Cost-effective method to synthesize a fluorescent internal dna standard for automated fragment sizing

Detalhes bibliográficos
Autor(a) principal: Brondani, Rosana Pereira Vianello
Data de Publicação: 2001
Outros Autores: Grattapaglia, Dario
Tipo de documento: Artigo
Idioma: eng
Título da fonte: Repositório Institucional da UCB
Texto Completo: http://twingo.ucb.br:8080/jspui/handle/10869/708
https://repositorio.ucb.br:9443/jspui/handle/123456789/7890
Resumo: We describe a simple and cost-effective method for the synthesis of an internal fluorescently labeled DNA standard for fragment sizing using an automated DNA sequencer. A set of primer pairs labeled with ROX was developed to amplify 12 DNA fragments, 58–417 bp, derived from a conserved region of plant chloroplast DNA. These amplified fragments were mixed together, constituting a fluorescent internal DNA size marker. The precision of the size standard was evaluated by estimating the size of 20 alleles that were amplified at four dinucleotide microsatellite loci with the synthesized size standard and the commercial internal sizing standard, GeneScanÒ Rox- 500. A number of intra-gel and inter-gel comparisons were run, and an analysis of variance was carried out. No significant difference was observed between the size estimates obtained with the synthesized DNA standard and the commercial standard. This facile and general PCR-based method for the synthesis of internal standards allows for significant savings in the implementation of large genotyping experiments using microsatellite or AFLP markers.
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spelling Brondani, Rosana Pereira VianelloGrattapaglia, Dario2016-10-10T03:53:00Z2016-10-10T03:53:00Z2001BRONDANI, Rosana Pereira Vianello; GRATTAPAGLIA, Dario. Cost-effective method to synthesize a fluorescent internal DNA standard for automated fragment sizing. Biotechniques, v. 31, p. 802-810, 2001.http://twingo.ucb.br:8080/jspui/handle/10869/708https://repositorio.ucb.br:9443/jspui/handle/123456789/7890We describe a simple and cost-effective method for the synthesis of an internal fluorescently labeled DNA standard for fragment sizing using an automated DNA sequencer. A set of primer pairs labeled with ROX was developed to amplify 12 DNA fragments, 58–417 bp, derived from a conserved region of plant chloroplast DNA. These amplified fragments were mixed together, constituting a fluorescent internal DNA size marker. The precision of the size standard was evaluated by estimating the size of 20 alleles that were amplified at four dinucleotide microsatellite loci with the synthesized size standard and the commercial internal sizing standard, GeneScanÒ Rox- 500. A number of intra-gel and inter-gel comparisons were run, and an analysis of variance was carried out. No significant difference was observed between the size estimates obtained with the synthesized DNA standard and the commercial standard. This facile and general PCR-based method for the synthesis of internal standards allows for significant savings in the implementation of large genotyping experiments using microsatellite or AFLP markers.Made available in DSpace on 2016-10-10T03:53:00Z (GMT). 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dc.title.pt_BR.fl_str_mv Cost-effective method to synthesize a fluorescent internal dna standard for automated fragment sizing
title Cost-effective method to synthesize a fluorescent internal dna standard for automated fragment sizing
spellingShingle Cost-effective method to synthesize a fluorescent internal dna standard for automated fragment sizing
Brondani, Rosana Pereira Vianello
title_short Cost-effective method to synthesize a fluorescent internal dna standard for automated fragment sizing
title_full Cost-effective method to synthesize a fluorescent internal dna standard for automated fragment sizing
title_fullStr Cost-effective method to synthesize a fluorescent internal dna standard for automated fragment sizing
title_full_unstemmed Cost-effective method to synthesize a fluorescent internal dna standard for automated fragment sizing
title_sort Cost-effective method to synthesize a fluorescent internal dna standard for automated fragment sizing
author Brondani, Rosana Pereira Vianello
author_facet Brondani, Rosana Pereira Vianello
Grattapaglia, Dario
author_role author
author2 Grattapaglia, Dario
author2_role author
dc.contributor.author.fl_str_mv Brondani, Rosana Pereira Vianello
Grattapaglia, Dario
dc.description.abstract.por.fl_txt_mv We describe a simple and cost-effective method for the synthesis of an internal fluorescently labeled DNA standard for fragment sizing using an automated DNA sequencer. A set of primer pairs labeled with ROX was developed to amplify 12 DNA fragments, 58–417 bp, derived from a conserved region of plant chloroplast DNA. These amplified fragments were mixed together, constituting a fluorescent internal DNA size marker. The precision of the size standard was evaluated by estimating the size of 20 alleles that were amplified at four dinucleotide microsatellite loci with the synthesized size standard and the commercial internal sizing standard, GeneScanÒ Rox- 500. A number of intra-gel and inter-gel comparisons were run, and an analysis of variance was carried out. No significant difference was observed between the size estimates obtained with the synthesized DNA standard and the commercial standard. This facile and general PCR-based method for the synthesis of internal standards allows for significant savings in the implementation of large genotyping experiments using microsatellite or AFLP markers.
dc.description.version.pt_BR.fl_txt_mv Sim
dc.description.status.pt_BR.fl_txt_mv Publicado
description We describe a simple and cost-effective method for the synthesis of an internal fluorescently labeled DNA standard for fragment sizing using an automated DNA sequencer. A set of primer pairs labeled with ROX was developed to amplify 12 DNA fragments, 58–417 bp, derived from a conserved region of plant chloroplast DNA. These amplified fragments were mixed together, constituting a fluorescent internal DNA size marker. The precision of the size standard was evaluated by estimating the size of 20 alleles that were amplified at four dinucleotide microsatellite loci with the synthesized size standard and the commercial internal sizing standard, GeneScanÒ Rox- 500. A number of intra-gel and inter-gel comparisons were run, and an analysis of variance was carried out. No significant difference was observed between the size estimates obtained with the synthesized DNA standard and the commercial standard. This facile and general PCR-based method for the synthesis of internal standards allows for significant savings in the implementation of large genotyping experiments using microsatellite or AFLP markers.
publishDate 2001
dc.date.issued.fl_str_mv 2001
dc.date.accessioned.fl_str_mv 2016-10-10T03:53:00Z
dc.date.available.fl_str_mv 2016-10-10T03:53:00Z
dc.type.status.fl_str_mv info:eu-repo/semantics/publishedVersion
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dc.identifier.citation.fl_str_mv BRONDANI, Rosana Pereira Vianello; GRATTAPAGLIA, Dario. Cost-effective method to synthesize a fluorescent internal DNA standard for automated fragment sizing. Biotechniques, v. 31, p. 802-810, 2001.
dc.identifier.uri.fl_str_mv http://twingo.ucb.br:8080/jspui/handle/10869/708
https://repositorio.ucb.br:9443/jspui/handle/123456789/7890
identifier_str_mv BRONDANI, Rosana Pereira Vianello; GRATTAPAGLIA, Dario. Cost-effective method to synthesize a fluorescent internal DNA standard for automated fragment sizing. Biotechniques, v. 31, p. 802-810, 2001.
url http://twingo.ucb.br:8080/jspui/handle/10869/708
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