HPLC and TLC methods for analysis of [F-18]FDG and its metabolites from biological samples

dc.contributor.authorJohanna Rokka
dc.contributor.authorTove J. Grönroos
dc.contributor.authorTapio Viljanen
dc.contributor.authorOlof Solin
dc.contributor.authorMerja Haaparanta-Solin
dc.contributor.organizationfi=MediCity|en=MediCity|
dc.contributor.organizationfi=PET-keskus|en=Turku PET Centre|
dc.contributor.organizationfi=kemian laitos|en=Department of Chemistry|
dc.contributor.organizationfi=tyks, vsshp|en=tyks, varha|
dc.contributor.organization-code1.2.246.10.2458963.20.14646305228
dc.contributor.organization-code1.2.246.10.2458963.20.27622076134
dc.contributor.organization-code2609810
dc.converis.publication-id26432483
dc.converis.urlhttps://research.utu.fi/converis/portal/Publication/26432483
dc.date.accessioned2022-10-28T13:41:53Z
dc.date.available2022-10-28T13:41:53Z
dc.description.abstractThe most used positron emission tomography (PET) tracer, 2-[F-18]fluoro-2-deoxy-o-glucose ([F-18]FDG), is a glucose analogue that is used to measure tissue glucose consumption. Traditionally, the Sokoloff model is the basis for [F-18]FDG modeling. According to this model, [F-18]FDG is expected to be trapped in a cell in the form of [F-18]FDG-6-phosphate ([189FDG-6-P). However, several studies have shown that in tissues, [F-18]FDG metabolism goes beyond [F-18]FDG-6-P. Our aim was to develop radioHPLC and radioTLC methods for analysis of [F-18]FDG metabolites from tissue samples. The radioHPLC method uses a sensitive on-line scintillation detector to detect radioactivity, and the radioTLC method employs digital autoradiography to detect the radioactivity distribution on a TLC plate. The HPLC and TLC methods were developed using enzymatically in vitro-produced metabolites of ["HMG as reference standards. For this purpose, three [F-18]FDG metabolites were synthesized: [F-18]FDG-6-P, [F-18]FD-PGL, and [F-18]FDG-1,6-P2. The two methods were evaluated by analyzing the [F-18]FDG metabolic profile from rodent ex vivo tissue homogenates. The HPLC method with an on-line scintillation detector had a wide linearity in a range of 5 Bq-5 kBq (LOD 46 Bq, LOQ 139 Bq) and a good resolution (Rs > 1.9), and separated [F-18]FDG and its metabolites clearly. The TLC method combined with digital autoradiography had a high sensitivity in a wide range of radioactivity (0.1 Bq-2 kBq, LOD 0.24 Bq, LOQ0.31 Bq), and multiple samples could be analyzed simultaneously. As our test and the method validation with ex vivo samples showed, both methods are useful, and at best they complement each other in analysis of [F-18]FDG and its radioactive metabolites from biological samples. (C) 2017 Elsevier B.V. All rights reserved.
dc.format.pagerange140
dc.format.pagerange149
dc.identifier.jour-issn1570-0232
dc.identifier.olddbid183703
dc.identifier.oldhandle10024/166797
dc.identifier.urihttps://www.utupub.fi/handle/11111/40989
dc.identifier.urnURN:NBN:fi-fe2021042717142
dc.language.isoen
dc.okm.affiliatedauthorRokka, Johanna
dc.okm.affiliatedauthorGrönroos, Tove
dc.okm.affiliatedauthorViljanen, Tapio
dc.okm.affiliatedauthorSolin, Olof
dc.okm.affiliatedauthorHaaparanta-Solin, Merja
dc.okm.affiliatedauthorDataimport, MediCity
dc.okm.affiliatedauthorDataimport, tyks, vsshp
dc.okm.discipline3126 Surgery, anesthesiology, intensive care, radiologyen_GB
dc.okm.discipline3126 Kirurgia, anestesiologia, tehohoito, radiologiafi_FI
dc.okm.internationalcopublicationnot an international co-publication
dc.okm.internationalityInternational publication
dc.okm.typeA1 ScientificArticle
dc.publisherELSEVIER SCIENCE BV
dc.publisher.countryNetherlandsen_GB
dc.publisher.countryAlankomaatfi_FI
dc.publisher.country-codeNL
dc.relation.doi10.1016/j.jchromb.2017.01.042
dc.relation.ispartofjournalJournal of Chromatography B
dc.relation.volume1048
dc.source.identifierhttps://www.utupub.fi/handle/10024/166797
dc.titleHPLC and TLC methods for analysis of [F-18]FDG and its metabolites from biological samples
dc.year.issued2017

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