Abstract
Gluten content from barley, rye, wheat and in certain oat varieties, must be avoid in individuals with celiac disease. In most of the Western countries, the level of gluten content in food to be considered as gluten-free products is below 20 parts per million measured by ELISA based on specific anti-gluten peptide antibody. However, in beverages or food suffering complex hydrolytic processes as beers, the relative proportion of reactive peptides for celiac patients and the analytical techniques may differ, because of the diversity of the resulting peptide populations after fermentations. A beer below 20 parts per million of gluten but yet detectable levels of gluten peptides by anti-gliadin 33-mer antibodies (G12 and A1) was analyzed. We identified and characterized the relevant peptides for either antibody recognition or immunoactivity in celiac patients. The beer was fractionated by HPLC. The relative reactivity of the different HPLC fractions to the G12/A1 antibodies correlated to the reactivity of peripheral blood mononuclear cells isolated from 14 celiac individuals. Peptides from representative fractions classified according to the relative reactivity to G12/A1 antibodies were identified by mass spectrometry. The beer peptides containing sequences with similarity to those of previously described G12 and A1 epitopes were synthesized and confirmed significant reactivity for the antibodies. The most reactive peptides for G12/A1 also confirmed the highest immunogenicity by peripheral blood mononuclear cell activation and interferon γ production from celiac patients. We concluded that preparative HPLC combined with anti-gliadin 33-mer G12/A1 antibodies were very sensitive and specific methods to analyze the relevant immunogenic peptides in hydrolyzed gluten.
Highlights
Celiac disease (CD) is the most common food intolerance in Western countries, with an estimated prevalence that may rise up to 1% in the Caucasian population [1]
Beer was separated into different fractions by reversed-phase HPLC (RP-HPLC) on a semi-preparative C18 column and, each fraction was separated by RP-HPLC on an analytical C18 column [14]
Due to their high content in proline and glutamine, a heterogeneous mixture of peptides could be resistant to proteolysis that could be toxic for CD patients
Summary
Celiac disease (CD) is the most common food intolerance in Western countries, with an estimated prevalence that may rise up to 1% in the Caucasian population [1]. Immunogenic gluten peptides are deamidated by tissue transglutaminase which association generates potent autoantigens These biochemical interactions elicit a T-cell mediated pathological response which consequences are the lymphocytary infiltration of the intestinal epithelia and the destruction of intestinal villi. This last effect makes CD patients to suffer from malabsorption and malnutrition that may lead to diarrhea, constipation, iron-deficiency anemia, osteoporosis, dermatitis herpetiformis and even neurological disorders [7,8,9]. Methods based on the antibodies for the immunogenic 33-mer peptide -G12 and A1- have been accumulating evidences for the detection of the dominant gluten immunogenic peptides for celiac patients in the food [2,12,13,14]. The most reactive peptides to G12/A1 showed the highest reactivity to peripheral blood mononuclear cells (PBMCs) proliferation and interferon c (INF-c) production from celiac patients
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