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Original Article

A Biotin-Coupled Bifunctional Enzyme Exhibiting Both Glutamine Synthetase Activity and Glutamate Decarboxylase Activity

, , , &
Pages 809-818 | Received 16 Jan 2009, Accepted 02 Jun 2009, Published online: 06 Nov 2009
 

Abstract

Purpose: To purify and study native form and enzymatic activity of the 42 kDa biotin-coupled protein (p42), which is related to glutamate action in chick retina.

Methods: p42 was purified using molecular filtration in the presence of 0.7 M sodium chloride. Purity and identification of p42 were studied by SDS-PAGE, 2D-PAGE, LC-MS/MS, and MALDI-TOF MS. The native form of p42 was investigated using native-PAGE and Ferguson plot. Biotin-coupled property was examined by Western blot analysis. Enzymatic actions of p42 were studied using glutamate as substrate in the presence or absence of glutamine.

Results: p42 was successfully purified from chick retinal protein solution using the molecular filtration. Western blot analysis with avidin showed that p42 was a biotin-coupled protein. Using SDS-PAGE, 2D-PAGE, LC-MS/MS, and MALDI-TOF MS, purified p42 was identified as a glutamine synthetase with four isoforms. Native-PAGE, followed by Ferguson plot analysis, showed two molecular forms of p42 corresponding to homotetramers and homooctamers. Enzymatic reaction followed by paper chromatography showed that p42 catalyzed the synthesis of glutamine from glutamate in the presence of ammonium ion, ATP, and magnesium ion. At prolonged reaction time, γ-aminobutyric acid (GABA) was also formed. With glutamate and glutamine present at equal concentrations in the reaction mixture, GABA could be rapidly detected, but GABA could not be detected when glutamate concentration was more than four-fold that of glutamine. The results indicated that p42 also had glutamate decarboxylase activity. Both enzymatic activities were inhibited by avidin. High concentrations of Mn2+ inhibited synthetase activity of p42 but not decarboxylase activity.

Conclusion: p42 was purified from chick retinal protein solution using molecular filtration in the presence of sodium chloride. The protein was a biotin-coupled bifunctional enzyme that contained glutamine synthetase activity and glutamate decarboxylase activity. Biotin was possibly involved in these activities. Mn2+ showed different effects on the two activities.

ACKNOWLEDGMENTS

This work was financially supported in part by The KKU’s Graduate Research Fund academic year 2005. The 2D-PAGE, LC-MS/MS, MALDI-TOF MS, and database search were performed at the Bioservice Unit, National Science and Technology Development Agency, Bangkok, Thailand.

Declaration of interest: The authors report no conflict of interest. The authors alone are responsible for the content and writing of the paper.

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