Mead, Smith & Williams (1955) introduced a method for the fluorimetric assay of ,B-glucuronidase activity; the method consisted of the enzymic hydrolysis of methylumbelliferyl (3glucuronide, followed by fluorimetric estimation of the liberated methylumbelliferone. Robinson (1956) synthesized methylumbelliferyl (3-glucoside and used it in the study of ,B-glucosidases from a variety of sources; like Mead et al. (1955), Robinson found the fluorogenic method convenient and extremely sensitive. Levvy, Hay & Marsh (1957) attempted to use methylumbelliferyl ,B-glucuronide in the study of limpet fl-glucuronidase; they found methylumbelliferone to be unstable, and so considered the method to be too exacting for general use.
the oxygen uptake and acetoacetate oxidation when added alone or with fumarate, but not in the presence of a-oxoglutarate. The reasons for these differences are discussed. Anaerobically, relatively slight inhibitions of the reduction of acetoacetate were observed. 6. The oxidation of L(+)-p-hydroxybutyrate is inhibited by dinitrophenol, whereas that of the D(-)-form is not. This is related to the fact that only the L(+)-form requires conversion into the coenzyme A derivative. The differences in the behaviour of the Land D-forms towards dinitrophenol were used to examine the configuration of the P-hydroxybutyrate formed in sheep-heart muscle aerobically and anaerobically. In both cases the D-form only was found.
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