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An improved radiochemical assay for uridine diphosphoglucose pyrophosphorylase
Authors:BD Hames
Institution:Department of Biology University of Essex Wivenhoe Park Colchester, C04 3SO, England
Abstract:UDP glucose is an important intermediate in numerous metabolic pathways (1). It is therefore not surprising that the enzyme which catalyses its formation, UDP-glucose pyrophosphorylase is ubiquitous (see (2) for references). The reaction catalysed by UDP-glucose pyrophosphorylase is:
glucose-1-P + UTP ? UDP glucose + PPi
and the enzyme has been assayed either in the direction of pyrophosphorolysis of the nucleoside diphosphate sugar or in the direction of UDP-glucose formation.Spectrophotometric assays of UDP-glucose pyrophosphorylase in the direction of pyrophosphorolysis are often nonspecific by virtue of the nature of the coupling enzymes (3), whereas similar assays in the direction of UDPG formation may lack the expected stoichiometry of reaction (3,4). Radioisotopic techniques for the assay of UDP-glucose pyrophosphorylase (5,6) are to be preferred to spectrophotometric assays both for their increased sensitivity and specificity. However, these methods depend upon the specific isolation of the radioactive UDP glucose formed, either by a somewhat tedious adsorption to and elution from charcoal (5) or a hazardous precipitation using mercuric acetate. For routine assay of a large number of samples it would be advantageous to replace these techniques with one involving a safer, more rapid method of radioactive UDP-glucose isolation. The radiochemical assay described in this note utilises the binding of UDP glucose to commercially available, anion-exchange filter-paper discs for this purpose. Although the technique was designed to assay UDP-glucose pyrophosphorylase in cell extracts of the cellular slime mould, Dictyostelium discoideum, it should be applicable to most sources of the enzyme.
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