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Detection and mapping of mtDNA SNPs in Atlantic salmon using high throughput DNA sequencing

BACKGROUND: Approximately half of the mitochondrial genome inherent within 546 individual Atlantic salmon (Salmo salar) derived from across the species' North Atlantic range, was selectively amplified with a novel combination of standard PCR and pyro-sequencing in a single run using 454 Titaniu...

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Autores principales: Fridjonsson, Olafur, Olafsson, Kristinn, Tompsett, Scott, Bjornsdottir, Snaedis, Consuegra, Sonia, Knox, David, de Leaniz, Carlos Garcia, Magnusdottir, Steinunn, Olafsdottir, Gudbjorg, Verspoor, Eric, Hjorleifsdottir, Sigridur
Formato: Texto
Lenguaje:English
Publicado: BioMed Central 2011
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3079667/
https://www.ncbi.nlm.nih.gov/pubmed/21473771
http://dx.doi.org/10.1186/1471-2164-12-179
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author Fridjonsson, Olafur
Olafsson, Kristinn
Tompsett, Scott
Bjornsdottir, Snaedis
Consuegra, Sonia
Knox, David
de Leaniz, Carlos Garcia
Magnusdottir, Steinunn
Olafsdottir, Gudbjorg
Verspoor, Eric
Hjorleifsdottir, Sigridur
author_facet Fridjonsson, Olafur
Olafsson, Kristinn
Tompsett, Scott
Bjornsdottir, Snaedis
Consuegra, Sonia
Knox, David
de Leaniz, Carlos Garcia
Magnusdottir, Steinunn
Olafsdottir, Gudbjorg
Verspoor, Eric
Hjorleifsdottir, Sigridur
author_sort Fridjonsson, Olafur
collection PubMed
description BACKGROUND: Approximately half of the mitochondrial genome inherent within 546 individual Atlantic salmon (Salmo salar) derived from across the species' North Atlantic range, was selectively amplified with a novel combination of standard PCR and pyro-sequencing in a single run using 454 Titanium FLX technology (Roche, 454 Life Sciences). A unique combination of barcoded primers and a partitioned sequencing plate was employed to designate each sequence read to its original sample. The sequence reads were aligned according to the S. salar mitochondrial reference sequence (NC_001960.1), with the objective of identifying single nucleotide polymorphisms (SNPs). They were validated if they met with the following three stringent criteria: (i) sequence reads were produced from both DNA strands; (ii) SNPs were confirmed in a minimum of 90% of replicate sequence reads; and (iii) SNPs occurred in more than one individual. RESULTS: Pyrosequencing generated a total of 179,826,884 bp of data, and 10,765 of the total 10,920 S. salar sequences (98.6%) were assigned back to their original samples. The approach taken resulted in a total of 216 SNPs and 2 indels, which were validated and mapped onto the S. salar mitochondrial genome, including 107 SNPs and one indel not previously reported. An average of 27.3 sequence reads with a standard deviation of 11.7 supported each SNP per individual. CONCLUSION: The study generated a mitochondrial SNP panel from a large sample group across a broad geographical area, reducing the potential for ascertainment bias, which has hampered previous studies. The SNPs identified here validate those identified in previous studies, and also contribute additional potentially informative loci for the future study of phylogeography and evolution in the Atlantic salmon. The overall success experienced with this novel application of HT sequencing of targeted regions suggests that the same approach could be successfully applied for SNP mining in other species.
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spelling pubmed-30796672011-04-20 Detection and mapping of mtDNA SNPs in Atlantic salmon using high throughput DNA sequencing Fridjonsson, Olafur Olafsson, Kristinn Tompsett, Scott Bjornsdottir, Snaedis Consuegra, Sonia Knox, David de Leaniz, Carlos Garcia Magnusdottir, Steinunn Olafsdottir, Gudbjorg Verspoor, Eric Hjorleifsdottir, Sigridur BMC Genomics Methodology Article BACKGROUND: Approximately half of the mitochondrial genome inherent within 546 individual Atlantic salmon (Salmo salar) derived from across the species' North Atlantic range, was selectively amplified with a novel combination of standard PCR and pyro-sequencing in a single run using 454 Titanium FLX technology (Roche, 454 Life Sciences). A unique combination of barcoded primers and a partitioned sequencing plate was employed to designate each sequence read to its original sample. The sequence reads were aligned according to the S. salar mitochondrial reference sequence (NC_001960.1), with the objective of identifying single nucleotide polymorphisms (SNPs). They were validated if they met with the following three stringent criteria: (i) sequence reads were produced from both DNA strands; (ii) SNPs were confirmed in a minimum of 90% of replicate sequence reads; and (iii) SNPs occurred in more than one individual. RESULTS: Pyrosequencing generated a total of 179,826,884 bp of data, and 10,765 of the total 10,920 S. salar sequences (98.6%) were assigned back to their original samples. The approach taken resulted in a total of 216 SNPs and 2 indels, which were validated and mapped onto the S. salar mitochondrial genome, including 107 SNPs and one indel not previously reported. An average of 27.3 sequence reads with a standard deviation of 11.7 supported each SNP per individual. CONCLUSION: The study generated a mitochondrial SNP panel from a large sample group across a broad geographical area, reducing the potential for ascertainment bias, which has hampered previous studies. The SNPs identified here validate those identified in previous studies, and also contribute additional potentially informative loci for the future study of phylogeography and evolution in the Atlantic salmon. The overall success experienced with this novel application of HT sequencing of targeted regions suggests that the same approach could be successfully applied for SNP mining in other species. BioMed Central 2011-04-07 /pmc/articles/PMC3079667/ /pubmed/21473771 http://dx.doi.org/10.1186/1471-2164-12-179 Text en Copyright ©2011 Fridjonsson et al; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Methodology Article
Fridjonsson, Olafur
Olafsson, Kristinn
Tompsett, Scott
Bjornsdottir, Snaedis
Consuegra, Sonia
Knox, David
de Leaniz, Carlos Garcia
Magnusdottir, Steinunn
Olafsdottir, Gudbjorg
Verspoor, Eric
Hjorleifsdottir, Sigridur
Detection and mapping of mtDNA SNPs in Atlantic salmon using high throughput DNA sequencing
title Detection and mapping of mtDNA SNPs in Atlantic salmon using high throughput DNA sequencing
title_full Detection and mapping of mtDNA SNPs in Atlantic salmon using high throughput DNA sequencing
title_fullStr Detection and mapping of mtDNA SNPs in Atlantic salmon using high throughput DNA sequencing
title_full_unstemmed Detection and mapping of mtDNA SNPs in Atlantic salmon using high throughput DNA sequencing
title_short Detection and mapping of mtDNA SNPs in Atlantic salmon using high throughput DNA sequencing
title_sort detection and mapping of mtdna snps in atlantic salmon using high throughput dna sequencing
topic Methodology Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3079667/
https://www.ncbi.nlm.nih.gov/pubmed/21473771
http://dx.doi.org/10.1186/1471-2164-12-179
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