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A simple method for measuring intracellular activities of glutamine synthetase and glutaminase in glial cells. | LitMetric

AI Article Synopsis

  • A new method is presented for measuring the activities of glial glutamine synthetase (GS) and glutaminase (GLNase) in live glial cells, which are crucial for recycling glutamate and glutamine in the brain.
  • The study involved culturing rat astrocytes and using radioactive labeled substrates to track the enzymatic activity, separating the products with anion exchange columns.
  • The method's effectiveness was validated with pharmacological inhibitors and HPLC to confirm amino acid levels, providing optimized conditions for future research on these enzymes in glial cells.

Article Abstract

Here we report and validate a simple method for measuring intracellular activities of glial glutamine synthetase (GS) and glutaminase (GLNase) in intact glial cells. These enzymes are responsible for glutamate and glutamine recycling in the brain, where glutamate and glutamine transport from the blood stream is strongly limited by the blood-brain barrier. The intracellular levels of glutamate and glutamine are dependent on activities of numerous enzymatic processes, including 1) cytosolic production of glutamine from glutamate by GS, 2) production of glutamate from glutamine by GLNase that is primarily localized between mitochondrial membranes, and 3) mitochondrial conversion of glutamate to the tricarboxylic cycle intermediate α-ketoglutarate in the reactions of oxidative deamination and transamination. We measured intracellular activities of GS and GLNase by quantifying enzymatic interconversions of L-[(3)H]glutamate and L-[(3)H]glutamine in cultured rat astrocytes. The intracellular substrate and the products of enzymatic reactions were separated in one step using commercially available anion exchange columns and quantified using a scintillation counter. The involvement of GS and GLNase in the conversion of (3)H-labeled substrates was verified using irreversible pharmacological inhibitors for each of the enzymes and additionally validated by measuring intracellular amino acid levels using an HPLC. Overall, this paper describes optimized conditions and pharmacological controls for measuring GS and GLNase activities in intact glial cells.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC3191570PMC
http://dx.doi.org/10.1152/ajpcell.00035.2011DOI Listing

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