Light contamination in stable isotope-labelled internal peptide standards is frequent and a potential source of false discovery and quantitation error in proteomics.
Mogjiborahman SalekJonas D FörsterWolf-Dieter LehmannAngelika Beate RiemerPublished in: Analytical and bioanalytical chemistry (2022)
In mass spectrometry-based proteomics, heavy internal standards are used to validate target peptide detections and to calibrate peptide quantitation. Here, we report light contamination present in heavy labelled synthetic peptides of high isotopic enrichment. Application of such peptides as assay-internal standards potentially compromises the detection and quantitation especially of low abundant cellular peptides. Therefore, it is important to adopt guidelines to prevent false-positive identifications of endogenous light peptides as well as errors in their quantitation from biological samples.
Keyphrases
- mass spectrometry
- liquid chromatography
- high performance liquid chromatography
- ms ms
- gas chromatography
- capillary electrophoresis
- liquid chromatography tandem mass spectrometry
- tandem mass spectrometry
- high resolution
- amino acid
- risk assessment
- drinking water
- high throughput
- human health
- solid phase extraction
- simultaneous determination
- label free
- patient safety
- health risk
- clinical practice
- emergency department
- heavy metals
- adverse drug