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Mutant rat trypsin selectively cleaves tyrosyl peptide bonds

A double mutant of rat trypsinogen (Asp189Ser, ΔAsp223) was constructed by site-directed mutagenesis. The recombinant protein was produced in Escherichia coli under the control of a periplasmic expression vector. The purified and enterokinase-activated enzyme was characterized by synthetic fluorogen...

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Published in:	Analytical biochemistry 2004-03, Vol.326 (2), p.190-199
Main Authors:	Pál, Gábor, Patthy, András, Antal, József, Gráf, László
Format:	Article
Language:	English
Subjects:	Amino Acid Sequence Amino Acid Substitution Animals Escherichia coli Escherichia coli - genetics Escherichia coli - metabolism Genetic Vectors - genetics Limited proteolysis Molecular Sequence Data Mutagenesis, Site-Directed Peptide Fragments - biosynthesis Peptide Fragments - chemistry Peptide Fragments - metabolism Peptide sequencing Rats Recombinant Proteins - biosynthesis Recombinant Proteins - metabolism Substrate Specificity Trypsin - chemistry Trypsin - genetics Trypsin - metabolism Trypsinogen - biosynthesis Trypsinogen - chemistry Trypsinogen - genetics Tyrosyl peptide bond cleavage
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cites	cdi_FETCH-LOGICAL-c332t-699e9eb00675431d337e5911887db3bd5449134a9b19bcede00deaeffc5373a03
container_end_page	199
container_issue	2
container_start_page	190
container_title	Analytical biochemistry
container_volume	326
creator	Pál, Gábor Patthy, András Antal, József Gráf, László
description	A double mutant of rat trypsinogen (Asp189Ser, ΔAsp223) was constructed by site-directed mutagenesis. The recombinant protein was produced in Escherichia coli under the control of a periplasmic expression vector. The purified and enterokinase-activated enzyme was characterized by synthetic fluorogenic tetrapeptide and natural polypeptide substrates and by a recently developed method. In case of this latter method the specificity profile of the enzyme was examined by simultaneous digestion of a mixture of oligopeptide substrates each differing only at the P 1 site residue, and the results were analyzed by high-performance liquid chromatography. All these assays unanimously demonstrated that the recombinant proteinase lacks trypsin-like activity but acquired a rather unique selectivity: it preferentially hydrolyses peptide bonds C-terminal to tyrosyl residues. This narrow specificity should be useful in peptide-analytical applications such as sequence-specific fragmentation of large proteins prior to sequencing.
doi_str_mv	10.1016/j.ab.2003.12.001
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subjects	Amino Acid Sequence Amino Acid Substitution Animals Escherichia coli Escherichia coli - genetics Escherichia coli - metabolism Genetic Vectors - genetics Limited proteolysis Molecular Sequence Data Mutagenesis, Site-Directed Peptide Fragments - biosynthesis Peptide Fragments - chemistry Peptide Fragments - metabolism Peptide sequencing Rats Recombinant Proteins - biosynthesis Recombinant Proteins - metabolism Substrate Specificity Trypsin - chemistry Trypsin - genetics Trypsin - metabolism Trypsinogen - biosynthesis Trypsinogen - chemistry Trypsinogen - genetics Tyrosyl peptide bond cleavage
title	Mutant rat trypsin selectively cleaves tyrosyl peptide bonds
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