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Stable activity of a deubiquitylating enzyme (Usp2-cc) in the presence of high concentrations of urea and its application to purify aggregation-prone peptides
August 2007
August 2007
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Abstract
Chemical synthesis of long or aggregation-prone peptide has been problematic. Its
biological production has an advantage in that point, but it often forms inclusion
body which creates difficulties in recovery of targets. As a deubiquitylating enzyme
(Usp2-cc) was shown in this study to maintain its activity even in the presence of
up to 4M urea, target peptide was purified by a single step of chromatography after
overexpression as inclusion body, solubilization in urea and cleavage by the enzyme
from the fusion protein consisting of GroES (used for high expression and easy to
handle), ubiquitin (as a cleavage site) and target peptide. This system is a convenient
tool for production of peptides that are difficult to be chemically synthesized and
biologically purified.