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A novel approach for production of an active N-terminally truncated Ulp1 (SUMO protease 1) catalytic domain from Escherichia coli inclusion bodies.

Protein Expr Purif. 2020; 
Linova MY1, Ris?r MW2, J?rgensen SE1, Mansour Z1, Kaya J1, Sigurdarson JJ1, Enghild JJ2, Karring H3.
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Codon Optimization … Codon-optimized cDNA of Ulp1 416-621 was synthesized at <b>Genscript</b>? and sub-cloned<br> into the pET28a(+) vector using Nde1 and Xho1 restriction sites, providing an in-frame fusion<br> to the N-terminal and C-terminal His-tags of the pET28a(+) vector … Get A Quote

摘要

The SUMO fusion system is widely used to facilitate recombinant expression and production of difficult-to-express proteins. After purification of the recombinant fusion protein, removal of the SUMO-tag is accomplished by the yeast cysteine protease, SUMO protease 1 (Ulp1), which specifically recognizes the tertiary fold of the SUMO domain. At present, the expression of the catalytic domain, residues 403-621, is used for obtaining soluble and biologically active Ulp1. However, we have observed that the soluble and catalytically active Ulp1403-621 inhibits the growth of E. coli host cells. In the current study, we demonstrate an alternative route for producing active Ulp1 catalytic domain from a His-tagged N-term... More

關鍵詞

Inclusion bodies; Refolding; SUMO-Specific protease; Small ubiquitin-like modifier (SUMO); Ubiquitin-like protease (Ulp); l-arginine
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