Fast and reliable screening of mutations in human tumors

Detalhes bibliográficos
Autor(a) principal: Marcelino, Luisa A.
Data de Publicação: 1999
Outros Autores: Galvin, M., Martins, G. M., Proença, M. J., Mayrand, E., Rueff, J. A., Monteiro, C. J.
Tipo de documento: Artigo
Idioma: eng
Título da fonte: Repositório Científico de Acesso Aberto de Portugal (Repositórios Cientìficos)
Texto Completo: https://doi.org/10.2144/99266rr01
Resumo: Human tumor samples were screened for point mutations by adapting a mobility-shift assay to automated DNA sizing. This screen identifies the type of point mutation and relative amount of mutated DNA sequences present in a sample. Test samples having known hypoxanthine-guanine phosphoribosyl transferase (hprt)/exon-3 sequence mutations were characterized by: (i) PCR amplification, (ii) fluorescent dye-primer extension with 36-atom linker derived deoxycytosine or deoxyuridine triphosphate and the remaining three natural nucleotides and (iii) sizing of the resulting fluorescently labeled modified strands, using an automated DNA sequencer. Routinely, a range of sizes is observed among the sequence variants of a single DNA target sequence. This is because nucleotide analogs are incorporated into DNA strands in a sequence-dependent manner, resulting in composition-dependent electrophoretic mobility. Thus, point mutations are identified as shifts in mobility between the fluorescently labeled modified strands of the control and test samples. The twenty different hprt/exon-3 single-base substitution mutations tested were easily identified, even at fourfold dilution with control DNA.
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spelling Fast and reliable screening of mutations in human tumorsUse of multiple fluorescence-based long linker arm nucleotides assay (mf-LLA)BiotechnologyBiochemistry, Genetics and Molecular Biology(all)Human tumor samples were screened for point mutations by adapting a mobility-shift assay to automated DNA sizing. This screen identifies the type of point mutation and relative amount of mutated DNA sequences present in a sample. Test samples having known hypoxanthine-guanine phosphoribosyl transferase (hprt)/exon-3 sequence mutations were characterized by: (i) PCR amplification, (ii) fluorescent dye-primer extension with 36-atom linker derived deoxycytosine or deoxyuridine triphosphate and the remaining three natural nucleotides and (iii) sizing of the resulting fluorescently labeled modified strands, using an automated DNA sequencer. Routinely, a range of sizes is observed among the sequence variants of a single DNA target sequence. This is because nucleotide analogs are incorporated into DNA strands in a sequence-dependent manner, resulting in composition-dependent electrophoretic mobility. Thus, point mutations are identified as shifts in mobility between the fluorescently labeled modified strands of the control and test samples. The twenty different hprt/exon-3 single-base substitution mutations tested were easily identified, even at fourfold dilution with control DNA.NOVA Medical School|Faculdade de Ciências Médicas (NMS|FCM)RUNMarcelino, Luisa A.Galvin, M.Martins, G. M.Proença, M. J.Mayrand, E.Rueff, J. A.Monteiro, C. J.2019-01-08T23:32:03Z1999-06-241999-06-24T00:00:00Zinfo:eu-repo/semantics/publishedVersioninfo:eu-repo/semantics/article15application/pdfhttps://doi.org/10.2144/99266rr01eng0736-6205PURE: 11160560http://www.scopus.com/inward/record.url?scp=0033000455&partnerID=8YFLogxKhttps://doi.org/10.2144/99266rr01info:eu-repo/semantics/openAccessreponame:Repositório Científico de Acesso Aberto de Portugal (Repositórios Cientìficos)instname:Agência para a Sociedade do Conhecimento (UMIC) - FCT - Sociedade da Informaçãoinstacron:RCAAP2024-03-11T04:27:25Zoai:run.unl.pt:10362/56908Portal AgregadorONGhttps://www.rcaap.pt/oai/openaireopendoar:71602024-03-20T03:32:59.547393Repositório Científico de Acesso Aberto de Portugal (Repositórios Cientìficos) - Agência para a Sociedade do Conhecimento (UMIC) - FCT - Sociedade da Informaçãofalse
dc.title.none.fl_str_mv Fast and reliable screening of mutations in human tumors
Use of multiple fluorescence-based long linker arm nucleotides assay (mf-LLA)
title Fast and reliable screening of mutations in human tumors
spellingShingle Fast and reliable screening of mutations in human tumors
Marcelino, Luisa A.
Biotechnology
Biochemistry, Genetics and Molecular Biology(all)
title_short Fast and reliable screening of mutations in human tumors
title_full Fast and reliable screening of mutations in human tumors
title_fullStr Fast and reliable screening of mutations in human tumors
title_full_unstemmed Fast and reliable screening of mutations in human tumors
title_sort Fast and reliable screening of mutations in human tumors
author Marcelino, Luisa A.
author_facet Marcelino, Luisa A.
Galvin, M.
Martins, G. M.
Proença, M. J.
Mayrand, E.
Rueff, J. A.
Monteiro, C. J.
author_role author
author2 Galvin, M.
Martins, G. M.
Proença, M. J.
Mayrand, E.
Rueff, J. A.
Monteiro, C. J.
author2_role author
author
author
author
author
author
dc.contributor.none.fl_str_mv NOVA Medical School|Faculdade de Ciências Médicas (NMS|FCM)
RUN
dc.contributor.author.fl_str_mv Marcelino, Luisa A.
Galvin, M.
Martins, G. M.
Proença, M. J.
Mayrand, E.
Rueff, J. A.
Monteiro, C. J.
dc.subject.por.fl_str_mv Biotechnology
Biochemistry, Genetics and Molecular Biology(all)
topic Biotechnology
Biochemistry, Genetics and Molecular Biology(all)
description Human tumor samples were screened for point mutations by adapting a mobility-shift assay to automated DNA sizing. This screen identifies the type of point mutation and relative amount of mutated DNA sequences present in a sample. Test samples having known hypoxanthine-guanine phosphoribosyl transferase (hprt)/exon-3 sequence mutations were characterized by: (i) PCR amplification, (ii) fluorescent dye-primer extension with 36-atom linker derived deoxycytosine or deoxyuridine triphosphate and the remaining three natural nucleotides and (iii) sizing of the resulting fluorescently labeled modified strands, using an automated DNA sequencer. Routinely, a range of sizes is observed among the sequence variants of a single DNA target sequence. This is because nucleotide analogs are incorporated into DNA strands in a sequence-dependent manner, resulting in composition-dependent electrophoretic mobility. Thus, point mutations are identified as shifts in mobility between the fluorescently labeled modified strands of the control and test samples. The twenty different hprt/exon-3 single-base substitution mutations tested were easily identified, even at fourfold dilution with control DNA.
publishDate 1999
dc.date.none.fl_str_mv 1999-06-24
1999-06-24T00:00:00Z
2019-01-08T23:32:03Z
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url https://doi.org/10.2144/99266rr01
dc.language.iso.fl_str_mv eng
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dc.relation.none.fl_str_mv 0736-6205
PURE: 11160560
http://www.scopus.com/inward/record.url?scp=0033000455&partnerID=8YFLogxK
https://doi.org/10.2144/99266rr01
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