Fast enzyme-linked electrochemical sensing of DNA hybridization at pencil graphite electrodes. Application to detect gene deletion in a human cell culture

Špaček, Jan; Eksin, E.; Havran, Luděk; Erdem, A.; Fojta, Miroslav

doi:https://dx.doi.org/10.1016/j.jelechem.2020.113951

Počet záznamů: 1

Fast enzyme-linked electrochemical sensing of DNA hybridization at pencil graphite electrodes. Application to detect gene deletion in a human cell culture

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SYSNO ASEP	0524530
Druh ASEP	J - Článek v odborném periodiku
Zařazení RIV	J - Článek v odborném periodiku
Poddruh J	Článek ve WOS
Název	Fast enzyme-linked electrochemical sensing of DNA hybridization at pencil graphite electrodes. Application to detect gene deletion in a human cell culture
Tvůrce(i)	Špaček, Jan (BFU-R)_ORCID Eksin, E. (TR) Havran, Luděk (BFU-R)_{RID, ORCID} Erdem, A. (TR) Fojta, Miroslav (BFU-R)_{RID, ORCID}
Celkový počet autorů	5
Číslo článku	113951
Zdroj.dok.	Journal of Electroanalytical Chemistry. - : Elsevier - ISSN 1572-6657 Roč. 862, APR 1 2020 (2020)
Poč.str.	7 s.
Forma vydání	Online - E
Jazyk dok.	eng - angličtina
Země vyd.	CH - Švýcarsko
Klíč. slova	single nucleotide polymorphisms ; sensitive detection ; genomagnetic assay ; pcr products ; biosensor
Vědní obor RIV	CG - Elektrochemie
Obor OECD	Electrochemistry (dry cells, batteries, fuel cells, corrosion metals, electrolysis)
CEP	GAP206/11/1638 GA ČR - Grantová agentura ČR
Způsob publikování	Omezený přístup
Institucionální podpora	BFU-R - RVO:68081707
UT WOS	000525903900004
EID SCOPUS	85080093599
DOI	10.1016/j.jelechem.2020.113951
Anotace	In this paper we present a rapid electrochemical enzyme-linked DNA hybridization assay using disposable pencil graphite electrodes (PeGE) to detect target DNA (tDNA) sequences in DNA fragments amplified by polymerase chain reaction. The procedure consists of several short (1-2 min) incubation steps, including adsorption of the tDNA at unpretreated PeGE from denaturing medium, surface blocking with milk proteins, hybridization with a biotinylated oligonucleotide probe and binding of streptavidin-alkaline phosphatase conjugate to the biotin tags. Then the PeGE is transferred into background electrolyte solution containing 1-naphthyl phosphate, which is enzymatically dephosphorylated to give electrochemically oxidizable indicator 1-naphthol. The assay, which can be performed within 7-8 min, offers a perfect discrimination between specific and nonspecific DNA amplicons and easy detection of about similar to 40 femtomoles of tDNA in large excesses of non-complementary DNA. An application on the detection of p53 gene deletion in a human cell culture, featuring a real biologicalmodel, is presented. The designed setup has a potential to be applied as one of simple, fast, robust ultralow cost do-it-yourself instruments recently introduced as diagnostic tools for third world countries. (c) 2020 Elsevier B.V. All rights reserved.
Pracoviště	Biofyzikální ústav
Kontakt	Jana Poláková, polakova@ibp.cz, Tel.: 541 517 244
Rok sběru	2021
Elektronická adresa	https://www.sciencedirect.com/science/article/pii/S157266572030134X?via%3Dihub

Počet záznamů: 1