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AuthorKalinina, Sviatlanadc.contributor.author
AuthorFreymueller, Christiandc.contributor.author
AuthorNaskar, Nilanjondc.contributor.author
Authorvon Einem, Bjoerndc.contributor.author
AuthorReess, Kirstendc.contributor.author
AuthorSroka, Ronalddc.contributor.author
AuthorRueck, Angelikadc.contributor.author
Date of accession2023-03-15T15:37:45Zdc.date.accessioned
Available in OPARU since2023-03-15T15:37:45Zdc.date.available
Date of first publication2021-05-31dc.date.issued
AbstractMetabolic FLIM (fluorescence lifetime imaging) is used to image bioenergetic status in cells and tissue. Whereas an attribution of the fluorescence lifetime of coenzymes as an indicator for cell metabolism is mainly accepted, it is debated whether this is valid for the redox state of cells. In this regard, an innovative algorithm using the lifetime characteristics of nicotinamide adenine dinucleotide (phosphate) (NAD(P)H) and flavin adenine dinucleotide (FAD) to calculate the fluorescence lifetime induced redox ratio (FLIRR) has been reported so far. We extended the FLIRR approach and present new results, which includes FLIM data of the various enzymes, such as NAD(P)H, FAD, as well as flavin mononucleotide (FMN). Our algorithm uses a two-exponential fitting procedure for the NAD(P)H autofluorescence and a three-exponential fit of the flavin signal. By extending the FLIRR approach, we introduced FLIRR1 as protein-bound NAD(P)H related to protein-bound FAD, FLIRR2 as protein-bound NAD(P)H related to free (unbound) FAD and FLIRR3 as protein-bound NAD(P)H related to protein-bound FMN. We compared the significance of extended FLIRR to the metabolic index, defined as the ratio of protein-bound NAD(P)H to free NAD(P)H. The statistically significant difference for tumor and normal cells was found to be highest for FLIRR1.dc.description.abstract
Languageendc.language.iso
PublisherUniversität Ulmdc.publisher
LicenseCC BY 4.0 Internationaldc.rights
Link to license texthttps://creativecommons.org/licenses/by/4.0/dc.rights.uri
KeywordFLIMdc.subject
KeywordFADdc.subject
KeywordFMNdc.subject
KeywordNAD(P)H metabolic indexdc.subject
KeywordFLIRR indexdc.subject
Keywordextended FLIRRdc.subject
KeywordOXPHOSdc.subject
Dewey Decimal GroupDDC 570 / Life sciencesdc.subject.ddc
LCSHNAD(P)H dehydrogenasesdc.subject.lcsh
LCSHCell metabolismdc.subject.lcsh
LCSHGlycolysisdc.subject.lcsh
TitleBioenergetic alterations of metabolic redox coenzymes as NADH, FAD and FMN by means of fluorescence lifetime imaging techniquesdc.title
Resource typeWissenschaftlicher Artikeldc.type
SWORD Date2022-09-06T13:34:45Zdc.date.updated
VersionpublishedVersiondc.description.version
DOIhttp://dx.doi.org/10.18725/OPARU-47787dc.identifier.doi
URNhttp://nbn-resolving.de/urn:nbn:de:bsz:289-oparu-47863-5dc.identifier.urn
GNDNitratreduktase (NAD(P)H)dc.subject.gnd
GNDGlykolysedc.subject.gnd
FacultyMedizinische Fakultätuulm.affiliationGeneral
InstitutionZentrum für Translationale Bildgebung (MoMAN)uulm.affiliationSpecific
Peer reviewjauulm.peerReview
DCMI TypeTextuulm.typeDCMI
CategoryPublikationenuulm.category
DOI of original publication10.3390/ijms22115952dc.relation1.doi
Source - Title of sourceInternational Journal of Molecular Sciencessource.title
Source - Place of publicationMDPIsource.publisher
Source - Volume22source.volume
Source - Issue11source.issue
Source - Year2021source.year
Source - Article number5952source.articleNumber
Source - eISSN1422-0067source.identifier.eissn
WoS000660166900001uulm.identifier.wos
Bibliographyuulmuulm.bibliographie
Is Supplemented Byhttps://www.mdpi.com/article/10.3390/ijms22115952/s1dc.relation.isSupplementedBy
Project uulmOMOXI / Verbundprojekt: Endoskopisches, optisches Imaging von Zellmetabolismus und Sauerstoffkonzentration für Diagnostik, Therapiemonitoring und Therapiekontrolle (OMOXI) - Teilvorhaben: Korrelation von OMI und Sauerstoff-Imaging in Zellmodellen für theragnostische Anwendungen im HNO-Bereich / BMBF / 13N14508uulm.projectOther


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