Soil samples from three forest soil pits were examined down to a depth of approximately three metres using 1 M ammonium acetate extraction and microwave-assisted extraction with concentrated nitric acid (HNO
Pure oats are generally
accepted to be safe for most celiac patients,
and consumption of oats provides advantageous dietary fibers. However,
oats can be contaminated by gluten proteins from wheat, barley, and/or
rye. The analytical challenge lies in the reliability of the quantification
method and how to maintain the contamination level under a gluten-free
food threshold of 20 mg/kg. In this study, we investigated barley-spiked
oat flour samples at four levels using four gluten ELISA kits. The
largest recovery variance was with the R5 kit that gave 5–6
times overestimation; the G12 kit cross-reacted with oat proteins
and gave 4–5 times overestimation at all spiked levels. The
Total Gluten and Morinaga kits gave satisfactory recoveries. Total
barley hordeins were isolated and characterized to be used as a common
calibrator in all four kits aiming at harmonizing the results and
to test the kits’ performance. Immunoblotting of total hordein
isolate revealed that Total Gluten and Morinaga antibodies provided
an overall detection, while R5 and G12 antibodies recognized specific
hordein groups leading to a larger difference when wheat and barley
were used as the calibrant. Calibration with total hordein isolate
corrected the overestimation problem and decreased the variability
between the four gluten kits.
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