Literature DB >> 20436924

On the Feasibility of Using the Intrinsic Fluorescence of Nucleotides for DNA Sequencing.

Mustafa H Chowdhury1, Krishanu Ray, Michael L Johnson, Stephen K Gray, James Pond, Joseph R Lakowicz.   

Abstract

There is presently a worldwide effort to increase the speed and decrease the cost of DNA sequencing as exemplified by the goal of the National Human Genome Research Institute (NHGRI) to sequence a human genome for under $1000. Several high throughput technologies are under development. Among these, single strand sequencing using exonuclease appear very promising. However, this approach requires complete labeling of at least two bases at a time, with extrinsic high quantum yield probes. This is necessary because nucleotides absorb in the deep ultra-violet (UV) and emit with extremely low quantum yields. Hence intrinsic emission from DNA and nucleotides is not being exploited for DNA sequencing. In the present paper we consider the possibility of identifying single nucleotides using their intrinsic emission. We used the finite-difference time-domain (FDTD) method to calculate the effects of aluminum nanoparticles on nearby fluorophores that emit in the UV. We find that the radiated power of UV fluorophores is significantly increased when they are in close proximity to aluminum nanostructures. We show that there will be increased localized excitation near aluminum particles at wavelengths used to excite intrinsic nucleotide emission. Using FDTD simulation we show that a typical DNA base when coupled to appropriate aluminum nanostructures leads to highly directional emission. Additionally we present experimental results showing that a thin film of nucleotides show enhanced emission when in close proximity to aluminum nanostructures. Finally we provide Monte Carlo simulations that predict high levels of base calling accuracy for an assumed number of photons that is derived from the emission spectra of the intrinsic fluorescence of the bases. Our results suggest that single nucleotides can be detected and identified using aluminum nanostructures that enhance their intrinsic emission. This capability would be valuable for the ongoing efforts towards the $1000 genome.

Entities:  

Year:  2010        PMID: 20436924      PMCID: PMC2860747          DOI: 10.1021/jp911229c

Source DB:  PubMed          Journal:  J Phys Chem C Nanomater Interfaces        ISSN: 1932-7447            Impact factor:   4.126


  34 in total

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6.  A system for rapid DNA sequencing with fluorescent chain-terminating dideoxynucleotides.

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7.  Fluorescently labeled model DNA sequences for exonucleolytic sequencing.

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8.  Single-molecule sequencing of an individual human genome.

Authors:  Dmitry Pushkarev; Norma F Neff; Stephen R Quake
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9.  Radiative decay engineering 5: metal-enhanced fluorescence and plasmon emission.

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10.  Aluminum nanoparticles as substrates for metal-enhanced fluorescence in the ultraviolet for the label-free detection of biomolecules.

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  4 in total

1.  Feasibility of Using Bimetallic Plasmonic Nanostructures to Enhance the Intrinsic Emission of Biomolecules.

Authors:  Mustafa H Chowdhury; Sudipto Chakraborty; Joseph R Lakowicz; Krishanu Ray
Journal:  J Phys Chem C Nanomater Interfaces       Date:  2011-09-01       Impact factor: 4.126

2.  Ensemble and Single Molecule Studies on the Use of Metallic Nanostructures to Enhance the Intrinsic Emission of Enzyme Cofactors.

Authors:  Mustafa H Chowdhury; Joseph R Lakowicz; Krishanu Ray
Journal:  J Phys Chem C Nanomater Interfaces       Date:  2011-04-21       Impact factor: 4.126

3.  Metallic-Nanostructure-Enhanced Fluorescence of Single Flavin Cofactor and Single Flavoenzyme Molecules.

Authors:  Yi Fu; Jian Zhang; Joseph R Lakowicz
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4.  The use of aluminum nanostructures as platforms for metal enhanced fluorescence of the intrinsic emission of biomolecules in the ultra-violet.

Authors:  Mustafa H Chowdhury; Krishanu Ray; Stephen K Gray; James Pond; Joseph R Lakowicz
Journal:  Proc SPIE Int Soc Opt Eng       Date:  2010-02
  4 in total

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