High-sensitivity, protein-independent detection of dsDNA sequences

dc.contributor.authorYan, Jiaqi
dc.contributor.authorBhadane, Rajendra
dc.contributor.authorXu, Wentao
dc.contributor.authorRan, Meixin
dc.contributor.authorMa, Xiaochao
dc.contributor.authorLi, Yuanqiang
dc.contributor.authorJahnke, Kevin
dc.contributor.authorMa, Xiaodong
dc.contributor.authorSalo-Ahen, Outi M. H.
dc.contributor.authorKostiainen, Mauri A.
dc.contributor.authorWeitz, David A.
dc.contributor.authorZhang, Hongbo
dc.contributor.organizationfi=biolääketieteen laitos|en=Institute of Biomedicine|
dc.contributor.organizationfi=Turun biotiedekeskus|en=Turku Bioscience Centre|
dc.contributor.organization-code1.2.246.10.2458963.20.77952289591
dc.contributor.organization-code2607100
dc.contributor.organization-code1.2.246.10.2458963.20.18586209670
dc.converis.publication-id515634781
dc.converis.urlhttps://research.utu.fi/converis/portal/Publication/515634781
dc.date.accessioned2026-04-24T21:51:19Z
dc.description.abstractCurrent methodologies for detecting the sequence of double-stranded DNA (dsDNA) require amplifying and denaturing the target into single-stranded DNA (ssDNA) to enable sequence detection through Watson-Crick base pairing. However, these approaches are limited by the risks of nonspecific amplification, reliance on complex, temperature-sensitive protein enzymes, and harsh reaction conditions, such as in strong base or acidic environments. Here, we introduce a dsDNA detection platform that integrates a peptide nucleic acid (PNA) as the dsDNA denaturation agent, with multicomponent deoxyribozyme as the ssDNA detection tool, in a droplet-based system. This protein- and amplification-free method offers single-nucleotide resolution, detects down to a single dsDNA molecule, and delivers results within 1 h at room temperature. This work introduces a conceptually unique approach, that may be useful for both diagnostics and therapeutics.
dc.identifier.eissn1091-6490
dc.identifier.jour-issn0027-8424
dc.identifier.urihttps://www.utupub.fi/handle/11111/59800
dc.identifier.urlhttps://doi.org/10.1073/pnas.2515765123
dc.identifier.urnURN:NBN:fi-fe2026042333427
dc.language.isoen
dc.okm.affiliatedauthorBhadane, Rajendra
dc.okm.affiliatedauthorRan, Meixin
dc.okm.affiliatedauthorZhang, Hongbo
dc.okm.discipline3111 Biomedicineen_GB
dc.okm.discipline3111 Biolääketieteetfi_FI
dc.okm.internationalcopublicationinternational co-publication
dc.okm.internationalityInternational publication
dc.okm.typeA1 ScientificArticle
dc.publisherProceedings of the National Academy of Sciences
dc.publisher.countryUnited Statesen_GB
dc.publisher.countryYhdysvallat (USA)fi_FI
dc.publisher.country-codeUS
dc.relation.articlenumbere2515765123
dc.relation.doi10.1073/pnas.2515765123
dc.relation.ispartofjournalProceedings of the National Academy of Sciences of the United States of America
dc.relation.issue6
dc.relation.volume123
dc.titleHigh-sensitivity, protein-independent detection of dsDNA sequences
dc.year.issued2026

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