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ARS Home » Southeast Area » Oxford, Mississippi » Natural Products Utilization Research » Research » Publications at this Location » Publication #98615

Title: EXTRACTION AND CHROMAOGRAPHIC PROTOCOLS FOR MEASURING ASPARAGINE SYNTHETASEACTIVITY IN CRUDE PLANT EXTRACTS

Author
item Romagni, Joanne
item Dayan, Franck

Submitted to: Analytical Biochemistry
Publication Type: Peer Reviewed Journal
Publication Acceptance Date: 1/1/2000
Publication Date: N/A
Citation: N/A

Interpretive Summary: The plant enzyme asparagine synthetase has been difficult to study because it is very unstable. As a result, scientific progress has been hindered. We have developed an improved extraction method that maintains a high level of enzyme activity. This new technique will help other researchers in their studies of this enzyme.

Technical Abstract: The relative instability associated with plant Asparagine synthetase (AS) has made it difficult to extract and assay this enzyme in an active form. We present an improved extraction prototol yielding highly active AS together with an easy and reproducible enzymatic assay using radiolabelled [14C]aspartate to monitor in vitro asparagine formation in crude plant extracts. We optimized conditions for the preparation of crude extracts containing plant AS, and developed a rapid and quantitative HPLC method to measure de novo asparagine synthesis. Optimal [14C]asparagine production was attained after two hours incubation at 25 oC. Under the conditions of this assay, maximum activity was achieved with a concentration of 1 mM glutamine in the assay buffer. This new extraction protocol increased the storage half-life of this enzyme to approximately 9 to 10 d when stored at -25 oC. Using this extraction and assay protocol, AS retains 80% of its activity within the first three days. Activity was measurable for up to twelve days.