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Low density DNA microarray for detection of most frequent TP53 missense point mutations

BACKGROUND: We have developed an oligonucleotide microarray (genosensor) utilizing a double tandem hybridization technique to search for 9 point mutations located in the most frequently altered codons of the TP53 gene. Isolated and multiplexed PCR products, 108 and 92 bp long, from exons 7 and 8, re...

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Autores principales: Rangel-López, Angélica, Maldonado-Rodríguez, Rogelio, Salcedo-Vargas, Mauricio, Espinosa-Lara, Juana Mercedes, Méndez-Tenorio, Alfonso, Beattie, Kenneth L
Formato: Texto
Lenguaje:English
Publicado: BioMed Central 2005
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC553977/
https://www.ncbi.nlm.nih.gov/pubmed/15713227
http://dx.doi.org/10.1186/1472-6750-5-8
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author Rangel-López, Angélica
Maldonado-Rodríguez, Rogelio
Salcedo-Vargas, Mauricio
Espinosa-Lara, Juana Mercedes
Méndez-Tenorio, Alfonso
Beattie, Kenneth L
author_facet Rangel-López, Angélica
Maldonado-Rodríguez, Rogelio
Salcedo-Vargas, Mauricio
Espinosa-Lara, Juana Mercedes
Méndez-Tenorio, Alfonso
Beattie, Kenneth L
author_sort Rangel-López, Angélica
collection PubMed
description BACKGROUND: We have developed an oligonucleotide microarray (genosensor) utilizing a double tandem hybridization technique to search for 9 point mutations located in the most frequently altered codons of the TP53 gene. Isolated and multiplexed PCR products, 108 and 92 bp long, from exons 7 and 8, respectively, were obtained from 24 different samples. Single-stranded target DNA was then prepared from isolated or multiplexed PCR products, through cyclic DNA synthesis. Independent ssDNA's were annealed with the corresponding pairs of labeled stacking oligonucleotides to create partially duplex DNA having a 7-nt gap, which contains the sequence that will be interrogated by the capture probes forming double tandem hybridization. In the case of multiplexed ssPCR products, only two stacking oligonucleotides were added per target, therefore the gap for the PCR products having two consecutive codons to be interrogated in exon 7 was 12 nt long, so only single tandem hybridization was produced with these respective probes. RESULTS: 18 codon substitutions were found by DNA sequencing. In 13 of them a perfect correlation with the pattern of hybridization was seen (In 5 no signal was seen with the wt probe while a new signal was seen with the appropriate mutant probe, and in 8 more, as expected, no signal was seen with any probe due to the absence of the corresponding probe in the array). In 3 other cases a mutation was falsely suggested by the combination of the absence of the wild type signal along with a false signal in the other probe. In the other 2 cases the presence of the mutation was not detected due to the production of a false hybridization signal with the wild type probe. In both cases (false mutation or no mutation detected) relatively stable mismatched target/probe duplexes should be formed. These problems could be avoided by the addition of probes to improve the performance of the array. CONCLUSION: Our results demonstrate that a simple TP53 microarray employing short (7-mer) probes, used in combination with single or double tandem hybridization approach and a simple or multiplex target preparation method, can identify common TP53 missense mutations from a variety of DNA sources with good specificity.
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spelling pubmed-5539772005-03-11 Low density DNA microarray for detection of most frequent TP53 missense point mutations Rangel-López, Angélica Maldonado-Rodríguez, Rogelio Salcedo-Vargas, Mauricio Espinosa-Lara, Juana Mercedes Méndez-Tenorio, Alfonso Beattie, Kenneth L BMC Biotechnol Methodology Article BACKGROUND: We have developed an oligonucleotide microarray (genosensor) utilizing a double tandem hybridization technique to search for 9 point mutations located in the most frequently altered codons of the TP53 gene. Isolated and multiplexed PCR products, 108 and 92 bp long, from exons 7 and 8, respectively, were obtained from 24 different samples. Single-stranded target DNA was then prepared from isolated or multiplexed PCR products, through cyclic DNA synthesis. Independent ssDNA's were annealed with the corresponding pairs of labeled stacking oligonucleotides to create partially duplex DNA having a 7-nt gap, which contains the sequence that will be interrogated by the capture probes forming double tandem hybridization. In the case of multiplexed ssPCR products, only two stacking oligonucleotides were added per target, therefore the gap for the PCR products having two consecutive codons to be interrogated in exon 7 was 12 nt long, so only single tandem hybridization was produced with these respective probes. RESULTS: 18 codon substitutions were found by DNA sequencing. In 13 of them a perfect correlation with the pattern of hybridization was seen (In 5 no signal was seen with the wt probe while a new signal was seen with the appropriate mutant probe, and in 8 more, as expected, no signal was seen with any probe due to the absence of the corresponding probe in the array). In 3 other cases a mutation was falsely suggested by the combination of the absence of the wild type signal along with a false signal in the other probe. In the other 2 cases the presence of the mutation was not detected due to the production of a false hybridization signal with the wild type probe. In both cases (false mutation or no mutation detected) relatively stable mismatched target/probe duplexes should be formed. These problems could be avoided by the addition of probes to improve the performance of the array. CONCLUSION: Our results demonstrate that a simple TP53 microarray employing short (7-mer) probes, used in combination with single or double tandem hybridization approach and a simple or multiplex target preparation method, can identify common TP53 missense mutations from a variety of DNA sources with good specificity. BioMed Central 2005-02-15 /pmc/articles/PMC553977/ /pubmed/15713227 http://dx.doi.org/10.1186/1472-6750-5-8 Text en Copyright © 2005 Rangel-López et al; licensee BioMed Central Ltd.
spellingShingle Methodology Article
Rangel-López, Angélica
Maldonado-Rodríguez, Rogelio
Salcedo-Vargas, Mauricio
Espinosa-Lara, Juana Mercedes
Méndez-Tenorio, Alfonso
Beattie, Kenneth L
Low density DNA microarray for detection of most frequent TP53 missense point mutations
title Low density DNA microarray for detection of most frequent TP53 missense point mutations
title_full Low density DNA microarray for detection of most frequent TP53 missense point mutations
title_fullStr Low density DNA microarray for detection of most frequent TP53 missense point mutations
title_full_unstemmed Low density DNA microarray for detection of most frequent TP53 missense point mutations
title_short Low density DNA microarray for detection of most frequent TP53 missense point mutations
title_sort low density dna microarray for detection of most frequent tp53 missense point mutations
topic Methodology Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC553977/
https://www.ncbi.nlm.nih.gov/pubmed/15713227
http://dx.doi.org/10.1186/1472-6750-5-8
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