| 人雄激素受体LBD基因高效表达条件的优化及产物纯化 |
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| 引用本文: | 陈玮,吴珍龄.人雄激素受体LBD基因高效表达条件的优化及产物纯化[J].西南农业大学学报,1999,21(3):209-214. |
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| 作者姓名: | 陈玮 吴珍龄 |
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| 作者单位: | 西南农业大学生物化学教研室,华西医科大学 |
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| 摘 要: | 人雄激素受体激素结合部的cDNA片段克隆到表达载体pTrxFus内,在大肠杆菌GI724中可被诱导表达。通过改变诱导培养时间,诱导剂浓度,诱导温度及培养基的PH,在34-37℃,PH6.4-7.7的培养基中,用100μg/mlTrp诱导培养4h,可获得高效表达的LBD融合蛋白产物。
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| 关 键 词: | 人雄激素受体 激素结合部 表达 优化 纯化 |
A STUDY ON OVERPRODUCTION OF LBD OF HAR IN E.coli AND PRODUCT PURIFICATION |
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| Chen Wei, Wu Zhenling, Yang Shenshan, Wu Wenbing, Wang Sangen, Li Bangxiu, He Mingyue.A STUDY ON OVERPRODUCTION OF LBD OF HAR IN E.coli AND PRODUCT PURIFICATION[J].Journal of Southwest Agricultural University,1999,21(3):209-214. |
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| Authors: | Chen Wei Wu Zhenling Yang Shenshan Wu Wenbing Wang Sangen Li Bangxiu He Mingyue |
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| Abstract: | pTrxAR was constructed by cloning hAR's LBD gene fragment into Cterminal of
Thioredoxin gene at pTrxFus. LBD gene fragment was expressed within Thioredoxin Fusion
Expression System. By inducing, the target gene was expressed, and the target protein was
detected with approximate expected molecular weight (46.56 KD). By changing the inducing
time, inducer concentration, inducing temperature and pH of medium, it was suggested that
satisfied expession could be obtained under 3437, 100 g/ml Trp, pH 6.47.7 and 4 h inducing
time, and the yield of target protein reaches 5070 mg/L bacteria.The LBD gene of hAR was
expressed as a form of inclusion bodies. It can not be purified by osmotic shock. The rough
inclusion bodies sample was gained by lysing the harvested bacteria, centrifuging the lysate
and washing the pellets. The target protoin was purified to homogeneity by solubilzation of
inclusion bodies and gel friltration (Sephacryl S200). The constituent of amino acids and
molecular weight of target protein are consistent to that of the expectaton. |
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| Keywords: | the human androgen receptor (hAR) the ligandbinding domain (LBD) expression optimization Purification |
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