Kinetic and affinity analyses of hybridization reactions between peptide nucleic acid probes and DNA targets using surface plasmon field-enhanced fluorescence spectroscopy

Abstract: Peptide nucleic acid (PNA), a polyamide DNA mimic, has inspired the development of a variety of hybridization-based methods for the detection, quantification, purification, and characterization of nucleic acids owing to the stability of the PNA/DNA duplex. In this work, PNA probes complementary to a specific sequence of Roundup Ready® soybean were immobilized onto a sensor surface via a self-assembled matrix employing streptavidin/biotin binding. The specific hybridization of PNA and DNA has been monitored by … Show more

“…Moreover, the transistor sensor sensitivity was investigated by conducting the control experiments with and with out target DNA injection down to a 1 nM concentration (Figure 2d). This remarkable sensitivity is similar to the sensitivity previously reported using fluorescence based sensors 25…”

“…Amine terminated PNA‐15mers (P2–15mers) were attached to the pMA layer (Scheme 1c), which were used as the selective probe to target DNA. PNA (P2–15mer) probes have been shown to be effective in discriminating between single base differences in applications using short sequences 25, 26. In the presence of an aqueous buffer, the anhydride groups on the polymer surface are hydrolyzed and converted to carboxylic acids, which were activated by circulating a solution containing 0.2 M N ‐ethyl‐ N′ ‐(3‐dimethylaminopropyl)‐carbodiimide hydrochloride (EDC) and 0.05 M N ‐hydroxysuccinimide (NHS) in the flow cell at a constant rate of 300 μL/min for 20 min.…”

“…This effect is also prevalent in the SPFS measurements, but to a lower extent since no gate bias is present. Operating in high ionic strength buffer solutions or diluting the probe density of the sensor matrix could limit the influence of Coulombic repulsion on the hybridization kinetics;25 however, both of these conditions would adversely affect the sensor sensitivity. Moreover, the transistor sensor sensitivity was investigated by conducting the control experiments with and with out target DNA injection down to a 1 nM concentration (Figure 2d).…”

In Situ, Label‐Free DNA Detection Using Organic Transistor Sensors

“…Moreover, the transistor sensor sensitivity was investigated by conducting the control experiments with and with out target DNA injection down to a 1 nM concentration (Figure 2d). This remarkable sensitivity is similar to the sensitivity previously reported using fluorescence based sensors 25…”

“…Amine terminated PNA‐15mers (P2–15mers) were attached to the pMA layer (Scheme 1c), which were used as the selective probe to target DNA. PNA (P2–15mer) probes have been shown to be effective in discriminating between single base differences in applications using short sequences 25, 26. In the presence of an aqueous buffer, the anhydride groups on the polymer surface are hydrolyzed and converted to carboxylic acids, which were activated by circulating a solution containing 0.2 M N ‐ethyl‐ N′ ‐(3‐dimethylaminopropyl)‐carbodiimide hydrochloride (EDC) and 0.05 M N ‐hydroxysuccinimide (NHS) in the flow cell at a constant rate of 300 μL/min for 20 min.…”

“…This effect is also prevalent in the SPFS measurements, but to a lower extent since no gate bias is present. Operating in high ionic strength buffer solutions or diluting the probe density of the sensor matrix could limit the influence of Coulombic repulsion on the hybridization kinetics;25 however, both of these conditions would adversely affect the sensor sensitivity. Moreover, the transistor sensor sensitivity was investigated by conducting the control experiments with and with out target DNA injection down to a 1 nM concentration (Figure 2d).…”

In Situ, Label‐Free DNA Detection Using Organic Transistor Sensors

“…[12,13]. These values are also close to the results obtained by SPFS for an interfacial architecture in which the capture probe layer was surface attached via a biotin-moiety attaching the probe sequence to a straptavidin matrix [14].…”

“…As a consequence, the affinity constants K A =k on /k off decreased by two orders of magnitude in going from a fully matched to a singly mismatched target sequence. This has been seen before with other interfacial architectures, e.g., based on biotinylated probe strands surface-immobilzed via a straptavidin matrix [12]. Within the Langmuir adsorption model, these affinity constants and the resulting K d values can then be compared with those obtained by titration experiments.…”

A Review on Security Issues in Wireless Sensor Network

Biofunctional Surfaces