Abstract
A radiochemical procedure for measuring aspartate aminotransferase activity in the nervous system is described. The method is based on the exchange of tritium atoms at positions 2 and 3 of l-2,3-[ 3H]aspartate with water when this amino acid is transaminated in the presence of α-ketoglutarate to form oxaloacetate. The tritiated water is separated from the radiolabeled aspartate by passing the reaction mixture over a cation exchange column. Confirmation that the radioactivity in the product is associated with water was obtained by separating it by anion exchange HPLC and by evaporation. The product formation is linear with time up to 120 min and with tissue in the 0.05- to 10-μg range. The apparent K m for aspartate in the rat brain homogenate is found to be 0.83 m m and that for α-ketoglutarate to be 0.12 m m. Methods that further improve the sensitivity of the assay are also discussed.
Published Version
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