𝔖 Bobbio Scriptorium
✦   LIBER   ✦

An Assay for Detecting Nanogram Levels of Proteolytic Enzymes

✍ Scribed by V.M. Koritsas; H.J. Atkinson

Publisher
Elsevier Science
Year
1995
Tongue
English
Weight
404 KB
Volume
227
Category
Article
ISSN
0003-2697

No coin nor oath required. For personal study only.

✦ Synopsis

A rapid, cheap, and sensitive method has been developed for determining proteolytic activity of different classes of endoproteinases. The method is based on a solid-phase assay employing as substrate biotinylated gelatin adsorbed onto microtiter plates. Enzymatic activity is measured by incubating proteinase with the immobilized biotin-protein. Any remaining, undigested substrate bound to the microtiter plate is assayed with streptavidin-alkaline phosphatase. It was established that papain, pepsin, thermolysin, and trypsin all hydrolyzed the biotinylated substrate to varying degrees. Furthermore, the activity of these proteinases was blocked by their respective inhibitors. The assay presented is quick, highly reproducible, inexpensive, and useful for detecting all classes of endoproteolytic enzymes. By using different biotinylated proteins or peptides as substrates, and employing specific buffers and inhibitors, this assay may be utilized for detecting other and more specific endoproteinases. " 1995 Academic Press, Inc.

πŸ“œ SIMILAR VOLUMES

A sensitive microplate assay for the det
A sensitive microplate assay for the detection of proteolytic enzymes using radiolabeled gelatin
✍ B.D. Robertson; G.E. Kwan-Lim; R.M. Maizels πŸ“‚ Article πŸ“… 1988 πŸ› Elsevier Science 🌐 English βš– 365 KB

A sensitive, microplate assay is described for the detection of a wide range of proteolytic enzymes, using radio-iodine-labeled gelatin as substrate. The technique uses the Bolton-Hunter reagent to label the substrate, which is then coated onto the wells of polyvinyl chloride microtiter plates. By m

A rapid method for the quantitative assa
A rapid method for the quantitative assay of proteolytic enzymes
✍ Walter L. Nelson; Edward I. Ciaccio; George P. Hess πŸ“‚ Article πŸ“… 1961 πŸ› Elsevier Science 🌐 English βš– 325 KB

Insoluble dye-protein complexes offer many advantages when used as substrates for proteolytie enzymes. The proteolytic split products can be separated from the starting substrat.e conveniently by filtration, and the concentration of the soluble colored products of hydrolysis can easily be measured a

An Enzyme-Linked Immunosorbant Assay (EL
An Enzyme-Linked Immunosorbant Assay (ELISA) for Detecting Antimitochondrial Antibody
✍ Marshall M. Kaplan; John V. Gandolfo; Elaine G. Quaroni πŸ“‚ Article πŸ“… 1984 πŸ› John Wiley and Sons 🌐 English βš– 457 KB

W e have developed an enzyme linked immunosorbant assay (ELISA) for antimitochondrial antibody. Polyvinyl microtiter plate wells are coated with partially purified rat kidney mitochondria, and excess protein binding sites are blocked with bovine serum albumin. Human serum, diluted 1: 1,000, is incub

An NADH-coupled assay for femtogram or n
An NADH-coupled assay for femtogram or nanogram quantities of chymotrypsin
✍ Edmund A. Mroz; Claude Lechene πŸ“‚ Article πŸ“… 1983 πŸ› Elsevier Science 🌐 English βš– 371 KB

Chymotrypsin can be determined with an NADH-coupled assay. Hydrolysis of the substrate benzoyhyrosine ethyl ester is monitored by coupling the liberation of ethanol to the production of NADH and determining the NADH spectrophotometrically or fluorometrically. Nanogram quantities of chymotrypsin can

Description of an enzyme-linked immunoso
Description of an enzyme-linked immunosorbent assay for the detection of protein tyrosine kinase
✍ Iciar LΓ‘zaro; Miguel Gonzalez; GarbiΓ±e Roy; Luisa M. Villar; Pedro Gonzalez-Porq πŸ“‚ Article πŸ“… 1991 πŸ› Elsevier Science 🌐 English βš– 415 KB

A solid immunoassay for the detection of protein tyrosine kinases has been developed. It is based on the binding of the synthetic polypeptide poly(Glu.Na,Tyr) 4:1 to microELISA wells, where the phosphorylation reaction takes place in the presence of ATP and enzyme. The phosphorylated tyrosine residu