of recombinant hTRX was determined by the insulin disulfide reduction assay. Results Comparison of cDNA sequence of the cloned fragments with that of the reported hTRX (GenBank J04026) demonstrated that there were two differences compared to the reported cDNA sequence for hTRX at bp180 and bp284, and the amino acids enceoded altered respectively, but motif of the sequence was identical to that of the reported hTRX. The recombinant hTRX can catalyze insulin reduction by DTT. Conclusion The successful cloning and expression of hTRX cDNA formed a basis for further study on biological functions and utilization of hTRX.
引用
收藏
页码:183 / 188
页数:6
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