A rapid field-use assay for mismatch number and location of hybridized DNAs

Cheng, I-Fang; Senapati, Satyajyoti; Cheng, Xinguang; Basuray, Sagnik; Chang, Hsien-Chang; Chang, Hsueh‐Chia

doi:10.1039/b925854j

Cited by 63 publications

(58 citation statements)

References 19 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…21,22 The resulting temperature gradients cause bulk electrothermal flow, which can dissipate the DEP trapping. Strategies for enhancing the net trapping force on nanoscale biomolecules over dissipative fluid flow due to Joule heating include the application of DEP to DNA immobilized on nanoparticles 23,24 or applying DEP towards the direct manipulation of DNA within devices containing sharp insulating tips or constrictions to enhance field gradients (E.dE/dx or rE 2 ). In our recent work, 25 we have extended this latter approach by coupling the dielectric constriction to an electrically floating electrode with immobilized DNA capture probes to enable low frequency ($1 KHz) DEP trapping of ss-DNA target ($150 bases) in high conductivity saline media (r m $ 1 S/m), without electrolysis.…”

Section: Introductionmentioning

confidence: 99%

Floating-electrode enhanced constriction dielectrophoresis for biomolecular trapping in physiological media of high conductivity

et al. 2012

View full text Add to dashboard Cite

We present an electrokinetic framework for designing insulator constriction-based dielectrophoresis devices with enhanced ability to trap nanoscale biomolecules in physiological media of high conductivity, through coupling short-range dielectrophoresis forces with long-range electrothermal flow. While a 500-fold constriction enables field focusing sufficient to trap nanoscale biomolecules by dielectrophoresis, the extent of this high-field region is enhanced through coupling the constriction to an electrically floating sensor electrode at the constriction floor. However, the enhanced localized fields due to the constriction and enhanced current within saline media of high conductivity (1 S/m) cause a rise in temperature due to Joule heating, resulting in a hotspot region midway within the channel depth at the constriction center, with temperatures of $8 -10 K above the ambient. While the resulting vortices from electrothermal flow are directed away from the hotspot region to oppose dielectrophoretic trapping, they also cause a downward and inward flow towards the electrode edges at the constriction floor. This assists biomolecular trapping at the sensor electrode through enabling long-range fluid sampling as well as through localized stirring by fluid circulation in its vicinity.

show abstract

Section: Introductionmentioning

confidence: 99%

Floating-electrode enhanced constriction dielectrophoresis for biomolecular trapping in physiological media of high conductivity

et al. 2012

View full text Add to dashboard Cite

show abstract

“…Fundamental improvements in analytical science must be implemented before such biomarker detection is feasible. The dielectrophoretic concentration method does not apply to small molecules, such as peptides, because of the small intensities of their induced dipoles, 4 unless this method is conducted in laboriously fabricated nanochannels. 6 Other analyte concentration techniques based on electrokinetic mechanisms have been suggested.…”

Section: Introductionmentioning

confidence: 99%

Selective dynamic concentration of peptides at poles of cation-selective nanoporous granules

et al. 2013

Self Cite

View full text Add to dashboard Cite

The authors exposed a non-equilibrium dynamic counterion and coion analyte concentration to an AC electric field to selectively concentrate peptides at the poles of a cation-selective granule. The counterion polarization results from the focusing of the electric field show a discontinuous drop in the intra-granule counterion electromigration flux at the pole. The coion concentration polarization is due to the combined external convective and electromigration fluxes toward the pole that neutralize the accumulating counterions. Because the electromigration mobility of the peptide anion analyte depends on the pH, the authors determined a 20 000-fold high concentration factor for a near-neutral pH of 6.0 to 7.7. Because the peptide is protonated at the acidic pole and its absolute charge ranges from À0.3 to À1.9, the concentration factor scales exponentially with the absolute charge, thus allowing extremely selective concentrations of various peptides, which is demonstrated by fluorescein isothiocyanate tagged angiotensin I (pI $ 5.8) and Texas red tagged avidin (pI $ 10.5). This dynamic concentration effect can substantially enhance the sensitivity of bio-assays. V C 2013 AIP Publishing LLC. [http://dx

