4.8 Article

DNA translocation through an array of kinked nanopores

Journal

NATURE MATERIALS
Volume 9, Issue 8, Pages 667-675

Publisher

NATURE PUBLISHING GROUP
DOI: 10.1038/NMAT2805

Keywords

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Funding

  1. Air Force Office of Scientific Research [FA 9550-10-1-0054]
  2. DOE Basic Energy Sciences [DE-FG02-02-ER15368]
  3. US Department of Energy, Office of Basic Energy Sciences, Division of Materials Sciences and Engineering
  4. US Department of Energy, Office of Science, Office of Basic Energy Sciences [DE-AC02-06CH11357]
  5. US Department of Energy's National Nuclear Security Administration [DE-AC04-94AL85000]
  6. Direct For Computer & Info Scie & Enginr
  7. Division of Computing and Communication Foundations [0915718] Funding Source: National Science Foundation
  8. Directorate For Engineering
  9. Div Of Chem, Bioeng, Env, & Transp Sys [0852657] Funding Source: National Science Foundation
  10. Division of Computing and Communication Foundations
  11. Direct For Computer & Info Scie & Enginr [0810294] Funding Source: National Science Foundation

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Synthetic solid-state nanopores are being intensively investigated as single-molecule sensors for detection and characterization of DNA, RNA and proteins. This field has been inspired by the exquisite selectivity and flux demonstrated by natural biological channels and the dream of emulating these behaviours in more robust synthetic materials that are more readily integrated into practical devices. So far, the guided etching of polymer films, focused ion-beam sculpting, and electron-beam lithography and tuning of silicon nitride membranes have emerged as three promising approaches to define synthetic solid-state pores with sub-nanometre resolution. These procedures have in common the formation of nominally cylindrical or conical pores aligned normal to the membrane surface. Here we report the formation of 'kinked' silica nanopores, using evaporation-induced self-assembly, and their further tuning and chemical derivatization using atomic-layer deposition. Compared with 'straight through' proteinaceous nanopores of comparable dimensions, kinked nanopores exhibit up to fivefold reduction in translocation velocity, which has been identified as one of the critical issues in DNA sequencing. Additionally, we demonstrate an efficient two-step approach to create a nanopore array exhibiting nearly perfect selectivity for ssDNA over dsDNA. We show that a coarse-grained drift-diffusion theory with a sawtooth-like potential can reasonably describe the velocity and translocation time of DNA through the pore. By control of pore size, length and shape, we capture the main functional behaviours of protein pores in our solid-state nanopore system.

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