A chromatographic and immunoprofiling approach to optimising workflows for extraction of gluten proteins from flour

•A single-step and a two-step procedure were compared.•Defatting flours had a detrimental effect on extraction efficiency.•Both procedures proved equally effective at extracting protein.•The two-step method gave a more complete extraction of gluten proteins. Ingestion of gluten proteins from wheat,...

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Veröffentlicht in:Journal of chromatography. B, Analytical technologies in the biomedical and life sciences Analytical technologies in the biomedical and life sciences, 2023-01, Vol.1215, p.123554-123554, Article 123554
Hauptverfasser: Daly, Matthew, Huang, Xin, Nitride, Chiara, Tranquet, Olivier, Rogers, Adrian, Shewry, Peter R., Gethings, Lee A., Mills, E.N. Clare
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Sprache:eng
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Zusammenfassung:•A single-step and a two-step procedure were compared.•Defatting flours had a detrimental effect on extraction efficiency.•Both procedures proved equally effective at extracting protein.•The two-step method gave a more complete extraction of gluten proteins. Ingestion of gluten proteins from wheat, and related prolamin proteins from barley, rye, and oats, can cause adverse reactions in individuals with coeliac disease and IgE-mediated allergies. As there is currently no cure for these conditions, patients must practice avoidance of gluten-containing foods. In order to support patients in making safe food choices, foods making a “gluten-free” claim must contain no more than 20 mg/Kg of gluten. Mass spectrometry methods have the potential to provide an alternative method for confirmatory analysis of gluten that is complementary to analysis currently undertaken by immunoassay. As part of the development of such methodology the effectiveness of two different extraction procedures was investigated using wholemeal wheat flour before and after defatting with water-saturated butan-1-ol. A single step extraction with 50 % (v/v) propan-2-ol containing 2 M urea and reducing agent (buffer 1) was compared with a two-step extraction using 60 % (v/v) aqueous ethanol (buffer 2) followed by re-extraction of the pellet using buffer 1, using either wheel mixing under ambient conditions (19 °C) or sonication at 60 °C. The procedures were compared based on total protein extraction efficiency and the composition of the extracts determined using a combination of HPLC, SDS-PAGE and immunoblotting with a panel of four gluten-specific monoclonal antibodies. Defatting generally had a detrimental effect on extraction efficiency and sonication at 60 °C only improved extraction efficiency with buffer 2. Although the single-step and two-step procedures were equally effective at extracting protein from the samples, analysis of extracts showed that the two-step method gave a more complete extraction of gluten proteins. Future studies will compare the effectiveness of these procedures when applied in the sample workflows for mass spectrometry based methods for determination of gluten in food.
ISSN:1570-0232
1873-376X
DOI:10.1016/j.jchromb.2022.123554