PROTEIN PURIFICATION USING INTEIN C TERMINAL CLEAVAGE
Project Number1R43GM057734-01
Contact PI/Project LeaderCHONG, SHAORONG
Awardee OrganizationNEW ENGLAND BIOLABS, INC.
Description
Abstract Text
DESCRIPTION: (Adapted from the applicant's abstract) Protein splicing
involves highly specific, self-catalyzed peptide bond cleavage reactions
which provide new avenue for protein engineering and protein synthesis.
Combining the unique self-catalytic property of the Saccharomyces
cerevisiae VMA intein (Sce VMA intein) with affinity chromatography, a
novel protein purification methodology has been developed which has the
potential to drastically reduce the production cost of industrial
enzymes. Utilizing the thio-inducible-N-terminal cleavage activity of
the Sce VMA intein, we have been able to obtain highly purified proteins
after a single column. However, the expression level of the fusion
protein varies with the target protein which can sometimes result in
very low yield. This project should solve this expression problem by
using the inducible C-terminal cleavage activity of the Sce VMA intein.
The target protein will be fused to the C-terminus of the intein
allowing the N-terminal sequence of the fusion protein to be optimized
for high level of protein expression. This C-terminal cleavage system
will first be studied in Escherichia coli and then applied to other
heterologous protein expression systems with secretory capability, e.g.
Pichia pastoris. The latter can potentially be automated for large-
scale industrial productions.
PROPOSED COMMERCIAL APPLICATION: NOT AVAILABLE
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