Kinetic measurement by LC/MS of γ-glutamylcysteine ligase activity

γ-Glutamylcysteine ligase (GCL) combines cysteine and glutamate through its gamma carboxyl moiety as the first step for glutathione (GSH) synthesis and is considered to be the rate-limiting enzyme in this pathway. The enzyme is a heterodimer, with a heavy catalytic and a light regulatory subunit, wh...

Full description

Saved in:
Bibliographic Details
Published in:Journal of chromatography. B, Analytical technologies in the biomedical and life sciences Analytical technologies in the biomedical and life sciences, 2005-11, Vol.827 (1), p.32-38
Main Authors: Chikh, Karim, Flourie, Françoise, Arab, Khelifa, Steghens, Jean Paul
Format: Article
Language:English
Subjects:
Amino Acid Sequence
Animals
Catalytic activity
Chromatography, Liquid - methods
Dipeptides - analysis
Fibroblasts - metabolism
Glutamate-Cysteine Ligase - metabolism
Glutathione - pharmacology
Glutathione metabolism
Humans
Hydrogen-Ion Concentration
Kinetics
LC/MS
Mass Spectrometry - methods
Microsomes, Liver - metabolism
Molecular Sequence Data
Oxidative stress
Rats
Reproducibility of Results
Sequence Alignment
γ-Glutamylcysteine ligase
Citations: Items that cite this one
Online Access:Get full text
Tags: Add Tag
No Tags, Be the first to tag this record!
Description
Summary:γ-Glutamylcysteine ligase (GCL) combines cysteine and glutamate through its gamma carboxyl moiety as the first step for glutathione (GSH) synthesis and is considered to be the rate-limiting enzyme in this pathway. The enzyme is a heterodimer, with a heavy catalytic and a light regulatory subunit, which plays a critical role in the anti-oxidant response. Besides the original method of Seelig designed for the measurement of a purified enzyme, few endpoint methods, often unrefined, are available for measuring it in complex biological samples. We describe a new, fast and reliable kinetic LC/MS method which enabled us to optimize its detection. l-2-Aminobutyrate is used instead of cysteine (to avoid glutathione synthetase interference) as triggering substrate with saturating concentrations of glutamate and ATP; the γ glutamylaminobutyrate formed is measured at m/ z = 233 at regular time intervals. Reaction rate is maximum because ATP is held constant by enzymatic recycling of ADP by pyruvate kinase and phosphoenolpyruvate. The repeatability of the method is good, with CV% of 6.5 and 4% for catalytic activities at, respectively 0.9 and 34 U/l. The affinities of rat and human enzymes for glutamate and aminobutyrate are in good agreement with previous published data. However, unlike the rat enzyme, human GCL is not sensitive to reduced glutathione and displays a more basic optimum pH.
ISSN:1570-0232
1873-376X
DOI:10.1016/j.jchromb.2004.04.040