Our aim is to develop a DNA sequencing device based upon the blockade of ionic current in the transmembrane protein pore alpha-hemolysin (aHL). Compared to other proposed nanopore-based approaches, the protein pore current blockade (PPCB) method is arguably the simplest, both conceptually and technologically, but recently has been passed over in favor of more complex methods. Recent electronic readout and bilayer lipid membrane advances by the proposers have greatly alleviated prior signal-to-noise ratio and robustness issues. New experimental data and an accurate Stochastic Model for DNA Motion (SMDM) within aHL now indicate threshold feasibility for sequencing by the PPCB method. Inspection of calculated SMDM responses to known input DNA sequences shows that the principal issue for sequencing via the PPCB method is random variance in the order the bases pass through the pore, leading to three quantifiable sources of error. This program will make specific structural and measurement parameter modifications to the present apparatus to reduce each type of error and to produce a minimal overall sequencing error. The final apparatus will be evaluated by sequencing kilobase strands of natural DNA

Public Health Relevance

This project offers a path to low cost DNA sequencing. Determining the DNA sequence is useful in basic research studying fundamental biological processes, as well as in applied fields such as diagnostic or forensic research. The advent of DNA sequencing has significantly accelerated biological research and discovery, but current methods are complicated and expensive, thus limiting their applicability. Simple, inexpensive DNA sequencing offers the capability to apply the benefits of the process to everyday medical and forensic applications.

Agency
National Institute of Health (NIH)
Institute
National Human Genome Research Institute (NHGRI)
Type
Research Project (R01)
Project #
1R01HG005095-01
Application #
7714702
Study Section
Special Emphasis Panel (ZHG1-HGR-N (M1))
Program Officer
Schloss, Jeffery
Project Start
2009-09-01
Project End
2013-06-30
Budget Start
2009-09-01
Budget End
2010-06-30
Support Year
1
Fiscal Year
2009
Total Cost
$961,514
Indirect Cost
Name
Electronic Biosciences, Inc.
Department
Type
DUNS #
129852864
City
San Diego
State
CA
Country
United States
Zip Code
92121
De Biase, Pablo M; Ervin, Eric N; Pal, Prithwish et al. (2016) What controls open-pore and residual currents in the first sensing zone of alpha-hemolysin nanopore? Combined experimental and theoretical study. Nanoscale 8:11571-9
De Biase, Pablo M; Markosyan, Suren; Noskov, Sergei (2015) BROMOC suite: Monte Carlo/Brownian dynamics suite for studies of ion permeation and DNA transport in biological and artificial pores with effective potentials. J Comput Chem 36:264-71
Markosyan, Suren; De Biase, Pablo M; Czapla, Luke et al. (2014) Effect of confinement on DNA, solvent and counterion dynamics in a model biological nanopore. Nanoscale 6:9006-16
Ervin, Eric N; Barrall, Geoffrey A; Pal, Prithwish et al. (2014) Creating a Single Sensing Zone within an Alpha-Hemolysin Pore Via Site Directed Mutagenesis. Bionanoscience 4:78-84
De Biase, Pablo M; Markosyan, Suren; Noskov, Sergei (2014) Microsecond simulations of DNA and ion transport in nanopores with novel ion-ion and ion-nucleotides effective potentials. J Comput Chem 35:711-21
Wang, Guihua; Wang, Liang; Han, Yujing et al. (2014) Nanopore detection of copper ions using a polyhistidine probe. Biosens Bioelectron 53:453-8
Wolna, Anna H; Fleming, Aaron M; An, Na et al. (2013) Electrical Current Signatures of DNA Base Modifications in Single Molecules Immobilized in the ?-Hemolysin Ion Channel. Isr J Chem 53:417-430
Wang, Guihua; Zhao, Qitao; Kang, Xiaofeng et al. (2013) Probing mercury(II)-DNA interactions by nanopore stochastic sensing. J Phys Chem B 117:4763-9
Jin, Qian; Fleming, Aaron M; Burrows, Cynthia J et al. (2012) Unzipping kinetics of duplex DNA containing oxidized lesions in an *-hemolysin nanopore. J Am Chem Soc 134:11006-11
An, Na; White, Henry S; Burrows, Cynthia J (2012) Modulation of the current signatures of DNA abasic site adducts in the ýý-hemolysin ion channel. Chem Commun (Camb) 48:11410-2

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