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Quality control of serum and plasma by quantification of (4E,14Z)-sphingadienine-C18-1-phosphate uncovers common preanalytical errors during handling of whole blood

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Autor
Liu X., Hoene M., Yin P., Fritsche L., Plomgaard P., Hansen J.S., Nakas C.T., Niess A.M., Hudemann J., Haap M., Mendy M., Weigert C., Wang X., Fritsche A., Peter A., Häring H.-U., Xu G., Lehmann R.
Fecha
2018
Language
en
DOI
10.1373/clinchem.2017.277905
Materia
biological marker
sphingadienine c18 1 phosphate
unclassified drug
biological marker
ethanolamine derivative
lactic acid
lysophospholipid
phosphate
sphingadienine
sphingosine
sphingosine 1-phosphate
analytical error
Article
biobank
blood cell
blood sampling
blood storage
cell separation
centrifugation
controlled study
human
metabolomics
protocol compliance
quadrupole mass spectrometry
serum
time of flight mass spectrometry
ultra performance liquid chromatography
validation process
blood
quality control
reproducibility
specimen handling
Biomarkers
Ethanolamines
Humans
Lactic Acid
Lysophospholipids
Phosphates
Quality Control
Reproducibility of Results
Specimen Handling
Sphingosine
American Association for Clinical Chemistry Inc.
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Resumen
BACKGROUND: Nonadherence to standard operating procedures (SOPs) during handling and processing of whole blood is one of the most frequent causes affecting the quality of serum and plasma. Yet, the quality of blood samples is of the utmost importance for reliable, conclusive research findings, valid diagnostics, and appropriate therapeutic decisions. METHODS: UHPLC-MS-driven nontargeted metabolomics was applied to identify biomarkers that reflected time to processing of blood samples, and a targeted UHPLC-MS analysis was used to quantify and validate these biomarkers. RESULTS: We found that (4E,14Z)-sphingadienine-C18-1-phosphate (S1P-d18:2) was suitable for the reliable assessment of the pronounced changes in the quality of serum and plasma caused by errors in the phase between collection and centrifugation of whole blood samples. We rigorously validated S1P-d18:2, which included the use of practicality tests on 1400 randomly selected serum and plasma samples that were originally collected during single- and multicenter trials and then stored in 11 biobanks in 3 countries. Neither life-threatening disease states nor strenuous metabolic challenges (i.e., high-intensity exercise) affected the concentration of S1P-d18:2. Cutoff values for sample assessment were defined (plasma, 0.085 g/mL; serum, 0.154 g/mL). CONCLUSIONS: Unbiased valid monitoring to check for adherence to SOP-dictated time for processing to plasma or serum and/or time to storage of whole blood at 4 °C is now feasible. This novel quality assessment step could enable scientists to uncover common preanalytical errors, allowing for identification of serum and plasma samples that should be excluded from certain investigations. It should also allow control of samples before long-term storage in biobanks. © 2018 American Association for Clinical Chemistry.
URI
http://hdl.handle.net/11615/75966
Colecciones
  • Δημοσιεύσεις σε περιοδικά, συνέδρια, κεφάλαια βιβλίων κλπ. [19735]

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