Bioanalytical method for NAD<sup>+</sup> detection in blood plasma utilizing solution-phase Candida boidinii formate dehydrogenase and electrochemical detection

Taron W.; Kasemphong T.; Sunon P.; Kaewket K.; Kamonsutthipaijit N.; Ketudat-Cairns J.R.; Bhakdisongkhram G.; Tulalamba W.; Sanguansuk S.; Viprakasit V.; Ngamchuea K.

Bioanalytical method for NAD<sup>+</sup> detection in blood plasma utilizing solution-phase Candida boidinii formate dehydrogenase and electrochemical detection

dc.contributor.author	Taron W.
dc.contributor.author	Kasemphong T.
dc.contributor.author	Sunon P.
dc.contributor.author	Kaewket K.
dc.contributor.author	Kamonsutthipaijit N.
dc.contributor.author	Ketudat-Cairns J.R.
dc.contributor.author	Bhakdisongkhram G.
dc.contributor.author	Tulalamba W.
dc.contributor.author	Sanguansuk S.
dc.contributor.author	Viprakasit V.
dc.contributor.author	Ngamchuea K.
dc.contributor.correspondence	Taron W.
dc.contributor.other	Mahidol University
dc.date.accessioned	2025-02-13T18:34:24Z
dc.date.available	2025-02-13T18:34:24Z
dc.date.issued	2025-01-01
dc.description.abstract	Nicotinamide adenine dinucleotide is a crucial coenzyme in cellular metabolism and is implicated in various diseases. This work introduces an electrochemical bioanalytical method utilizing solution-phase Candida boidinii formate dehydrogenase (CbFDH) for detecting its oxidized form (NAD+) in human blood plasma samples. The detection mechanism involves the catalytic conversion of NAD+ to NADH, facilitated by CbFDH in the presence of formate. This NADH is then quantified by electrochemical measurements at disposable carbon screen-printed electrodes. The reaction is completed within one minute. The assay exhibits a linear response range from 3.74 μM to 2.00 mM, a sensitivity of 8.98 ± 0.18 μA mM−1, and a limit of detection (3sb/m) of 1.12 μM. It demonstrates selectivity against common interferences found in plasma samples, including glucose, urea, creatinine, guanosine 5′-monophosphate, cytidine 5′-monophosphate, flavin adenine dinucleotide, adenosine 5′-triphosphate, and lactate, with interference levels below 5% relative to the unperturbed NAD+ signal. Recovery studies showed 98.0-104.4% recoveries, with further validation against a colorimetric alcohol dehydrogenase assay confirming accuracy in plasma samples.
dc.identifier.citation	Analyst (2025)
dc.identifier.doi	10.1039/d4an01560f
dc.identifier.eissn	13645528
dc.identifier.issn	00032654
dc.identifier.scopus	2-s2.0-85216970010
dc.identifier.uri	https://repository.li.mahidol.ac.th/handle/20.500.14594/105281
dc.rights.holder	SCOPUS
dc.subject	Chemistry
dc.subject	Environmental Science
dc.subject	Biochemistry, Genetics and Molecular Biology
dc.title	Bioanalytical method for NAD<sup>+</sup> detection in blood plasma utilizing solution-phase Candida boidinii formate dehydrogenase and electrochemical detection
dc.type	Article
mu.datasource.scopus	https://www.scopus.com/inward/record.uri?partnerID=HzOxMe3b&scp=85216970010&origin=inward
oaire.citation.title	Analyst
oairecerif.author.affiliation	Siriraj Hospital
oairecerif.author.affiliation	Suranaree University of Technology
oairecerif.author.affiliation	ATGenes Limited Company
oairecerif.author.affiliation	Synchrotron Light Research Institute

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Bioanalytical method for NAD<sup>+</sup> detection in blood plasma utilizing solution-phase Candida boidinii formate dehydrogenase and electrochemical detection

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