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Simple radioassay for uridine phosphorylase and 5'-nucleotidase
Authors:H Kizaki  G Weber
Institution:Department of Fisheries and Oceans, Fisheries and Environmental Sciences, Halifax Laboratory, P.O. Box 550, Halifax, Nova Scotia, B3J 2S7, Canada
Abstract:A method is described whereby a large number of chromatographic fractions containing protein or enzyme components may be run on a single-starch gel. A multiple punch for making the sample holes, gel slab support, and a gel slicer used to cut several slices from the one gel for staining for the various enzyme or protien constituents are described. An example is given of a run using fractions obtained from a Sephadex G-200 column chromatography run of a herring muscle extract. Densitometry may be used to assay the stained gels. In another example a commercially obtained muscle lactate dehydrogenase preparation was chromatographed on a Sephadex G-200 column. The electrophoretic run of the fractions revealed the presence of both heart-type A and muscle-type B lactate dehydrogenase subunits and showed that the column run had effected a partial separation of the various tetramers.
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