A secretory system for extracellular production of spider neurotoxin huwentoxin-I in Escherichia coli

神经毒素 大肠杆菌 细胞外 蜘蛛 微生物学 化学 生物 生物化学 动物 基因
作者
Changjun Liu,Qing Yan,Ke Yi,Tianhao Hu,Jianjie Wang,Zheyang Zhang,Huimin Li,Yutao Luo,Dongyi Zhang,Er Meng
出处
期刊:Preparative Biochemistry & Biotechnology [Informa]
卷期号:53 (8): 914-922 被引量:1
标识
DOI:10.1080/10826068.2022.2158473
摘要

Due to their advantages in structural stability and versatility, cysteine-rich peptides, which are secreted from the venom glands of venomous animals, constitute a naturally occurring pharmaceutical arsenal. However, the correct folding of disulfide bonds is a challenging task in the prokaryotic expression system like Escherichia coli due to the reducing environment. Here, a secretory expression plasmid pSE-G1M5-SUMO-HWTX-I for the spider neurotoxin huwentoxin-I (HWTX-I) with three disulfides as a model of cysteine-rich peptides was constructed. By utilizing the signal peptide G1M5, the fusion protein 6 × His-SUMO-HWTX-I was successfully secreted into extracellular medium of BL21(DE3). After enrichment using cation-exchange chromatography and purification utilizing the Ni-NTA column, 6 × His-SUMO-HWTX-I was digested via Ulp1 kinase to release recombinant HWTX-I (rHWTX-I), which was further purified utilizing RP-HPLC. Finally, both impurities with low and high molecular weights were completely removed. The molecular mass of rHWTX-I was identified as being 3750.8 Da, which was identical to natural HWTX-I with three disulfide bridges. Furthermore, by utilizing whole-cell patch clamp, the sodium currents of hNav1.7 could be inhibited by rHWTX-I and the IC50 value was 419 nmol/L.
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