期刊论文详细信息
Brazilian Archives of Biology and Technology
A comparison between enzyme immunoassay and HPLC for ochratoxin A detection in green, roasted and instant coffee
Simone Fujii2  Elisabete Yurie Sataque Ono1  Ricardo Marcelo Reche Ribeiro2  Fernanda Garcia Algarte Assunção2  Cássia Reika Takabayashi2  Tereza Cristina Rocha Moreira De Oliveira2  Eiko Nakagawa Itano1  Yoshio Ueno1  Osamu Kawamura1  Elisa Yoko Hirooka2 
[1] ,Universidade Estadual de Londrina Departamento de Tecnologia de Alimentos e Medicamentos
关键词: Ochratoxin;    immunoassay;    HPLC;    monoclonal antibody;    coffee;   
DOI  :  10.1590/S1516-89132007000200020
来源: SciELO
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【 摘 要 】

An indirect competitive enzyme-linked immunosorbent assay (ic-ELISA) for ochratoxin A (OTA) detection in green, roasted and instant coffees was developed using anti-OTA monoclonal antibody. Immunological reagents prepared were OTA-BSA (4.76 mg/mL), anti-OTA.7 MAb (2x10³-fold dilution) and HRP-anti IgG (10³-fold dilution). The detection limit was 3.73 ng OTA/g and correlation coefficients (r) between this immunoassay and high performance liquid chromatography were 0.98 for green coffee, 0.98 for roasted and 0.86 for instant. OTA levels detected by ic-ELISA were higher than by HPLC, with ELISA/HPLC ratio of 0.66 - 1.46 (green coffee), 0.96 - 1.11 (roasted) and 0.93 - 1.82 (instant). ELISA recoveries for OTA added to coffee (5 - 70 ng/g) were 81.53 % for green coffee, 46.73 % for roasted and 64.35 % for instant, while recoveries by HPLC were 80.54 %, 45.91 % and 55.15 %, respectively. Matrices interferences were minimized by samples dilution before carrying out the ELISA assay. The results indicate that MAb-based ic-ELISA could be a simple, sensitive and specific screening tool for OTA detection, contributing to quality and safety of coffee products.

【 授权许可】

CC BY-NC   
 All the contents of this journal, except where otherwise noted, is licensed under a Creative Commons Attribution License

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