Product Overview
Background
Rat uPA total antigen assay is intended for the quantitative determination of total plasminogen activator antigen in rat plasma.
Urokinase plasminogen activator is a serine protease that activates plasminogen to plasmin in the blood fibrinolytic system. It is also implicated in events related to cell invasion/migration (3).
Assay Principle
Rat uPA will bind to the capture antibody coated on the microtiter plate. Free, latent, and complexed enzyme will react with the capture antibody on the plate. After appropriate washing steps, polyclonal anti-rat uPA primary antibody binds to the captured enzyme. Excess antibody is washed away and bound polyclonal antibody is then reacted with the secondary antibody conjugated to horseradish peroxidase. TMB substrate is used for color development at 450 nm. A standard calibration curve is prepared along with the samples to be measured using dilutions of uPA.
Typical Standard Curve
Reference
1. Declerck, P.J., et al.; (1995) Thromb Haemostas: 74(5): 1305-9
2. Singh, I., et al.; (2003) Circulation: 107(6): 869-875
3. Kjøller, L,; (2002) Biol. Chem.: 383: 5-19
4. Yang, Y.H., et al.; (2001) J. Immunol.: 167(2): 1047-52