A lysozyme assay method for low activity

Most of the methods currently available for the determination of RNase activity are dependent on the measurement of acid-soluble products released 'by hydrolysis of RNA. The major advantages of these methods are that they are sensitive, reproducible, and convenient for large numbers of samples (l-3)

Assay of small-intestinal lactase activity in jejunal biopsies is usually performed with the Tris/glucose oxidase reagent of Dahlqvist (1,2) or more or less modified methods. The glucose oxidase methods are simple and well suited for differentiation of the low activities in lactase-deficient indivi

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

The use of the p-nitrophenyl-cu-L-rhamnopyranoside for the specific measurement of the (Yrhamnosidase activity of naringinase, by calorimetrically following the appearance of p-nitrophenolate anion, is proposed. Use of this synthetic substrate did not change the pH, temperature, or ionic strength op