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Competitive ELISA using conjugated antibody can also be used to quantify levels of
circulating antibody in test serum. The solid phase has the antigen to which the
antibody will attach directly coated on to it. The test serum and the conjugated form
of antibody are mixed together and added to the reaction wells. The conjugated and
test antibody then compete to bind to the antigen. The level of antibody can again be
determined by the reduction in signal observed by addition of the substrate.

7.3.6 Dissociation enhanced lanthanide fluorescence immunoassay (DELFIA)


DELFIAis a time-resolved fluorometric assay which relies on the unique properties of
lanthanide chelate antibody labels. The lanthanides will generate a fluorescent signal
when stimulated with light of a specific wavelength. The light signal generated has a
long decay which enhances the negative to positive ratio of the assay. DELFIA offers a
signal enhancement greater than that possible from conventional enzyme-linked
assays. The lanthanide chelates are conjugated onto the secondary antibody and as
there are a number of lanthanides each with a unique signal which can be used,
multiplexing(more than one test carried out in the same reaction vessel) is possible.
The assay is carried out similarly to standard ELISA and may be competitive or non-
competitive. The assay is concluded by adding an enhancement solution which causes
dissociation of the lanthanide from the antibody molecules. The signal is generated
by stimulating the lanthanide with light of a specific wavelength and measuring the

Plate coated
with antibody

Native and conjugated
antigen compete for
coating antibody

Substrate added
to generate
coloured product

Sample and
conjugated
antigen added

Concentration

0

Absorbance

Standard curve
used to interpret
results

Fig. 7.15Competitive ELISA.

290 Immunochemical techniques
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