We show an excellent differentiation between complementary and non-complementary DNA sequences via hybridization neither of tDNA adsorbed at SPCE with biotinylated Inhibitors,Modulators,Libraries may probes, as well as highly specific detection of PCR-amplified genomic DNA fragments by means of a newly introduced PEX-based assay. In connection with a reverse transcription-PCR (RT-PCR) technique, application of the enzyme-linked electrochemical assay in gene expression monitoring is demonstrated.2.?Results and DiscussionIt has been reported previously that some types of carbon electrodes (such as carbon paste [26, 27], graphite-composite [18], pyrolytic graphite or screen-printed electrodes [13]) can be used as substrates for DNA hybridization Inhibitors,Modulators,Libraries without any special surface modifications, interfacing and/or covalent immobilization of capture probes (reviewed in [28, 29]).
Physisorbed single-stranded (ss) DNA (or Inhibitors,Modulators,Libraries peptide nucleic acid [26]) was shown to be able of forming duplex with complementary DNA strands in solution to which the ssDNA-modified electrode was exposed. Sensors based on probe or tDNA adsorption at carbon electrodes have been combined Inhibitors,Modulators,Libraries with various detection principles, including Inhibitors,Modulators,Libraries label-free detection employing intrinsic DNA electroactivity [30], application of non-covalent redox indicators (such as [Co(phen)3]3+/2+, methylene blue [27], Meldola’s blue [31] or others) or probes labeled with Inhibitors,Modulators,Libraries enzymes [13, 18].
Here we applied an enzyme-linked voltammetric Inhibitors,Modulators,Libraries technique, proposed previously Inhibitors,Modulators,Libraries for hybridization analysis of repetitive DNA sequences [13], to detect hybridization between non-repetitive, random-sequence Drug_discovery tDNAs and complementary biotinylated probes at the SPCE surface.
Figure 1A shows scheme GSK-3 of the experiment. The tDNA was adsorbed at the SPCE at open current circuit from a small (6-��l) aliquot of the sample. When the Gwent C 10903P14 ink? was used for the SPCE preparation, no pretreatment of the electrode prior to DNA adsorption was necessary to obtain well defined and reasonably reproducible responses. After adsorption of the tDNA, the unoccupied electrode surface was blocked by bovine serum albumin, followed by subsequent application of the biotinylated probe solution and the SALP conjugate solution.
Blocking of the electrode prior to the hybridization step was critical for specificity of the sensor responses: when it was omitted or performed after incubation with the biotinylated probe, false positive responses selleckbio were obtained due to unspecific adsorption of the probe at the electrode surface [13].
Finally, the electrode was dipped into solution of the substrate (1-naphthyl phosphate) in background electrolyte, and after a short incubation time during which the substrate was enzymatically converted into the electroactive indicator (1-naphthol), signal of the latter was measured using linear sweep voltammetry www.selleckchem.com/products/Perifosine.html (LSV).