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Improved quality of 1H NMR spectroscopic data for enhanced metabolic profiling of low molecular weight metabolites in human serum Authors Authors and affiliations

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dc.contributor.author Stolzenburg, Svenja
dc.contributor.author Lauridsen, Micheal B.
dc.contributor.author Toft, Henrik
dc.contributor.author Zalloua, Pierre A.
dc.contributor.author Baunsgaard, Dorrit
dc.date.accessioned 2019-07-22T07:29:15Z
dc.date.available 2019-07-22T07:29:15Z
dc.date.copyright 2011 en_US
dc.date.issued 2019-07-22
dc.identifier.issn 1573-3890 en_US
dc.identifier.uri http://hdl.handle.net/10725/11116
dc.description.abstract NMR based metabolic profiling of blood samples in epidemiological studies can be used for molecular phenotyping and biomarker discovery. Often metabolic changes in blood are more subtle and demand a high quality spectrum especially when looking at low molecular weight compounds. In order to improve 1H NMR spectroscopic data we compared different serum sample preparation methods. Application of phosphate buffer reduces chemical shift variation, enhances resolution of signal multiplicity, facilitates visual inspection of NMR spectra and annotation of signals compared to traditionally used saline. For analysis of low molecular weight compounds we found that standard 1D spectra of ultrafiltrated serum samples show enhanced spectral quality of small metabolites as compared to transverse relaxation edited spectra (also called Carr–Purcell–Meiboom–Gill, CPMG) spectra of unfiltered serum samples due to improved signal-to-noise ratio. Thus, NMR signals attributable to different amino acids and other small metabolites could readily be detected in spectra of ultrafiltrated serum, but remained invisible in the corresponding CPMG spectra. An OPLS model of fasting blood glucose showed an increase of Q2 when using spectra from ultrafiltrated serum (Q2 = 0.261) compared to using CPMG spectra (Q2 = 0.173). Similar results were observed for OPLS models of BMI (Q2 = 0.253 and Q2 = 0.216, respectively). Furthermore, a reduction in model dimensionality was observed when using ultrafiltrated serum data. In conclusion we recommend sample preparation of serum samples in phosphate buffer instead of saline. Ultrafiltration of serum samples prior to NMR analysis is beneficial especially for low concentrated small metabolites. en_US
dc.language.iso en en_US
dc.title Improved quality of 1H NMR spectroscopic data for enhanced metabolic profiling of low molecular weight metabolites in human serum Authors Authors and affiliations en_US
dc.type Article en_US
dc.description.version Published en_US
dc.author.school SOM en_US
dc.author.idnumber 20030001 en_US
dc.author.department N/A en_US
dc.description.embargo N/A en_US
dc.relation.journal Metabolomics en_US
dc.journal.volume 7 en_US
dc.journal.issue 2 en_US
dc.article.pages 270-277 en_US
dc.identifier.doi https://doi.org/10.1007/s11306-010-0248-1 en_US
dc.identifier.ctation Stolzenburg, S., Lauridsen, M. B., Toft, H., Zalloua, P. A., & Baunsgaard, D. (2011). Improved quality of 1 H NMR spectroscopic data for enhanced metabolic profiling of low molecular weight metabolites in human serum. Metabolomics, 7(2), 270-277. en_US
dc.author.email pierre.zalloua@lau.edu.lb en_US
dc.identifier.tou http://libraries.lau.edu.lb/research/laur/terms-of-use/articles.php en_US
dc.identifier.url https://link.springer.com/article/10.1007/s11306-010-0248-1 en_US
dc.orcid.id https://orcid.org/0000-0002-8494-5081 en_US
dc.author.affiliation Lebanese American University en_US


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