Probing the active site of homoserine trans-succinylase

Ran Rosen; Dörte Becher; Knut Büttner; Dvora Biran; Michael Hecker; Eliora Z. Ron

doi:10.1016/j.febslet.2004.10.037

Probing the active site of homoserine trans-succinylase

Ran Rosen, Dörte Becher, Knut Büttner, Dvora Biran, Michael Hecker, Eliora Z. Ron^*

^*Corresponding author for this work

Biotechnology

Research output: Contribution to journal › Article › peer-review

46 Scopus citations

Abstract

Homoserine trans-succinylase is the first enzyme in methionine biosynthesis of Escherichia coli and catalyzes the activation of homoserine via a succinylation reaction. The in vivo activity of this enzyme is subject to tight regulation by several mechanisms, including repression and activation of gene expression, feedback inhibition, temperature regulation and proteolysis. This complex regulation reflects the key role of this enzyme in bacterial metabolism. Here, we demonstrate - using proteomics and high-resolution mass spectrometry - that succinyl is covalently bound to one of the two adjacent lysine residues at positions 45 and 46. Replacing these lysine residues by alanine abolished the enzymatic activity. These findings position the lysine residues, one of which is conserved, at the active site.

Original language	English
Pages (from-to)	386-392
Number of pages	7
Journal	FEBS Letters
Volume	577
Issue number	3
DOIs	https://doi.org/10.1016/j.febslet.2004.10.037
State	Published - 19 Nov 2004

Keywords

Escherichia coli
Mass spectrometry
Methionine biosynthesis
Proteomics
Succinyl homoserine
Two-dimensional gel electrophoresis

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10.1016/j.febslet.2004.10.037

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abstract = "Homoserine trans-succinylase is the first enzyme in methionine biosynthesis of Escherichia coli and catalyzes the activation of homoserine via a succinylation reaction. The in vivo activity of this enzyme is subject to tight regulation by several mechanisms, including repression and activation of gene expression, feedback inhibition, temperature regulation and proteolysis. This complex regulation reflects the key role of this enzyme in bacterial metabolism. Here, we demonstrate - using proteomics and high-resolution mass spectrometry - that succinyl is covalently bound to one of the two adjacent lysine residues at positions 45 and 46. Replacing these lysine residues by alanine abolished the enzymatic activity. These findings position the lysine residues, one of which is conserved, at the active site.",

keywords = "Escherichia coli, Mass spectrometry, Methionine biosynthesis, Proteomics, Succinyl homoserine, Two-dimensional gel electrophoresis",

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AU - Rosen, Ran

AU - Becher, Dörte

AU - Büttner, Knut

AU - Biran, Dvora

AU - Hecker, Michael

AU - Ron, Eliora Z.

PY - 2004/11/19

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AB - Homoserine trans-succinylase is the first enzyme in methionine biosynthesis of Escherichia coli and catalyzes the activation of homoserine via a succinylation reaction. The in vivo activity of this enzyme is subject to tight regulation by several mechanisms, including repression and activation of gene expression, feedback inhibition, temperature regulation and proteolysis. This complex regulation reflects the key role of this enzyme in bacterial metabolism. Here, we demonstrate - using proteomics and high-resolution mass spectrometry - that succinyl is covalently bound to one of the two adjacent lysine residues at positions 45 and 46. Replacing these lysine residues by alanine abolished the enzymatic activity. These findings position the lysine residues, one of which is conserved, at the active site.

KW - Escherichia coli

KW - Mass spectrometry

KW - Methionine biosynthesis

KW - Proteomics

KW - Succinyl homoserine

KW - Two-dimensional gel electrophoresis

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Probing the active site of homoserine trans-succinylase

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