| Literature DB >> 32552602 |
Memoona Iqbal1, Muhammad Sulyman Saleem1, Muhammad Imran1, Waseem Ahmad Khan2, Kamran Ashraf3, M Yasir Zahoor1, Imran Rashid3, Habib-Ur Rehman4, Asif Nadeem1, Saadat Ali1, Sarwat Naz5, Wasim Shehzad1.
Abstract
Food adulteration has a direct impact on public health, religious faith, fair-trades, and wildlife. In the present study, a reliable and sensitive assay has been developed for verifying meat adulteration in food chain. The multiplex PCR system was optimised for identification of chicken, cow/buffalo, sheep/goat, horse/donkey, pork, and dog DNAs in a single reaction mixture simultaneously. The primers were designed using 12 S rRNA gene sequences with fragment size in the range of 113 bp to 800 bp, which can be easily visualised on agarose gel electrophoresis making the technique economical. After validation of accuracy, specificity, and sensitivity, commercially available meat products (n = 190) were screened, comprising both raw and cooked meat samples. The results demonstrated a high rate of adulteration (54.5%) in meat products. The technique developed here can be easily used for screening of different meat products for export and import purposes as well as for food inspection and livestock diagnostic laboratories.Entities:
Keywords: 12S r RNA ; Multiplex PCR; Pakistan; admixture; adulteration; meat species
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Year: 2020 PMID: 32552602 DOI: 10.1080/19393210.2020.1778098
Source DB: PubMed Journal: Food Addit Contam Part B Surveill ISSN: 1939-3210 Impact factor: 3.407