PARAINFLUENZA ELISA

GM1009.jpg

Indirect immunoenzyme assay to test antibodies against parainfluenza virus in human serum/plasma.

  • Serum dilution and sorbent treatment, when necessary, directly in the well
  • Suitable for automated ELISA systems
Product PARAINFLUENZA 1 ELISA IgG/IgM
Reference
G/M1009
Nº Test
96
CE
Product PARAINFLUENZA 2 ELISA IgG/IgM
Reference
G/M1010
Nº Test
96
CE
Product PARAINFLUENZA 3 ELISA IgG/IgM
Reference
G/M1011
Nº Test
96
CE

The ELISA method is based upon the reaction of antibodies in the sample tested with the antigen adsorbed on the polystyrene surface. Unbound immunoglobulins are washed off. An enzyme-labelled anti-human globulin binds the antigenantibody complex in a second step. After a new washing step, bound conjugate is developed with the aid of a substrate solution (TMB) to render a blue coloured soluble product which turns into yellow after adding the acid stopping solution.

  • High performance and guaranteed stability with lyophilized conjugates when necessary.
  • Samples and controls are equally processed to compensate pipetting variability.
  • Colour-coded plates with individual break-apart wells.
  • Coloured, ready-to-use liquid reagents.
Product PARAINFLUENZA 1 ELISA IgG/IgM
Reference
G/M1009
Nº Test
96
CE
Product PARAINFLUENZA 2 ELISA IgG/IgM
Reference
G/M1010
Nº Test
96
CE
Product PARAINFLUENZA 3 ELISA IgG/IgM
Reference
G/M1011
Nº Test
96
CE

The ELISA method is based upon the reaction of antibodies in the sample tested with the antigen adsorbed on the polystyrene surface. Unbound immunoglobulins are washed off. An enzyme-labelled anti-human globulin binds the antigenantibody complex in a second step. After a new washing step, bound conjugate is developed with the aid of a substrate solution (TMB) to render a blue coloured soluble product which turns into yellow after adding the acid stopping solution.

  • High performance and guaranteed stability with lyophilized conjugates when necessary.
  • Samples and controls are equally processed to compensate pipetting variability.
  • Colour-coded plates with individual break-apart wells.
  • Coloured, ready-to-use liquid reagents.
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