A simple and sensitive method for assay of a ribonucleotide reductase system

A sensitive, rapid, and accurate assay for measuring ribonucleotide reductase activity, including the reduction of CDP. UDP, GDP. and ADP to their corresponding deoxyribonucleotides, is described. Using polyethyleneiminecellulose thin-layer chromatography, I was able to separate the substrates, the

A simple, rapid, and highly sensitive radiochemical assay for measuring the activity of dopamine+hydroxylase in tissues and serum is described. Enzyme activity is detected by converting [l-'"Cltyramine to [l-"Cloctopamine which is then subjected to periodate cleavage to form ["Clformamide. This radi

A simple, rapid, and sensitive fluorometric assay for measuring the activity of tyrosine hydroxylase is described. The enzyme activity is detected by converting tyrosine to 3,4-dihydroxyphenylalanine (dopa), which is then subjected to conversion to the highly fluorescent product by the trihydroxyind

A simplified assay method is described for the determination of protein kinase activity. Enzymatic activity is followed by measuring the incorporation of 32P from the terminal phosphoryl group of nucleoside triphosphates into protein substrate. Separation of the resulting 32P-labeled phosphoprotein

A new, sensitive and simple method to determine the activity of ethoxycoumarin deethylation is described. ## Ethoxycoumarin deethylation was introduced as a measure of mixedfunction oxidation by Ullrich and Weber in 1972 (1). Although the method was not very sensitive, e.g., was not able to detec

A spectrophotometric method for the assay of hyaluronidase activity, based on the binding of a carbocyanine dye (l-ethyl-2-[3-( l-ethyl-naphtho[l,M] to undegraded substrate, is described. The binding results in a spectral shift with an absorbance maximum at 640 nm which is propo~ional to the amount