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A facile tritium release assay for mammalian l-dihydroorotate dehydrogenase

โœ Scribed by Thomas W. Kensler; David A. Cooney; Hiremagalur N. Jayaram; Clay Schaeffer; David D. Choie


Publisher
Elsevier Science
Year
1981
Tongue
English
Weight
422 KB
Volume
117
Category
Article
ISSN
0003-2697

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โœฆ Synopsis


Capitalizing on the high concentrations of L-aspartate transcarbamylase and L-dihydroorotase present in the high-speed supernatant from mutant BHK 21 cells resistant to N-(phosphonacetyl)-L-aspartate, I-[ 5,6-'Hldihydroorotic acid has been biosynthesized with these crude enzymes from L-[2,4-'HJaspartic acid and carbamyl phosphate. The product was purified by paper chromatography in solvents which separate it from both L-aspartic and Ncarbamyl-L-aspartic acids. Using this substrate, it has been demonstrated that mitochondria from mouse liver catalyze the release of tritium in a time-and protein-dependent manner as a distillable form susceptible to quantitative trapping in 100% (w/v) KOH; presumably this form is 'H20. Other subcellular fractions release only minor amounts of radioactivity. When comparisons were made of the specific activities of L-dihydroorotate dehydrogenase measured by published techniques as well as by the present tritium release assay, the results were in acceptable agreement. Because of its notable sensitivity, facility, and precision, the technique described herein can be especially recommended for use in analytical studies requiring the manipulation of large numbers of vessels.


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