肠肽酶
融合蛋白
劈理(地质)
融合
大小排阻色谱法
化学
大肠杆菌
色谱法
生物化学
蛋白质纯化
生物
酶
重组DNA
基因
古生物学
语言学
哲学
断裂(地质)
作者
Wen Li,Mingming Gao,Wenchao Liu,Yuelin Kong,Hong Tian,Wenbing Yao,Xiangdong Gao
出处
期刊:Protein and Peptide Letters
[Bentham Science Publishers]
日期:2012-10-01
卷期号:19 (12): 1324-1329
被引量:6
标识
DOI:10.2174/092986612803521710
摘要
Previously we constructed a fusion protein based on GLP-1 and globular adiponectin but unfortunately its yield was low because it was mainly expressed as inclusion bodies. Herein to optimize the soluble expression of this fusion protein we tried several fusion tag systems. Fusion tags, including GST-, Trx- and MBP-tag, greatly improved the soluble expression of the fusion protein. However, these tag-fusion proteins were aggregation-prone as judged by Native PAGE and gel filtration chromatography, and this aggregation reduced the specificity of enterokinase-mediated enzyme cleavage which was essential to remove the fusion tags. To improve the specificity of protein cleavage, we employed on-column cleavage for downstream purification. Finally using optimized expression followed by on-column cleavage, we obtained the product fusion protein with a yield of 1.2 mg per g wet bacterial cells which was 8-fold higher than before. This method improved the yield and simplified the process, and as a convenient method it can also be used for the preparation of other aggregation-prone proteins.
科研通智能强力驱动
Strongly Powered by AbleSci AI