Detection of Single Nucleotide Polymorphisms in p53 Mutation Hotspots and Expression of Mutant p53 in Human Cell Lines Using an Enzyme‐Linked Electrochemical Assay

Horáková, Petra; Šimková, Eva; Vychodilová, Zdenka; Brázdová, Marie; Fojta, Miroslav

doi:10.1002/elan.200904656

Cited by 20 publications

(23 citation statements)

References 16 publications

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“…Application of PCR to pre-amplify specific DNA fragments for the methylation analysis (as is routinely used e.g., in the case of single nucleotide polymorphisms typing [98,99]) is not possible because during the amplification reaction, the DNA methylation pattern is lost. Thus, to catch the methylation at the DNA sequence level, it seems to be necessary to modify with osmium directly the genomic DNA isolated from the biological material.…”

Section: Probing Of 5-methylcytosine With Oslmentioning

confidence: 99%

Osmium Tetroxide Complexes as Versatile Tools for Structure Probing and Electrochemical Analysis of Biopolymers

Fojta¹,

Kostečka²,

Pivoňková³

et al. 2011

CAC

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Osmium tetroxide complexes with nitrogenous ligands and analogous complexes of six-valent osmium proved excellent tools for selective labeling of biopolymers (nucleic acids, proteins and polysaccharides). Reactions of these species with target moieties within the biopolymer molecules (pyrimidine nucleobases, tryptophan residues or sugar moieties) are facile at physiological conditions and are in general structure-selective, allowing their application in DNA and protein structure probing. The modification products can be detected by a variety of widely accessible analytical techniques, including biochemical (enzymatic) approaches, immunoassays, chemical DNA sequencing, spectrophotometry and electrochemistry. Particularly the electrochemical techniques are promising for utilization in biosensors and routine bioassays due to the possibility of highly sensitive and selective detection of the labeled biopolymers adducts based on distinct electrochemical properties of the introduced osmium moieties. Utilization of the osmium tags in probing DNA structural transitions, sensing of DNA hybridization, damage and DNA methylation, labeling of peptides and proteins, probing accessibility of tryptophan residues in proteins and their complexes, and labeling of sugar moieties, are reviewed.

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Section: Probing Of 5-methylcytosine With Oslmentioning

confidence: 99%

Osmium Tetroxide Complexes as Versatile Tools for Structure Probing and Electrochemical Analysis of Biopolymers

Fojta¹,

Kostečka²,

Pivoňková³

et al. 2011

CAC

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“…The PeGEs have been successfully applied in various modes of DNA sensing, using either label‐free detection (usually via electrooxidation signal of guanine, e. g. ) or employing enzyme‐linked techniques involving bioaffinity labeling . The latter techniques have utilized also other types of graphite‐based electrodes and some of them involved application of magnetic beads, using the “double‐surface” approach . Their applications included, for example, determination of lengths of repetitive DNA sequences , detection of point mutations , or simply monitoring of PCR amplification of specific DNA fragments .…”

Section: Resultsmentioning

confidence: 99%

“…The latter techniques have utilized also other types of graphite‐based electrodes and some of them involved application of magnetic beads, using the “double‐surface” approach . Their applications included, for example, determination of lengths of repetitive DNA sequences , detection of point mutations , or simply monitoring of PCR amplification of specific DNA fragments . The approach presented here involves application of bare (and used‐as‐received) PeGE and does not involve magnetic beads, which is inherently positively reflected in cost effectivity of the electroanalytical part.…”

Section: Resultsmentioning

confidence: 99%

“…Labeling of different probes by two different enzymes which convert their specific substrates to electrochemicaly well distinguishable, simultaneously detectable products was also described . Incorporation of biotinylated nucleotides by DNA polymerases was utilized for SNP typing or detection of PCR amplicons indicating presence of target sequence for annealing primers in a template DNA .…”

Section: Introductionmentioning

confidence: 99%

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Electrochemical Detection of SNP in Human Mitochondrial DNA Using Cyclic Primer Extension with Biotinylated Nucletides and Enzymatic Labeling at Disposable Pencil Graphite Electrodes

et al. 2018

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A novel method of SNP typing in human mitochondrial DNA utilizing enzymatic labeling and electrochemical detection at disposable pencil graphite electrodes is described. The procedure is based on amplification of DNA stretches by cyclic primer extension (PEx) of SNP‐specific diagnostic primers in a mixture of biotinylated and natural nucleotides. The diagnostic primers are designed to recognize, by its 3'‐terminal nucleotide, the SNP‐site in target template. Under optimized conditions of the PEx reaction, efficient polymerase synthesis of biotin‐labeled strands takes place only in the case of full complementarity between the diagnostic primer and the target SNP site. There is also benefit from introducing many biotin molecules per extended DNA strand, resulting in another level of signal amplification. After adsorption of biotinylated PEx products at the electrode surface, streptavidin‐alkaline phosphatase conjugate was bound to the biotin tags, 1‐naphthol was enzymatically produced and electrochemically detected. Several critical steps and parameters of the assay, including termination of 3’‐OH ends of residual amplification primers, temperature for annealing of diagnostic primers, relative amount of biotinylated deoxynucleoside triphosphate in the PEx mixture and number of PEx cycles were optimized in this study to attain best SNP resolution, and reduction of time needed for the analysis.

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“…The same group proposed the detection of nucleotide polymorphisms in p53 mutation hotspots and expression of mutant p53 in human cell lines [77]. Combining the double-surface technique [70] with RT-PCR and PEX [76], they were able to detect single-nucleotide polymorphism in samples received from cell cultures, differentiating mutant and wild-type genotypes where mutant genotypes indicate the inability of p53 to act as a tumor suppressor.…”

Section: Real Samplesmentioning

confidence: 98%

Sequence-specific electrochemical detection of nucleic acids in real samples

Duwensee¹,

Mix

Flechsig

2010

Bioanal Rev

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This paper reviews past and current developments in the field of electrochemical biosensors with a focus on the sequence-specific detection of nucleic acids in real samples. After electrochemical hybridization sensors had been first described in 1993, it took nearly a decade until some of the many proposed protocols were indeed applied to real samples like blood or tissue. Electrochemical transduction schemes used either rely on electroactive moieties such as intercalators, groove binders, covalently attached labels, and products of enzyme markers or they are completely indicator free like impedance-based detection principles. Most detection schemes require a polymerase chain reaction amplification step to allow for sufficient selectivity and sensitivity. Today, several companies develop electrochemical microarrays able to detect dozens to many thousands of sequences in a single experiment.

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Detection of Single Nucleotide Polymorphisms in p53 Mutation Hotspots and Expression of Mutant p53 in Human Cell Lines Using an Enzyme‐Linked Electrochemical Assay

Cited by 20 publications

References 16 publications

Osmium Tetroxide Complexes as Versatile Tools for Structure Probing and Electrochemical Analysis of Biopolymers

Osmium Tetroxide Complexes as Versatile Tools for Structure Probing and Electrochemical Analysis of Biopolymers

Electrochemical Detection of SNP in Human Mitochondrial DNA Using Cyclic Primer Extension with Biotinylated Nucletides and Enzymatic Labeling at Disposable Pencil Graphite Electrodes

Sequence-specific electrochemical detection of nucleic acids in real samples

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