Highly-Sensitive Detection of Multiple Porcine-Specific Peptides in Processed Foods by LC/MS/MS Method
Applications | 2017 | ShimadzuInstrumentation
The unauthorized addition of pork to processed foods poses economic, safety and ethical challenges, especially for consumers observing halal or kosher dietary laws. DNA-based assays often fail after heat treatment, so a peptide-based approach offers greater reliability for confirming permissible food status.
This study consolidated seven heat-stable porcine-specific peptide markers into a single LC–MS/MS MRM method to detect and semi-quantify trace amounts of pork in processed food matrices, ensuring sensitive and selective halal authentication.
Sample preparation comprised four steps:
Shimadzu LCMS-8060 triple-quadrupole mass spectrometer coupled to Nexera X2 UHPLC. Phenomenex Aeris Peptide XB-C18 column (150×2.1 mm, 1.7 µm) with a water/acetonitrile gradient (0.1 % formic acid).
Specificity tests confirmed no cross-reactivity with beef and distinguished one homologous peptide in chicken by unique fragment ions. All seven markers remained detectable after heating at 200 °C for 30 min. Screening of commercial items correctly identified pork in non-halal products and no markers in certified halal foods. Spiking experiments in mutton curry demonstrated detection limits down to 0.1 % (wt) for key peptides YDII, LVVI and SALA. Calibration curves for four peptides showed linearity (R2 ≥ 0.995) across 0.1–5 % spiking with inter-day RSD ≤16 %.
Further developments may include:
The presented LC–MS/MS MRM assay offers a robust, heat-stable peptide-based solution for detecting trace porcine material in processed foods, enhancing the accuracy of halal and kosher compliance testing.
LC/MS, LC/MS/MS, LC/QQQ
IndustriesFood & Agriculture
ManufacturerShimadzu
Summary
Significance of the topic
The unauthorized addition of pork to processed foods poses economic, safety and ethical challenges, especially for consumers observing halal or kosher dietary laws. DNA-based assays often fail after heat treatment, so a peptide-based approach offers greater reliability for confirming permissible food status.
Objectives and overview of the study
This study consolidated seven heat-stable porcine-specific peptide markers into a single LC–MS/MS MRM method to detect and semi-quantify trace amounts of pork in processed food matrices, ensuring sensitive and selective halal authentication.
Methodology and instrumentation
Sample preparation comprised four steps:
- Protein extraction from meat or processed food using urea/thiourea buffer.
- Reduction with dithiothreitol, alkylation with iodoacetamide, and tryptic digestion.
- SPE cleanup of digest using methanol and formic acid conditioning.
- UHPLC–MRM analysis targeting seven porcine peptides.
Used instrumentation
Shimadzu LCMS-8060 triple-quadrupole mass spectrometer coupled to Nexera X2 UHPLC. Phenomenex Aeris Peptide XB-C18 column (150×2.1 mm, 1.7 µm) with a water/acetonitrile gradient (0.1 % formic acid).
Main results and discussion
Specificity tests confirmed no cross-reactivity with beef and distinguished one homologous peptide in chicken by unique fragment ions. All seven markers remained detectable after heating at 200 °C for 30 min. Screening of commercial items correctly identified pork in non-halal products and no markers in certified halal foods. Spiking experiments in mutton curry demonstrated detection limits down to 0.1 % (wt) for key peptides YDII, LVVI and SALA. Calibration curves for four peptides showed linearity (R2 ≥ 0.995) across 0.1–5 % spiking with inter-day RSD ≤16 %.
Benefits and practical applications
- High sensitivity and selectivity for processed and cooked foods.
- Reliable detection at levels as low as 0.1 % pork in complex matrices.
- Supports halal and kosher certification, food safety and quality control.
Future trends and potential applications
Further developments may include:
- Expanding peptide panels for multi-species food authentication.
- Automating and streamlining sample preparation workflows.
- Incorporating high-resolution MS and advanced data analysis tools.
- Validating the method across diverse processed food matrices.
Conclusion
The presented LC–MS/MS MRM assay offers a robust, heat-stable peptide-based solution for detecting trace porcine material in processed foods, enhancing the accuracy of halal and kosher compliance testing.
References
- N. A. Fadzlillah, Y. B. Che Man, M. A. Jamaludin, S. Ab. Rahman, H. A. Al-Kahtani, 2nd Int. Conf. Humanities, Historical and Social Sciences, PEDR 17 (2011) 159–163.
- M. E. Ali, M. Kashif, K. Uddin, U. Hashim, S. Mustafa, Y. B. Che Man, Food Anal. Methods 5 (2012) 123–130.
- S. Soares, J. S. Amaral, M. B. Oliveira, I. Mafra, Meat Sci. 94 (2013) 115–120.
- D. Kesuma, L. G.-S. Lim, Z. Zhan, Shimadzu Application News AD-0120 (2016).
- C. von Bargen, J. Dojahn, D. Waidelich, H. U. Humpf, J. Brockmeyer, J. Agric. Food Chem. 61 (2013) 11986–11994.
- C. von Bargen, J. Brockmeyer, H. U. Humpf, J. Agric. Food Chem. 62 (2014) 9428–9435.
- S. A. Sarah, W. N. Faradalila, M. S. Salwani, I. Amin, S. A. Karsani, A. Q. Sazili, Food Chem. 199 (2016) 157–164.
- A. J. Barnes, N. J. Loftus, J. Iida, ASMS 2015, WP099.
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