A method for the determination of amylase activity and a useful highly stable color reagent aqueous solution therefore are disclosed. The solution comprises, as a color reagent, an aromatic nitro containing compound such as 3,5-dinitrosalicyic acid, a color stabilizing chelating compound such as ethylenediaminetetraacetic acid, and a hydroxide base. Eliminating the necessity for centrifuging prior to the determination of amylase activity can be achieved by including potassium hydroxide for at least a part of the base in the solution.
A method is disclosed for determining glucose whereby glucose is reacted with an aromatic reagent containing one or more nitro groups and the reaction is monitored at electrodes which measure the current produced by the reduction of one or more of the nitro groups.
A chromogenic substrate for the assay of polysaccharide endo-hydrolases is the reaction product of a polysaccharide susceptible to endo-hydrolase degradation, a chemical reagent for increasing the solubility of the polysaccharide so as to increase its susceptibility to enzyme degradation, and a dye substance for coloring the polysaccharide and rendering it capable of estimation by absorption spectrometry. The amount of chemical reagent should be such as to produce a degree of chemical substitution in the range 0.06 to 0.6 DS.
Method, kits and reagents for the simultaneous, kinetic spectrophotometric analysis of blood serum samples for multiple components. Pairs of components which may be simultaneously analyzed are: cholesterol and triglyceride; glucose and urea; uric acid and gamma glutamyl transferase; calcium and magnesium; albumins and total protein.
