A homogeneous immunoassay for the mycotoxin T-2 utilizing liposomes, monoclonal antibodies, and complement. Academic Article uri icon

abstract

  • The trichothecene mycotoxin T-2 is a fungal metabolite known to contaminate agricultural products and cause intoxication of humans and animals. We have developed a homogeneous competition inhibition assay for T-2 mycotoxin based on complement-mediated lysis of liposomes. The T-2 mycotoxin was converted to an acid chloride derivative, subsequently coupled to the amino group of phosphatidylethanolamine, and incorporated with the phospholipid into unilamellar liposomes. Carboxyfluorescein, which is self-quenched at high concentrations, was entrapped in the liposomes as a release marker. We used a monoclonal IgG1 antibody specific for T-2 mycotoxin and a polyclonal anti-mouse Ig as a secondary antibody since the anti-T-2 IgG1 does not activate complement. In the absence of free T-2, the liposomes were lysed within 30 min after the addition of complement, releasing carboxyfluorescein into the surrounding buffer. In the presence of free T-2 toxin, the binding of antibodies to the liposomes was reduced, causing a corresponding decrease in lysis. This assay proved to be sensitive to T-2 toxin levels as low as 2 ng, which is 10-fold more sensitive than the present enzyme immunoassay using the same antibodies.

published proceedings

  • Anal Biochem

altmetric score

  • 12

author list (cited authors)

  • Ligler, F. S., Bredehorst, R., Talebian, A., Shriver, L. C., Hammer, C. F., Sheridan, J. P., Vogel, C. W., & Gaber, B. P.

citation count

  • 34

complete list of authors

  • Ligler, FS||Bredehorst, R||Talebian, A||Shriver, LC||Hammer, CF||Sheridan, JP||Vogel, CW||Gaber, BP

publication date

  • June 1987