show abstract

“…Induced DC and AC NP dipoles (related to dielectrophoresis) have been used to assemble NP crystals by embedded micro-electrodes to provide the requisite high field. 20,21 The resulting NP crystals are ideal for plasmonic hot spots, since the spacing of the regimented NP crystal can be controlled by the applied voltage. Conic nanocapillaries 22,23 will be used here for such field-induced NP assembly because the submicron-tip can focus the electric field into sufficient high intensity for NP assembly without embedded-electrodes.…”

mentioning

confidence: 99%

“…Strong shear during electrophoretic packing has probably endowed this high selectivity. 20 Using the protocol above, the LOD and dynamic range of the target was determined (Fig. 2(e)).…”

mentioning

confidence: 99%

Plasmonic hotspots of dynamically assembled nanoparticles in nanocapillaries: Towards a micro ribonucleic acid profiling platform

et al. 2013

Self Cite

View full text Add to dashboard Cite

Plasmonic hot spots, generated by controlled 20-nm Au nanoparticle (NP) assembly, are shown to suppress fluorescent quenching effects of metal NPs, such that hair-pin FRET (Fluorescence resonance energy transfer) probes can achieve label-free ultrasensitive quantification. The micron-sized assembly is a result of intense induced NP dipoles by focused electric fields through conic nanocapillaries. The efficient NP aggregate antenna and the voltage-tunable NP spacing for optimizing hot spot intensity endow ultra-sensitivity and large dynamic range (fM to pM). The large shear forces during assembly allow high selectivity (2-mismatch discrimination) and rapid detection (15 min) for a DNA mimic of microRNA. V C 2013 AIP Publishing LLC.[http://dx.doi.org/10.1063/1.4832095] Irregular expressions of a panel of microRNAs (miRNA) in blood and other physiological fluids may allow early diagnosis of many diseases, including cancer and cardiovascular diseases. 1 However, quantifying all relevant miRNAs (out of 1000), with similar sequences over 22 bases 2 and large variations in expression level (as much as 100 fold) at small copy numbers, requires a new molecular diagnostic platform with high-sensitivity, high-selectivity, and large dynamic range. Current techniques for miRNA profiling, such as Northern blotting, 3 microarray-based hybridization, 4 and real-time quantitative polymerase chain reaction 5 are expensive and complex. A simple and rapid miRNA array would allow broad distribution of molecular diagnostic devices for cancer and chronic diseases, eventually into homes for frequent prescreening of many diseases.At their low concentrations in untreated samples, optical sensing of miRNA is most promising. Plasmonically excited Raman scattering (SERS) and fluorescence sensors from metallic nanoparticles (NPs) or surfaces have enhanced the sensitivity of optical molecular sensors by orders of magnitude. 6-9 However, probe-less SERS sensing or fluorescent sensing of unlabeled targets are insufficiently specific for miRNA targets in heterogeneous samples. Plasmonic detection is also very compatible with FRET probes whose donor dye offers small light sources to excite fluorescently labelled targets upon hybridization. 7,10 A particular family of FRET reporters does offer label-free sensing: hairpin oligo probes whose end-tagged fluorophores are quenched by the Au NP to which they are functionalized. 11 The fluorescent signal is only detected when the hairpin is broken by the hybridizing target nucleic acid or protein (for an aptamer probe), and the more rigid paired segment separates the end fluorophore from the quenching surface to produce a fluorescent signal. It is often hoped that plasmonics on the metal surface will enhance the intensity to overcome the quenching effect, if the linearized hairpin is within the NP plasmonic penetration length. However, since fluorescent quenching decays slowly (linearly) with fluorophore-metal spacing 10 whereas the plasmonic intensity decays exponentially from a flat surface, careful ex...

show abstract

A rapid field-use assay for mismatch number and location of hybridized DNAs

Abstract: Molecular dielectrophoresis (DEP) is employed to rapidly ( Show more

Cited by 63 publications

References 19 publications

Floating-electrode enhanced constriction dielectrophoresis for biomolecular trapping in physiological media of high conductivity

Floating-electrode enhanced constriction dielectrophoresis for biomolecular trapping in physiological media of high conductivity

Selective dynamic concentration of peptides at poles of cation-selective nanoporous granules

Plasmonic hotspots of dynamically assembled nanoparticles in nanocapillaries: Towards a micro ribonucleic acid profiling platform

Contact Info

Product

Resources

About