Uracil base PCR implemented for reliable DNA walking
PCR-based DNA walking is of efficacy for capturing unknown flanking genomic sequences. Here, an uracil base PCR (UB-PCR) with satisfying specificity has been devised for DNA walking. Primary UB-PCR replaces thymine base with uracil base, resulting in a primary PCR product composed of U-DNAs. A singl...
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Veröffentlicht in: | Analytical biochemistry 2025-01, Vol.696, p.115697, Article 115697 |
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Sprache: | eng |
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Zusammenfassung: | PCR-based DNA walking is of efficacy for capturing unknown flanking genomic sequences. Here, an uracil base PCR (UB-PCR) with satisfying specificity has been devised for DNA walking. Primary UB-PCR replaces thymine base with uracil base, resulting in a primary PCR product composed of U-DNAs. A single-primer (primary nested sequence-specific primer) single-cycle amplification, using the four normal bases (adenine, thymine, cytosine, and guanine) as substrate, is then performed on the primary PCR product. Clearly, only those U-DNAs, ended by the primary nested sequence-specific primer at least at one side, will produce the corresponding normal single strands. Next, the single-cycle product undergoes uracil-DNA glycosylase treatment to destroy the U-DNAs, while the normal single strands are unaffected. Afterward, secondary even tertiary PCR is performed to exclusively enrich the target product. The feasibility of UB-PCR has been checked by obtaining unknown sequences bordering the three selected genetic sites.
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•Primary UB-PCR uses dUTP instead of dTTP as substrate.•The single-primer single-cycle PCR only replicates a U-DNA with pnSSP site(s).•UNG treatment improves the specificity of UB-PCR.•Two rounds of UB-PCRs can generally produce a wanted walking result. |
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ISSN: | 0003-2697 1096-0309 1096-0309 |
DOI: | 10.1016/j.ab.2024.115697 |