A Continuous, Nonradioactive Assay for Histone Acetyltransferases

A modified method for the assay of histone acetyltransferase is presented. Previously reported methods depended upon the determination of the incorporation of radioactivity from [Wlacetyl coenzyme A into trichloroacetic acid (TCA)-precipitable material. However, as shown in this paper, [14C]acetylat

Microsomal cysteine-S-conjugate \(\boldsymbol{N}\)-acetyltransferase, an enzyme specific for \(\mathbf{S}\)-substituted cysteines, plays an important role in the detoxicative metabolism of xenobiotics by catalyzing the \(\mathbf{N}\)-acetylation of cysteine-S-conjugates. Cysteine-S-conjugate \(\bold

A sensitive assay for type IV collagen degradation using an avidin-biotin sandwich technique is described. Biotinylated type IV collagen is allowed to bind to an avidin-coated microtiter plate. The solution to be assayed is incubated with the biotinylated collagen bound to the avidin plate. Collagen

A method is described for the assay of histone methyltransferase using soluble histones as substrate. The precipitation of the methylated protein on chromatography paper allows for greater sensitivity and more rapid sample processing than have previously been reported. After incubation of the enzyme

Wheat germ agglutinin (WGA) binds with high affinity and specificity to several sites on chitin polymers. Based on these properties we have modified and adapted a previously patented (U.S. patent 5,888,757) nonradioactive, high throughput screening assay for antimicrobial agents, making it suitable