Article ID | Journal | Published Year | Pages | File Type |
---|---|---|---|---|
2021167 | Protein Expression and Purification | 2009 | 5 Pages |
Abstract
In the present study, functionally active, recombinant chitribrisin, which is a thrombin-like enzyme in the venom of the Chinese green pit viper (Trimeresurus albolabris), was expressed and purified using a prokaryotic system. The fusion protein of chitribrisin, together with TrxA and 6à His via an E. coli expression vector pET-32a(+), was successfully expressed in E. coli BL21(DE3) cells. After the fusion protein was isolated and purified by chelated Ni2+ resin and specifically cleaved by enterokinase, the recombinant chitribrisin showed a strong fibrinogenolytic activity against the α and β chains of human plasminogen-free fibrinogen and weak fibrinogen clotting activity. In addition, multiple sequence alignment revealed that the expressed chitribrisin was homologous to GPV-TL1 and GPV-TL2 from the snake venom of T. albolabris from central Thailand in terms of the amino acid sequence identities. However, there were some differences in the amino acid sequences of the proteins from the same species from different geographical locations. The causes for the geographical variation in TELs in the same species remain to be investigated. Mutagenesis of chitribrisin should be performed in future studies to study the structural and functional relationship and to identify the critical residues responsible for the properties of the thrombin-like enzyme.
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Authors
Yixin Lin, Xiaodong Yu, Qiyi He, Heng Li, Dehua Li, Xixun Song, Yusheng Wang, Haoping Wen, Huanhuan Deng, Jiangyu Deng,