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Publication Date:
June 2005
ISSN:
1437-4315
DOI:
10.1515/BC.2004.148

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Biological Chemistry

Editor-in-Chief: Brüne, Bernhard

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Structural characterization of extracellular lipase from Streptomyces rimosus: assignment of disulfide bridge pattern by mass spectrometry

Ivana Leščić1 / Martin Zehl2 / Roland Müller3 / Bojana Vukelić4 / Marija Abramić5 / Jasenka Pigac6 / Günter Allmaier7 / Biserka Kojić-Prodić8

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Corresponding author

Citation Information: Biological Chemistry. Volume 385, Issue 12, Pages 1147–1156, ISSN (Online) 1437-4315, ISSN (Print) 1431-6730, DOI: 10.1515/BC.2004.148, June 2005

Publication History:
Received:
June 16, 2004
Accepted:
September 29, 2004
Published Online:
2005-06-01

Abstract

The cloning, sequencing and high-level expression of the gene encoding extracellular lipase from Streptomyces rimosus R6-554W have been recently described, and the primary structure of this gene product was deduced using a bioinformatic approach. In this study, capillary electrophoresis-on-the-chip and mass spectrometry were used to characterize native and overexpressed extracellular lipase protein from S. rimosus. The exact molecular mass of the wild-type and the overexpressed lipase, determined by matrix-assisted laser desorption/ionization (MALDI) mass spectrometry, were in excellent agreement (Δm=0.11 Da and Δm=0.26 Da, respectively) with a value of 24165.76 Da calculated from the structure deduced from the nucleotide sequence, considering the mature enzyme with all six cysteines forming disulfide bridges. The primary structure derived from the nucleotide sequence was completely verified using a combination of tryptic digestion and formic acid cleavage of the protein, followed by peptide mass fingerprinting. Selected peptides were further investigated by MALDI low-energy collision-induced dissociation hybrid tandem mass spectrometry, allowing the unambiguous determination of their predicted amino acid sequence. No post-translational modifications of mature S. rimosus lipase were detected. Comparison of the peptide mass fingerprints from the reduced and non-reduced overexpressed enzyme unequivocally revealed three intramolecular disulfide bonds with the following linkages: C27-C52, C93-C101 and C151-C198.

Keywords: amino acid sequence; capillary electrophoresis-on-the-chip; GDSL lipolytic enzyme; low-energy collision-induced dissociation; matrix-assisted laser desorption/ionization; streptomycetes

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