Use of PCR-PIRA for screening of a point mutation at codon 12 in K-ras oncogene obtained from paraffin embedded tissue sections.

Use of PCR-PIRA for screening of a point mutation at codon 12 in K-ras oncogene obtained from paraffin embedded tissue sections.

Among various methods which have been developed for facilitating the screening of point mutations in human genomic DNA, PCR-Primer Introduced Restriction Analysis (PCR-PIRA) is of particular interest due to its practicality and short procedure allowing detection of point mutations by simple restrict...

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Main Authors: N. Chewawiwat, V. Lulitanond, K. Nimmanahaeminda, K. Thamprasert, D. Nicomrat, M. Ponglikitmongkol
Other Authors: Mahidol University
Format: Article
Published: 2018
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Medicine
Online Access:https://repository.li.mahidol.ac.th/handle/123456789/17346
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spelling th-mahidol.173462018-07-04T13:55:50Z Use of PCR-PIRA for screening of a point mutation at codon 12 in K-ras oncogene obtained from paraffin embedded tissue sections. N. Chewawiwat V. Lulitanond K. Nimmanahaeminda K. Thamprasert D. Nicomrat M. Ponglikitmongkol Mahidol University Medicine Among various methods which have been developed for facilitating the screening of point mutations in human genomic DNA, PCR-Primer Introduced Restriction Analysis (PCR-PIRA) is of particular interest due to its practicality and short procedure allowing detection of point mutations by simple restriction enzyme digestion directly after PCR amplification. However, one limitation of PCR-PIRA method is the absence of restriction sites in the region of detection, thus creation of the recognition site in primers has been introduced. Detection of a point mutation at codon 12 in K-ras oncogene by BstNI requires one base change in the primer sequence so that only the normal but not mutant PCR product will be digested by the enzyme. However, false positive results generated from undigested normal DNA sequence are always obtained. This effect is compounded when it is used to analyse mixed cell populations in paraffin embedded section of cancer cells. Assay of a mutant band generated from normal DNA by densitometric quantitation enabled the determination of background values and thereby eliminated false positive results. Samples with higher ratios between mutant and normal bands than the background one after the first PCR-PIRA would be subjected to the second PCR-PIRA in order to confirm the results. Screening of such mutations in cervical carcinomas from paraffin embedded sections using the above criteria should reduce misinterpretation of PCR-PIRA results. 2018-07-04T06:55:50Z 2018-07-04T06:55:50Z 1995-12-01 Article The Southeast Asian journal of tropical medicine and public health. Vol.26 Suppl 1, (1995), 329-332 01251562 2-s2.0-0029442361 https://repository.li.mahidol.ac.th/handle/123456789/17346 Mahidol University SCOPUS https://www.scopus.com/inward/record.uri?partnerID=HzOxMe3b&scp=0029442361&origin=inward
institution Mahidol University
building Mahidol University Library
continent Asia
country Thailand
Thailand
content_provider Mahidol University Library
collection Mahidol University Institutional Repository
topic Medicine
spellingShingle Medicine
N. Chewawiwat
V. Lulitanond
K. Nimmanahaeminda
K. Thamprasert
D. Nicomrat
M. Ponglikitmongkol
Use of PCR-PIRA for screening of a point mutation at codon 12 in K-ras oncogene obtained from paraffin embedded tissue sections.
description Among various methods which have been developed for facilitating the screening of point mutations in human genomic DNA, PCR-Primer Introduced Restriction Analysis (PCR-PIRA) is of particular interest due to its practicality and short procedure allowing detection of point mutations by simple restriction enzyme digestion directly after PCR amplification. However, one limitation of PCR-PIRA method is the absence of restriction sites in the region of detection, thus creation of the recognition site in primers has been introduced. Detection of a point mutation at codon 12 in K-ras oncogene by BstNI requires one base change in the primer sequence so that only the normal but not mutant PCR product will be digested by the enzyme. However, false positive results generated from undigested normal DNA sequence are always obtained. This effect is compounded when it is used to analyse mixed cell populations in paraffin embedded section of cancer cells. Assay of a mutant band generated from normal DNA by densitometric quantitation enabled the determination of background values and thereby eliminated false positive results. Samples with higher ratios between mutant and normal bands than the background one after the first PCR-PIRA would be subjected to the second PCR-PIRA in order to confirm the results. Screening of such mutations in cervical carcinomas from paraffin embedded sections using the above criteria should reduce misinterpretation of PCR-PIRA results.
author2 Mahidol University
author_facet Mahidol University
N. Chewawiwat
V. Lulitanond
K. Nimmanahaeminda
K. Thamprasert
D. Nicomrat
M. Ponglikitmongkol
format Article
author N. Chewawiwat
V. Lulitanond
K. Nimmanahaeminda
K. Thamprasert
D. Nicomrat
M. Ponglikitmongkol
author_sort N. Chewawiwat
title Use of PCR-PIRA for screening of a point mutation at codon 12 in K-ras oncogene obtained from paraffin embedded tissue sections.
title_short Use of PCR-PIRA for screening of a point mutation at codon 12 in K-ras oncogene obtained from paraffin embedded tissue sections.
title_full Use of PCR-PIRA for screening of a point mutation at codon 12 in K-ras oncogene obtained from paraffin embedded tissue sections.
title_fullStr Use of PCR-PIRA for screening of a point mutation at codon 12 in K-ras oncogene obtained from paraffin embedded tissue sections.
title_full_unstemmed Use of PCR-PIRA for screening of a point mutation at codon 12 in K-ras oncogene obtained from paraffin embedded tissue sections.
title_sort use of pcr-pira for screening of a point mutation at codon 12 in k-ras oncogene obtained from paraffin embedded tissue sections.
publishDate 2018
url https://repository.li.mahidol.ac.th/handle/123456789/17346
_version_ 1763497987024093184

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