| Literature DB >> 26920302 |
Rosario Linacero1, Isabel Ballesteros2, Africa Sanchiz2, Nuria Prieto1, Elisa Iniesto1, Yolanda Martinez1, Mercedes M Pedrosa2, Mercedes Muzquiz2, Beatriz Cabanillas3, Mercè Rovira4, Carmen Burbano2, Carmen Cuadrado5.
Abstract
A quantitative real-time PCR (RT-PCR) method, employing novel primer sets designed on Jug r 1, Jug r 3, and Jug r 4 allergen-coding sequences, was set up and validated. Its specificity, sensitivity, and applicability were evaluated. The DNA extraction method based on CTAB-phenol-chloroform was best for walnut. RT-PCR allowed a specific and accurate amplification of allergen sequence, and the limit of detection was 2.5pg of walnut DNA. The method sensitivity and robustness were confirmed with spiked samples, and Jug r 3 primers detected up to 100mg/kg of raw walnut (LOD 0.01%, LOQ 0.05%). Thermal treatment combined with pressure (autoclaving) reduced yield and amplification (integrity and quality) of walnut DNA. High hydrostatic pressure (HHP) did not produce any effect on the walnut DNA amplification. This RT-PCR method showed greater sensitivity and reliability in the detection of walnut traces in commercial foodstuffs compared with ELISA assays.Entities:
Keywords: Juglans regia; Pressure processing; Processed foods; Real-time PCR; Thermal processing; Walnut allergen detection
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Year: 2016 PMID: 26920302 DOI: 10.1016/j.foodchem.2016.01.132
Source DB: PubMed Journal: Food Chem ISSN: 0308-8146 Impact factor: 7.514