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Randomly Amplified DNA Fingerprinting: A Culmination of DNA Marker Technologies Based on Arbitrarily-Primed PCR Amplification

Arbitrarily-primed DNA markers can be very useful for genetic fingerprinting and for facilitating positional cloning of genes. This class of technologies is particularly important for less studied species, for which genome sequence information is generally not known. The technologies include Randoml...

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Autores principales: Waldron, Julie, Peace, Cameron P., Searle, Iain R., Furtado, Agnelo, Wade, Nick, Findlay, Ian, Graham, Michael W., Carroll, Bernard J.
Formato: Texto
Lenguaje:English
Publicado: 2002
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC161367/
https://www.ncbi.nlm.nih.gov/pubmed/12488579
http://dx.doi.org/10.1155/S1110724302206026
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author Waldron, Julie
Peace, Cameron P.
Searle, Iain R.
Furtado, Agnelo
Wade, Nick
Findlay, Ian
Graham, Michael W.
Carroll, Bernard J.
author_facet Waldron, Julie
Peace, Cameron P.
Searle, Iain R.
Furtado, Agnelo
Wade, Nick
Findlay, Ian
Graham, Michael W.
Carroll, Bernard J.
author_sort Waldron, Julie
collection PubMed
description Arbitrarily-primed DNA markers can be very useful for genetic fingerprinting and for facilitating positional cloning of genes. This class of technologies is particularly important for less studied species, for which genome sequence information is generally not known. The technologies include Randomly Amplified Polymorphic DNA (RAPD), DNA Amplification Fingerprinting (DAF), and Amplified Fragment Length Polymorphism (AFLP). We have modified the DAF protocol to produce a robust PCR-based DNA marker technology called Randomly Amplified DNA Fingerprinting (RAF). While the protocol most closely resembles DAF, it is much more robust and sensitive because amplicons are labelled with either radioactive (33)P or fluorescence in a 30-cycle PCR, and then separated and detected on large polyacrylamide sequencing gels. Highly reproducible RAF markers were readily amplified from either purified DNA or alkali-treated intact leaf tissue. RAF markers typically display dominant inheritance. However, a small but significant portion of the RAF markers exhibit codominant inheritance and represent microsatellite loci. RAF compares favorably with AFLP for efficiency and reliability on many plant genomes, including the very large and complex genomes of sugarcane and wheat. While the two technologies detect about the same number of markers per large polyacrylamide gel, advantages of RAF over AFLP include: (i) no requirement for enzymatic template preparation, (ii) one instead of two PCRs, and (iii) overall cost. RAF and AFLP were shown to differ in the selective basis of amplification of markers from genomes and could therefore be used in complementary fashion for some genetic studies.
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spelling pubmed-1613672003-07-01 Randomly Amplified DNA Fingerprinting: A Culmination of DNA Marker Technologies Based on Arbitrarily-Primed PCR Amplification Waldron, Julie Peace, Cameron P. Searle, Iain R. Furtado, Agnelo Wade, Nick Findlay, Ian Graham, Michael W. Carroll, Bernard J. J Biomed Biotechnol Research Article Arbitrarily-primed DNA markers can be very useful for genetic fingerprinting and for facilitating positional cloning of genes. This class of technologies is particularly important for less studied species, for which genome sequence information is generally not known. The technologies include Randomly Amplified Polymorphic DNA (RAPD), DNA Amplification Fingerprinting (DAF), and Amplified Fragment Length Polymorphism (AFLP). We have modified the DAF protocol to produce a robust PCR-based DNA marker technology called Randomly Amplified DNA Fingerprinting (RAF). While the protocol most closely resembles DAF, it is much more robust and sensitive because amplicons are labelled with either radioactive (33)P or fluorescence in a 30-cycle PCR, and then separated and detected on large polyacrylamide sequencing gels. Highly reproducible RAF markers were readily amplified from either purified DNA or alkali-treated intact leaf tissue. RAF markers typically display dominant inheritance. However, a small but significant portion of the RAF markers exhibit codominant inheritance and represent microsatellite loci. RAF compares favorably with AFLP for efficiency and reliability on many plant genomes, including the very large and complex genomes of sugarcane and wheat. While the two technologies detect about the same number of markers per large polyacrylamide gel, advantages of RAF over AFLP include: (i) no requirement for enzymatic template preparation, (ii) one instead of two PCRs, and (iii) overall cost. RAF and AFLP were shown to differ in the selective basis of amplification of markers from genomes and could therefore be used in complementary fashion for some genetic studies. 2002 /pmc/articles/PMC161367/ /pubmed/12488579 http://dx.doi.org/10.1155/S1110724302206026 Text en Copyright © 2002, Hindawi Publishing Corporation
spellingShingle Research Article
Waldron, Julie
Peace, Cameron P.
Searle, Iain R.
Furtado, Agnelo
Wade, Nick
Findlay, Ian
Graham, Michael W.
Carroll, Bernard J.
Randomly Amplified DNA Fingerprinting: A Culmination of DNA Marker Technologies Based on Arbitrarily-Primed PCR Amplification
title Randomly Amplified DNA Fingerprinting: A Culmination of DNA Marker Technologies Based on Arbitrarily-Primed PCR Amplification
title_full Randomly Amplified DNA Fingerprinting: A Culmination of DNA Marker Technologies Based on Arbitrarily-Primed PCR Amplification
title_fullStr Randomly Amplified DNA Fingerprinting: A Culmination of DNA Marker Technologies Based on Arbitrarily-Primed PCR Amplification
title_full_unstemmed Randomly Amplified DNA Fingerprinting: A Culmination of DNA Marker Technologies Based on Arbitrarily-Primed PCR Amplification
title_short Randomly Amplified DNA Fingerprinting: A Culmination of DNA Marker Technologies Based on Arbitrarily-Primed PCR Amplification
title_sort randomly amplified dna fingerprinting: a culmination of dna marker technologies based on arbitrarily-primed pcr amplification
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC161367/
https://www.ncbi.nlm.nih.gov/pubmed/12488579
http://dx.doi.org/10.1155/S1110724302206026
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