AI Article Synopsis

  • Milk is commonly adulterated by mixing cow's milk with milk from other animals like goats and sheep, which can pose health risks, especially for those allergic to cow's milk proteins.
  • A new qualitative PCR method was created to accurately detect cow's milk addition in goat and sheep milk, distinguishing it even at low concentrations (down to 1%).
  • Testing showed that 50% of commercial goat milk samples did not comply with labeling regulations, and the PCR method proved more sensitive and efficient than existing tests, with future plans to assess its use in other dairy products.

Article Abstract

Milk is the most consumed liquid food in the world due to its high nutritional value and relatively low cost, characteristics that make it vulnerable to adulteration. One of the most common types of milk adulteration involves the undeclared addition of cow's milk to milk from other mammalian species, such as goats, sheep, buffalo or donkeys. The incidence of such adulteration not only causes a crisis in terms of commercial market and consumer uncertainty but also poses a risk to public health, as allergies can be triggered by proteins in undeclared cow's milk. In this study, a specific qualitative touchdown (TD) PCR method was developed to detect the undeclared addition of cow's milk in goat and sheep milk based on the discrimination of the peak areas of the melting curves after the modification of bovine-specific primers. The developed methodology has high specificity for the DNA templates of other species, such as buffalos and donkeys, and is able to identify the presence of cow's milk down to 1%. Repeatability was tested at low bovine concentrations of 5% and 1% and resulted in %RSD values of 1.53-2.04 for the goat-cow assay and 2.49-7.16 for the sheep-cow assay, respectively. The application of this method to commercial goat milk samples indicated a high percentage of noncompliance in terms of labeling (50%), while a comparison of the results to rapid immunochromatographic and ELISA kits validated the excellent sensitivity and applicability of the proposed PCR methodology that was able to trace more adulterated samples. The developed assays offer the advantage of multiple detection in a single run, resulting in a cost- and time-efficient method. Future studies will focus on the applicability of these assays in dairy products such as cheese and yogurt.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11052330PMC
http://dx.doi.org/10.3390/molecules29081820DOI Listing

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