A dual-constriction biological nanopore resolves homonucleotide sequences with high fidelity

Single-molecule long-read DNA sequencing with biological nanopores is fast and high-throughput but suffers reduced accuracy in homonucleotide stretches. We now combine the CsgG nanopore with the 35-residue N-terminal region of its extracellular interaction partner CsgF to produce a dual-constriction...

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Veröffentlicht in:Nature biotechnology 2020-12, Vol.38 (12), p.1415-1420
Hauptverfasser: Van der Verren, Sander E., Van Gerven, Nani, Jonckheere, Wim, Hambley, Richard, Singh, Pratik, Kilgour, John, Jordan, Michael, Wallace, E. Jayne, Jayasinghe, Lakmal, Remaut, Han
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Sprache:eng
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Zusammenfassung:Single-molecule long-read DNA sequencing with biological nanopores is fast and high-throughput but suffers reduced accuracy in homonucleotide stretches. We now combine the CsgG nanopore with the 35-residue N-terminal region of its extracellular interaction partner CsgF to produce a dual-constriction pore with improved signal and base-calling accuracy for homopolymer regions. The electron cryo-microscopy structure of CsgG in complex with full-length CsgF shows that the 33 N-terminal residues of CsgF bind inside the β-barrel of the pore, forming a defined second constriction. In complexes of CsgG bound to a 35-residue CsgF constriction peptide, the second constriction is separated from the primary constriction by ~25 Å. We find that both constrictions contribute to electrical signal modulation during single-stranded DNA translocation. DNA sequencing using a prototype CsgG–CsgF protein pore with two constrictions improved single-read accuracy by 25 to 70% in homopolymers up to 9 nucleotides long. Equipping a protein nanopore with a second constriction improves sequencing of homopolymer DNA stretches.
ISSN:1087-0156
1546-1696
DOI:10.1038/s41587-020-0570-8