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42 Food Allergens 813
modifications and more (Monaci et al. 2006). Many technolo-
gies, including protein separation via two-dimensional elec-
trophoresis or liquid chromatography (LC), mass spectrometry
and arrays (to map protein–protein interactions), are applied in
proteomic-based studies. Shefcheck and Musser (2004) showed
useful application of LC-based proteins separation with MS
analysis (LC-MS/MS) to detect peanut allergen Ara h1 in ice
cream with a detection level of 10 mg/kg. Proteomic studies can
offer more detailed information about allergens (Shefcheck and
Musser 2004), help in the identification of new allergens (Yu
et al. 2003) and provide objective evaluation of changes induced
by genetic modification (Herman et al. 2003). However, the
requirement of a highly skilled operator, the high cost of mass
spectrometers, the length of time required for sample preparation
and analysis, and the need for separate protocols and optimisa-
tion for each sample prevent current proteomic approaches to be
used for routine detection of food allergens. Nevertheless, pro-
teomics remains a promising tool in allergen studies due to its
great potential for detection and identification of food allergens
in complex mixtures. Recent developments in mass spectrometer
instrumentation and software offer ultra-high throughput, high
sensitivity, and high-resolution capabilities (Chassaigne et al.
2009). Currently, attempts to couple more efficient protein sepa-
ration (microfluidic) and detection technologies with MS analy-
sis are progressing. Proteomic approaches could therefore soon
be widely applicable for detection and identification of food
allergens.
DNA-Based Allergen Detection Methods
Detection of allergens in food, by traditional protein-based de-
tection methods, can sometimes be very difficult, as they are of-
ten present in minute amounts and are masked by the food matrix
(Keck-Gassenmeier et al. 1999). DNA-based allergen detection
methods have emerged as an alternative and complementary
method to detect allergens where effective protein-based aller-
gen detection methods are unavailable. DNA-based tests also
possess high accuracy and sensitivity and, in general, are able to
withstand harsh processing conditions better than corresponding
allergenic proteins (Mustorp et al. 2008). On the other hand, in
some food, DNA are partially or totally degraded and conse-
quently false-negative results could occur, while the food may
still contain the allergen. In addition, some food matrix com-
ponents may reduce DNA amplification efficiency. DNA-based
methods, in comparison to ELISA-based methods, are relatively
more complicated, require more equipment and have lengthier
protocols. For this reason, DNA-based methods have been con-
sidered impractical for routine detection. They may, however,
be desirable for use by regulatory agencies and in institutions
where there is easy access to appropriate equipment.
The sensitivity of the DNA-based methods strongly depends
on the amount and on the quality of the template DNA since the
DNA encoding the allergen in the food samples may be present
in low amounts and may also be degraded as a result of process-
ing (Holzhauser et al. 2006). Three DNA-based approaches are
currently available to detect food allergens.
Polymerase Chain Reaction (PCR) with
Gel Electrophoresis
The assay involves DNA extraction from food, amplification of
specific DNA fragment using primers that bind selectively to
complementary parts of the DNA to be amplified, followed by
agarose gel electrophoresis (Besler 2001). PCR consists of three
steps, determined by different temperatures in every cycle of
amplification: denaturation of double strands DNA, annealing
of the primers and extension of the primers by the enzyme Taq
polymerase (Poms et al. 2004). The amplified product is loaded
to run agarose gel electrophoresis and visualised by staining the
gel. PCR with gel electrophoresis approach is good for qualita-
tive detection of allergen in the food.
PCR with ELISA
This assay is a combination of a highly specific DNA-based
method with the relatively simple and highly sensitive ELISA
assay for semi-quantitative analysis (Poms et al. 2004). As in
other PCR-based methods, extraction and purification of DNA
from a food sample and amplification of specific DNA fragment
encoding to suspected allergen using primers in a thermocy-
cler are prerequisite for PCR-ELISA assay. The ELISA compo-
nent of the test involves immobilisation of the amplified PCR
product on a solid phase (a microplate), denaturation of double
strand, hybridisation with specific probe, detection of the probe
with enzyme-conjugated antibody and observation of the en-
zymatic colour reaction after addition of substrate (Holzhauser
et al. 2002). The DNA concentration can be determined via
absorbance obtained from an enzyme–substrate reaction.
Real-Time PCR
Real-time PCR allows gel-free detection ‘in real time’ with high
accuracy by using a target-specific oligonucleotide probe with a
reporter dye and a quencher dye attached (Desjardin et al. 1998).
Oliver and Vieths (2004) reported real-time PCR method to be as
sensitive as sandwich ELISA in detecting peanut allergens in 33
food samples. Many different types of real-time PCR assay kits
are commercially available to detect many of the priority food
allergens (Poms et al. 2004), including kits for detecting allergen
encoding genes from mustard, sesame and celery (Mustorp et al.
2008).
CONCLUSION
Food allergy will likely continue to be an important food safety
issue in the coming decades. Although substantial progress has
been made in the field in the last 20 years, much still remains
unknown. One area still requiring significant work is the ques-
tion of the minimum eliciting dose required to provoke reactions
in sensitised individuals. Increasing prevalence rates along with
the possibility of severe allergic reactions after exposure to very
low level of allergens in sensitised consumers continue to be
a concern. Although exact threshold doses for food allergens
are not known at present, levels of detection offered by current