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内含肽介导的胸腺素α1-胸腺五肽融合肽在大肠杆菌中的表达、纯化及特性研究

Intein-mediated expression, purification, and characterization of thymosin α1-thymopentin fusion peptide in Escherichia coli.

作者信息

Li Juan, Zheng Lei, Li Pingli, Wang Fengshan

机构信息

Institute of Biochemical and Biotechnological Drugs, School of Pharmaceutical Sciences, Shandong University, Jinan 250012, China.

出版信息

Protein Expr Purif. 2012 Jul;84(1):1-8. doi: 10.1016/j.pep.2012.04.013. Epub 2012 Apr 25.

Abstract

Thymosin α1-thymopentin (Tα1-TP5) fusion peptide has been proved to be an immune regulator based on its higher immunoregulatory activity than Tα1 and TP5. To obtain Tα1-TP5 more effectively and economically, Tα1-TP5 was genetically fused to a self-cleaving intein-chitin binding domain tag for purification via chitin beads in Escherichia coli. After affinity purification, the target peptide was released from the chitin beads via self-cleaving intein ((INTervening protEIN) induced by dithiothreitol. Further, Tα1-TP5 was purified by Superdex 30 and identified by Tricine-SDS-PAGE and electrospray ionization-mass spectrometry. Finally, about 7.6 mg Tα1-TP5 purified from the soluble fraction and inclusion bodies was obtained from 1 L culture media. The purity was 95% after a series of chromatographic purification steps. In vitro, the purified Tα1-TP5 could stimulate the proliferation of mouse splenic lymphocytes. Overall, this work demonstrated that Tα1-TP5 was purified with low cost and high efficiency, greatly expanding its potential use as an immune regulator.

摘要

胸腺素α1-胸腺五肽(Tα1-TP5)融合肽已被证明是一种免疫调节剂,因为它比Tα1和TP5具有更高的免疫调节活性。为了更有效且经济地获得Tα1-TP5,将Tα1-TP5与一个自我切割的内含肽-几丁质结合结构域标签进行基因融合,以便在大肠杆菌中通过几丁质珠进行纯化。亲和纯化后,通过二硫苏糖醇诱导的自我切割内含肽(INTervening protEIN)从几丁质珠上释放目标肽。此外,Tα1-TP5通过Superdex 30进行纯化,并通过Tricine-SDS-PAGE和电喷雾电离质谱进行鉴定。最后,从1 L培养基中获得了约7.6 mg从可溶性部分和包涵体中纯化的Tα1-TP5。经过一系列色谱纯化步骤后,纯度达到了95%。在体外,纯化的Tα1-TP5能够刺激小鼠脾淋巴细胞的增殖。总体而言,这项工作表明Tα1-TP5以低成本和高效率进行了纯化,极大地扩展了其作为免疫调节剂的潜在用途。

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