Targeted and Untargeted Amine Metabolite Quantitation in Single Cells with Isobaric Multiplexing

dc.contributor.authorHeininen, Juho
dc.contributor.authorMovahedi, Parisa
dc.contributor.authorKotiaho, Tapio
dc.contributor.authorKostiainen, Risto
dc.contributor.authorPahikkala, Tapio
dc.contributor.authorTeppo, Jaakko
dc.contributor.organizationfi=data-analytiikka|en=Data-analytiikka|
dc.contributor.organizationfi=terveysteknologia|en=Health Technology|
dc.contributor.organization-code1.2.246.10.2458963.20.28696315432
dc.contributor.organization-code1.2.246.10.2458963.20.68940835793
dc.converis.publication-id459037549
dc.converis.urlhttps://research.utu.fi/converis/portal/Publication/459037549
dc.date.accessioned2025-08-27T23:25:24Z
dc.date.available2025-08-27T23:25:24Z
dc.description.abstract<p>We developed a single cell amine analysis approach utilizing isobarically multiplexed samples of 6 individual cells along with analyte abundant carrier. This methodology was applied for absolute quantitation of amino acids and untargeted relative quantitation of amines in a total of 108 individual cells using nanoflow LC with high-resolution mass spectrometry. Together with individually determined cell sizes, this provides quantification of intracellular concentrations within individual cells. The targeted method was partially validated for 10 amino acids with limits of detection in low attomoles, linear calibration range covering analyte amounts typically from 30 amol to 120 fmol, and correlation coefficients (R) above 0.99. This was applied with cell sizes recorded during dispensing to determine millimolar intracellular amino acid concentrations. The untargeted approach yielded 249 features that were detected in at least 25% of the single cells, providing modest cell type separation on principal component analysis. Using Greedy forward selection with regularized least squares, a sub-selection of 100 features explaining most of the difference was determined. These features were annotated using MS2 from analyte standards and accurate mass with library search. The approach provides accessible, sensitive, and high-throughput method with the potential to be expanded also to other forms of ultrasensitive analysis.</p>
dc.identifier.eissn1521-3765
dc.identifier.jour-issn0947-6539
dc.identifier.olddbid203938
dc.identifier.oldhandle10024/186965
dc.identifier.urihttps://www.utupub.fi/handle/11111/51480
dc.identifier.urlhttps://doi.org/10.1002/chem.202403278
dc.identifier.urnURN:NBN:fi-fe2025082786258
dc.language.isoen
dc.okm.affiliatedauthorMovahedi, Parisa
dc.okm.affiliatedauthorPahikkala, Tapio
dc.okm.discipline116 Chemical sciencesen_GB
dc.okm.discipline3111 Biomedicineen_GB
dc.okm.discipline317 Pharmacyen_GB
dc.okm.discipline116 Kemiafi_FI
dc.okm.discipline3111 Biolääketieteetfi_FI
dc.okm.discipline317 Farmasiafi_FI
dc.okm.internationalcopublicationnot an international co-publication
dc.okm.internationalityInternational publication
dc.okm.typeA1 ScientificArticle
dc.publisherWiley-VCH
dc.publisher.countryGermanyen_GB
dc.publisher.countrySaksafi_FI
dc.publisher.country-codeDE
dc.relation.articlenumbere202403278
dc.relation.doi10.1002/chem.202403278
dc.relation.ispartofjournalChemistry - A European Journal
dc.relation.issue72
dc.relation.volume30
dc.source.identifierhttps://www.utupub.fi/handle/10024/186965
dc.titleTargeted and Untargeted Amine Metabolite Quantitation in Single Cells with Isobaric Multiplexing
dc.year.issued2024

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